Title of Invention	DETECTION OF GLUCOSE IN SOLUTIONS ALSO CONTAINING AN ALPHA-HYDROXY ACID OR A BETADIKETONE
Abstract	Compositions and methods for determining the presence or concentration of glucose in a sample which may also contain an alpha-hydroxy acid or a beta-diketone.The method uses a compound having at least two recognition elements for glucose, oriented such that the interaction between the compound and glucose is more stable than the interaction between the compound and the alpha-hydroxy acid or beta-diketone, such that the presence of the alpha-hydroxy acid or the beta-diketone does not substantially interfere with said determination.

Title of Invention

DETECTION OF GLUCOSE IN SOLUTIONS ALSO CONTAINING AN ALPHA-HYDROXY ACID OR A BETADIKETONE

Abstract

Compositions and methods for determining the presence or concentration of glucose in a sample which may also contain an alpha-hydroxy acid or a beta-diketone.The method uses a compound having at least two recognition elements for glucose, oriented such that the interaction between the compound and glucose is more stable than the interaction between the compound and the alpha-hydroxy acid or beta-diketone, such that the presence of the alpha-hydroxy acid or the beta-diketone does not substantially interfere with said determination.

Full Text	TITLE CF THE INVENTION DETECTION OF GLUCOSE IN SOLUTIONS ALSO CONTAINING AN ALPHA-HYDROXY ACID OR A BETA-DIKETONE CROSS-REFERENCE TO RELATED APPLICATIONS The present application is a continuation-in-part of application Serial No. ]0/029,184 filed December 28, 2001, which is a contimation-in-part of application Serial No. 09/754,217 filed January 5, 2001 and claims the benefit of application Serial No. 60/363,885 filed March 14, 2002, application Serial No. 60/329,746 filed October 18, 2001 and application Serial No. 60/269,887 filed February 21, 2001. STATEMENT REGARDING FEDERALLY SPONSORED RESEARCH OR DEVELOPMENT Not applicable. BACKGROUND D OF THE INVENTION 1. Field of the Invention The present invention relates to the detection of glucose in samples which ray also contain potential interfering compounds, Such as α-hydroxy acids or (3- diketones. 2. Description of the Related Art The complexation of carbohydrates, including glucose, with phenylboronic acid las been known for a long time and the reversibility of that interaction has served as a basis for the chromatographic separation of sugars. Specifically, in 1959, Iorand and Edwards reported association constants fcr aqueous associations of phenylboronic acid with many saturated polyols; binding interactions ranged fron very weak (e.g., ethylene glycol, Kd=360 mM) to moderately strong (e.g., glucose, Kd=9.1 mM) . See J. Yoon, et al., Bioorganic and Medicinal Chemistry 1(4):267-71 (3993). The binding mechanism is believed to occur throuch bonding of adjacent hydroxyl groups on glucose to hycroxyl groups on a boronate moiety. U.S. Patent '5,503,773 (James, et al.) describes a fluorescent boronic acid-containing compound that emits fluorescence of a high intensity upon binding to saccharides, including glucose. The fluorescent compound has a molecular structure comprising a fluorophore, at least one phenylboronic acid moiety and at least one amine-providinig nitrogex atom where the nitrogen atom is disposed in the vicinity of the phenylboronic acid moiety so as to interact intramolecularly with the boronic acid. Such interaction thereby causes the compound to emit fluorescence upon saccharide binding. See also T. James, et al., J. Am. Chem. Soc. 117(35):8982-87 (1995). Additionally, fluorescent sensors using an anthrylboronic acid-containing compound for detecting blood glucose are known in the art. For example, J. Yoon, et al., J. Am. Chum. Soc. 114:5874-5875 (1992) describe that anthrylboronic acid can be used as a fluorescent chemosensor for signaling carbohydrate binding, including binding of glucose and fructose. Unfortunately, compounds which interact with glucose in the manner described above also have a tendency to interact with other compounds having hydroxyl groups, thus reducing the specilicity of a glucose assay, especially when assaying physiological samples which may contain interfering amounts of lactate, acetoacetate, etc. For example, some diabetic patients also develop lactic acidosis, in which blood lactate levels are greater than 5 mmol/liter. Thus, there remains a great need for glucose assays which are relatively insensitive to potentially interfering hydroxyl compounds, such as. lactate. BRIEF SUMMARY OF THE INVENTION In one aspect, the present invention is directed to a method for detecting the presence or concentration of glucose in a sample which may also contain an α-hydroxy acid or a β-diketone, which comprises: a) exposing the sample to a compound having at least two recognition elements for glucose, oriented such that the interaction between the compound and glucose is more stable than the interaction between the compound and the a-hydroxy acid or β-diketone, said compound also containing a detectable moiety having a detectable quality that changes in a concentration-dependent manner when said compound is exposed to glucose in said sample; and b) measuring any change in said detectable quality to thereby determine the presence or concentration of glucose in said sample, wherein the presence of the α- hydroxy acid or the β-diketone does not substantially interfere with said determination. In another aspect, the present invention is directed to a compound having the following structure wherein: -R1 and R2 are the sane or different and are selected from the following: ) hydrogen; ii) a substituent to modify the pKa and hydrolytic stability of the R8 moiety, iii) a detectable moiety, or iv) a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -R3 is hydrogen or a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -R4 and R5 are the same or different and are selected from the following: ) hydrogen, ii) a substituent to modify the pKa and hydrolytic stability of the R8 moiety, iii) a detectable moiety, or iv) a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -each Z is independently carbon or nitrogen; -R``6 and R7 are the sane or different and are i) linking groups having from zero to ten contiguous or branched carbon said/or heteroatoms, or ii) a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -R is selected from the following: i) an aliphatic and/or aromatic spacer containing from 1 to 10 contiguous atoms selected from the group consisting of carbon, oxygen, nitrogen, sulfur and phosphorus, ii) a detectable moiety, of iii) a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -each R8 is the same or different and is an optionally protected moiety which when unprotected is capable of interaction with the vicinal diol groups present in glucose; and -R9 and R10 are the same or different, and are i) hydrogen, ii) a detectable moiety, iii) a group which is a) a linking group capable of attachment to a solid support of a polymeric matrix, said support or matrix optionally containing a detectable moiety, and/or b) includes a functional group capable of altering the physical properties of the compound; with the proviso that the indicator compound contains at least one detectable moiety associated therewith, either directly or as part of the solid support or polymeric matrix. In another aspect, the present invention is directed to a detection system which comprises a compound described above. BRIEF DESCRIPTION OF THE DRAWINGS Figure 1 illustrates the normalized fluorescence emission (I/Io @ 420 nm) of an indicator as described in Example 1. Figure 2 illustrates the normalized fluorescence emission (I/I0 @ 428 nm) of an indicator as described in Example 2. Figure 3 illustrates the normalized fluorescence emission (I/I0 @ 428 nm) of an indicator as described in Example 3. Figure 4 illustrates the normalized fluorescence emission (I/I0 @ 427 nm) of an indicator as described in Example 4. Figure 5 illustrates the normalized fluorescence emission (I/I0 @ 540 nm) of an indicator as described in Example 5. Figure 6 illustrates the absorbance spectra of an indicator as described in Example 6. Figures 7-8 illustrate the ratio of the absorbance (450 nm/530 nm) of an indicator as described in Example 6. Figure 9 illustrates the normalized fluorescence emission (I/I0 at 550 nm) of an indicator as described in Example 6. Figure 10 illustrates the fluorescence spectrum, in the absence of glucose and in the presence of 100 mM glucose, of an indicator as described in Example 6. Figure 11 illustrates the normalized fluorescence emission (I/I0 at 550 nm) , in the presence of glucose and lactate, of an indicator as described in Example 6. Figure 12 illustrates the normalized fluorescence emission (I/I0 at 525 nm) of an indicator exposed to glucose as described in Example 10. Figure 13 illustrates the normalized fluorescence emission (I/I0 at 530 nm) of an indicator exposed to lactate as described in Example 10. Figure 14 shows the relative fluorescence emission (I @ 430 rm) of an indicat or exposed to glucose and lactate as described in Example 11. Figure 15 shows the relative fluorescence emission (I @ 4 30 nm) of an indicator exposed to glucose and lactate as described in Example 12. Figure 16 illustrates the fluorescence of an indicator exposed to glucose and lactate as described in Example 13. DETAILED DESCRIPTION OF THE INVENTION In one aspect, the present invention provides a way to detect the presence or concentration of glucose in a sample which may also contain interfering compounds, such as α-hydroxy acids or β-diketones. Such potentially interfering compounds incude lactate, acetoacetate, (3- hydroxy butyric acid, etc. The present invention is carried out using an indicator compound which is capable of recognizing glucose in a sample, but which is less likely to recognize interfering conpounds in the sample. The indicator compound has a least two recognition elements for glucose, oriented such that the interaction between the indicator compound and glucose is more stable than the interaction between the indicator compound and the interfering compounds. Suitable recognition elements include moieties which are capable of a preferaily reversible interaction with glucose, especially with the diol groups present in glucose. Several such recognition elements are known, and preferably include boronic acid, boronate ion, arsenious acid, arsenite ion, telluric acid, tellurate ion, germanic acid, germanate ion, etc. Most preferred are recognition elements containing boron. It will be understood that until use, the recognition elements may be capped with a protecting group. Such groups are well known, and include neoper:yl glycol, pinacol, etc. In certain embodiments, the capped recognition element is decapped in the medium in which the compound is to be used (see, e.g., Example 5). The recognition elements are preferably spaced on the indicator compound a sui :able distance from each other so as to allow at least two of the recognition elements to interact with a glucose nolecule, resulting in increased specificity. In general the recognition elements may have a spacer of up to about 30 atoms between them. Preferably, the recognition elements are oriented such that they are capable of being about 6Å apart when interacting with glucose The indicator compourds of the present invention have a detectable quality that changes in a concentration- dependent manner when the compound is exposed to a sample containing glucose. Many such qualities are known and may be used xn the present invention. For example, the indicator compound may include a luminescent (fluorescent or phosphorescent) or chemiluminescent moiety, an absorbance based moiety, etc. The indicator compound may include an energy donor noiety and an energy acceptor moiety, each spaced such that there is a detectable change when the indicator compound interacts with glucose. The indicator compound may include a fluorophore and a quencher, configured such that the fluorophore is quenched by the quencher when glucose is absent. In that situation, when glucose is present, the indicator undergoes a configurational change which causes the quencher to move sufficiently distant from the fluorophore so that fluorescence is emitted. Conversely, the fluorophore and quencher may be configured such that in the absence of glucose, they are sufficiently separated and the fluorophore emits fluorescence; upon interaction with glucose, the fluorophore and quencher are moved in sufficient proximity to cause quenching. The configurational change concept is described in more detail in our co-pending application Serial No. 09/754,219, filed January 5, 2001, entitled "Detection of Analytes", incorporated herein by reference. Alternatively, the indicator may include a moiety such as a fluorophore capable of interacting with the recognition element or another moiety spatially disposed with respect to the reccgnition element such that in the absence of glucose, the fluorophore emits fluorescence. Upon addition of glucose, the glucose competes with the interaction between the fluorophore and the recognition element, or the interaction between the fluorophore and the other moiety spatially disposed with respect to the recognition element, causing a reduction in fluorescence. An example of that concept is illustrated in Example 6. It will also be recognized that the indicator may be chosen such that the fluorophore emits no fluorescence, or a relatively low leveL of fluorescence, when the fluorophore interacts wi ;h the recognition element or another moiety spatially disposed with respect to the recognition element in tie absence of glucose. Upon addition of glucose, the glucose competes with the interaction between the fluorophore and the recognition element, or the interact .on between the fluorophore and the other moiety spatially disposed with respect to the recognition element, causing an increase in fluorescence. Other detectable moieties include those whose fluorescence is affected by glucose interaction via photoinduced electron transfer or inductive effects. These include the lantharide chelates disclosed in copending U.S. Application Serial No. 09/265,979 filed March 11, 1999 (and published as PCT International Application WO 99/46600 on September 16, 1999), incorporated herein by reference; polyaromatic hydrocarbons and their derivatives; coumarins; BoDiPy; dansyl; catechols; etc. Another class of moieties include those whose abso::bance spectrum changes upon interaction of the indicator compound with glucose, including Alizarin Red, etc. Another class of moieties include those whose fluorescence is modulated by proximity effects, e.g., energy donor/acceptor pairs such as dansyl/dabsyl, etc. Preferably, the detectable quality is a detectable spectral change, such as changes in absorptive characteristics (e.g., absorbtivity and/or spectral shift), in fluorescent decay time (determined by time domain or frequency domain measurement), fluorescent intensity, fluorescent ahasotropy or polarization; a spectral shift of the emission spectrum; a change in time-resolved anisotropy decay (determined by time domain or frequency domain measurement) , etc. The indicator compounds of the present invention, if soluble, may be used directly in solution if so desired. On the other hand, if the desired application so requires, the indicator compounds may be immobilized (such as by mechanical entrapment or covalent or ionic attachment) onto or within an insoluble surface or matrix such as glass, plastic, polymeric materials, etc. When the indicator compound i 3 entrapped within, for example, another polymer, the entrapping material preferably should be sufficiently permeable to glucose to allow suitable interaction between glucose and the indicator compound. If the indicator compounds are sparingly soluble or insoluble in water, yet detection in an aqueous medium is desired, the indicator compound may be co-polymerized with a hydrophilic mononer to form a hydrophilic macromolecule as described in co-pending U.S. application Serial No. 09/632,624, filed August 4, 2000, the contents of which are incorporated herein by reference. Preferred indicator compounds have the following structure: wherein: -R1 and R2 are the same or different and are selected from the following: hydrogen; ii) a substituent to modify the pKa and hydrolytic stability of the R8 moiety, iii) a detectable moiety, or iv) a linking group capable of attachment to a solid support or a polymeric matrix, sa..d support or matrix optionally containing a detectable moiety; -R3 is hydrogen or a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -R4 and R5 are the sane or different and are selected from the following: i) hydrogen, ii) a substituent to modify the pKa and hydrolytic stability of the R8 moiety, iii) a detectable moiety, or iv) a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -each Z is independently carbon or nitrogen; -R6 and R7 are the same or different and are i) linking groups havnig from zero to ten contiguous or branched carbon and/or heteroatoms, or ii) a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -R is selected from the following: i) an aliphatic and/or aromatic spacer containing from 1 to 10 contiguous atoms selected from the group consisting of carbon, oxygen, nitrogen, sulfur and phosphorus, ii) a detectable moiety, or iii) a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety; -each R8 is the same or different and is an optionally protected moiety whicn when unprotected is capable of interaction with the vicinal diol groups present in glucose; and -R9 and R10 are the sane or different, and are i) hydrogen, ii) a detectable moiety, iii) a group which is a) a linking group capable of attachment to a solid support or a polymeric matrix, said support or matrix optionally containing a detectable moiety, ard/or b) includes a functional group capable of altering the physical properties of the compound; with the proviso that the indicator compound contains at least one detectable moiety associated therewith, either directly or as part of the solid support or polymeric matrix. Suitable groups for modifying the: pKa and hydrolytic stability of the R8 moities would be readily apparent to one of ordinary skill, and include groups such as halogen; nitro; amino; halogen substituted alkyl; optionally substituted carboxyl; acyl; keto; nitrile; amide; ester; alkoxy; etc.. Suitable linking groups for any substituent may include groups from about 1 to about 20 contiguous atoms, which may be branched or substituted and which may include one or more hetreroatoms, which terminate in a functional group capable of further reaction or attachment to a polymer or support. Examples of suitable linking groups include alkyl; aryl; acyl; polyamide; polyether; all optionally substituted, and combinations thereof. R9 and R10 may further include functional groups capable of altering the physical properties of the compound, such as solubility, pKa, etc. For example, these include optionally substituted carboxylates, amino groups, quartenary ammonium groups, sulfonates, PEG, etc. It will be understood that when any of the substituents is a detecable moiety, that could also include suitable linking groups which link the detectable moiety to the rest of the indicator compound. Suitable linking groups include those listed above. Suitable detectable moieties include those defined above. R8 is preferably selected from the group consisting of boronic acid, boronate ion, arsenious acid, arsenite ion, telluric acid, tellurate ion, germanic acid, germanate ion, and combinations thereof. It will also be understood from the above definition that the present compounds and detection systems may be in polymeric form. Thus, an integral compound (containing recognition elements and detectable moiety) could be linked to an existing polymer, or the integral compound in monomeric form could be polymerized or co- polymerized with another suitable monomer to form a polymer. Alternatively, two separate monomeric components (e.g., one containing the recognition elements, and one containing a detectable moiety) could be co-polymerized so that the resulting polymer contains all necessary elements of the system (see Example 6). Many uses exist for the indicator compounds of the present invention, including uses as indicators in the fields of energy, medicine and agriculture. For example, the indicator compounds can be used to detect sub-levels or supra-levels of gluccse in physiological buffers or fluids, such as blood, plasma, serum, interstitial fluid, cerebrospinal fluid, urine, saliva, intraocular fluid, lymph, tears, or sweat, thus providing valuable information for diagnosing or monitoring such diseases as diabetes and adrenal insufficiency. Medical/pharmaceutical production of glucose for human therapeutic application requires monitoring and control. Uses for the present invention in agriculture include detecting levels of gluccse in soybeans and other agricultural products. Glucose must be carefully monitored in critical harvest decisions for such high value products as wine crapes. As glucose is the most expensive carbon source and feedstock in fermentation processes, glucose monitoring for optimum reactor feed rate control is importart in power alcohol production. Reactor mixing and control of glucose concentration also is critical to quality control during production of soft drinks and fermented beverages, which consumes the largest amounts of glucose and fermentable (vicinal diol) sugars internationally. When the indicator compounds incorporate fluorescent indicator substituents, various detection techniques also are known in the art. For example, the compounds of the invention can be used ir fluorescent sensing devices (e.g., U.S. Patent No. 5,517,313) or can be bound to polymeric material such as test paper for visual inspection. This latter technique would permit, for example, glucose measurement in a manner analogous to determining pH with a strip of litmus paper. The compounds described herein may also be utilized as simple reagents with standard benchtop analytical instrumentation such as spectrofluorometers or clinical analyzers as made by Shimadzu, Hitachi, Jasco, Beckman and others. These molecules would also provide analyte specific chemical/optica . signal transduction for fiber optic-based sensors and analytical fluorometers as made by Ocean Optics (Dunedin Florida), or Oriel Optics. U.S. Patent 5,517,311, the disclosure of which is incorporated herein by reference, describes a fluorescence sensing device in which the compounds of the present invention can be used to determine the presence or concentration of glucose in a liquid medium. The sensing device comprises a layered array of a fluorescent indicator molecule-contaning matrix (hereafter "fluorescent matrix"), a high-pass filter and a photodetector. In this device, a light source, preferably a light-emitting diode ("LED"), is located at least partially within the indicator material, or in a waveguide upon which the indicator matrix is disposed, such that incident light from the light source causes the indicator molecules to fluoresce. The high-pass filter allows emitted light to reach the photodetector, while filtering out scattered incident light from the light source. The fluorescence of the indicator molecules employed in the device described in U.S. Patent 5,517,313 is modulated, e.g., attenuated or enhanced, by the local presence of glucose. In the sensor described in U.S. Patent 5,517,313, the material which contains the indicator molecule is permeable to the analyte. Thus, the analyte can diffuse into the material from the surrounding test medium, thereby affecting the fluorescence emitted by the indicator compounds. The light source, indicator compound-containing material, high-pass filter and photodetector are configured such that at least a portion of the fluorescence emitted by the indicator compounds impacts the photodetector, generating an electrical signal which is indicative of the concentration of glucose in the surrounding medium. In accordance with other possible embodiments for using the indicator compounds of the present invention, sensing devices also are described in U.S. Patent Nos. 5,910,661, 5,917,605 and 5,894,351, all incorporated herein by reference. The compounds of the present invention can also be used in an implantable device, for example to continuously monitor blood glucose levels in vivo. Suitable devices are described in, for example, co- pending U.S. Patent Appllication Serial No. 09/383,148 filed August 26, 1999, as well as U.S. Patent Nos. 5,833,603, 6,002,954 and 6,011,984, all incorporated herein by reference. The compounds of the present invention can be prepared by persons skilled in the art without an undue amount of experimentation using readily known reaction mechanisms and reagents, for example including reaction mechanisms which are consistent with the general procedures described below. Example 1 Water soluble copolymer of anthracene derivative and MAPTAC I. Synthesis of mono-boronate-anthracene indicator co-polymerized in water-soluble polymer: A. 9-[3-(methacrylamido)propylamine]methylanthracene To a suspension of N-(3-aminopropyl)methacrylamide hydrochloride salt (11.82g, 66.0 mmole, 3.0 equiv.) and DBMP (10mg as inhibitor; in 250 mL CHCl3 at 0°C was added dropwise DIEA (18.5 g, :5.0 mL, 144 mmole, 6.5 equiv.) over a 20 min period. The mixture was allowed to warm to 25°C and then recooled to 0°C. To the cooled mixture was added dropwise a solution of 9-chloromethylanthracene (5.0 g, 22 mmole) in CHCl3 (100 mL) over a 1 hour period. The mixture was subsequently stirred at 25°C for 1 hour, 50°C for 12 hours and then 70°C for 2 hours. At this time, the mixture was washed with 4 x 60 mL portions of water, and the combined aqueous layers were extracted with CH2Cl2. The combined organic extracts were dried over anhydrous Na2SO4, decanted and concentrated in vacuo. The crude material was purified by silica gel chromatography (flash silica gel, 2-5% CH3OH/CH2Cl2) to yield 2.44 g (33%) of a solid product. TLC: Merck silica gel 6( plates, Rf 0.39 with 90/10 CH2Cl2/CH3OH, see with UV (254/366), ninhydrin stain. B. 9-[N-[2-(5,5-dimethylborinan-2-yl)benzyl]-N-[3- (methacrylamido) propylan ino ] methylanthracene. To a solution of 9-[3-(methacrylamido)propylamino]- methylanthracene (2.44 c, 7.34 mmole) and DBMP (10 mg as inhibitor) in 200 ml CHCl3 at 0°C was added DIEA (2.85 g, 3.84 mL, 22.0 mmole, 3.C equiv.) in portions over a 10 rain period, followed by the dropwise addition of a solution of (2-bromometh/lphenyl)boronic acid neopentyl ester (2.4 9 g, 8.81 mmols, 1.2 equiv.; over a 30 min period. The mixture was subsequently stirred at 25°C for 20 hours. At this time, the mixture was washed with water, and the combined aqueous layers were extracted with CH2Cl2. The combined organic extracts were dried over anhydrous Na2SO4, decanted and concentrated in vacuo. The crude material was purified by silica gel chromatography (flash silica gel, 2-5% CH3OH/CH2Cl2) to yield 2.50 g (76%) of a lightly yellow crystalline solid. Mp: 72-73°C. TLC: Merck silica gel 60 plates,Rf 0.36 with 90/10 CH2Cl2/CH3OH, see with UV '254/366), ninhydrin stain. C. Water soluble copolymer of 9- [N- [2- (5 ,5-dimethyl- boxinan-2-yl)benzyl] -N- [3- (methacrylamido)propylamino] - methylanthracene and MAPTAC (1:20 molar ratio) . To a solution of 9-[N - [2- (5,5-dimethylborinan-2-yl) - benzyl] -N- [3- (methacrylamido) propylaraino]methylanthracene (0.0490 g, 0.105 mmole) e.rtd [3-(methacrylamido)propyl]- trimethylammonium chloride (MAPTAC, 50 wt % aqueous solution, 0.48 g, 0.90 mL, 2.1 mmole, 20 equiv.) in 1.5 mL ethylene glycol was added 4 , 4 '-azobis (cyanovaleric acid) (0.008 g, 0.03 mmole, 1.4 mole % of total monomer). The solution was purged with argon gas for 5 minutes and then heated to 60°C in the dark for 18 hours. At this time, the viscous solution was cooled to 25°C, diluted with 5 mL water and dialyzed through a cellulose acetate membrane (MWCO 3500) against 3 x 4 L of water. The dialyzed material was concentrated to dryness to yield 0.339 g (68%) of a yellow glassy solid. II. Modulation of Fluorescence With Glucose and Lactate. The modulation of the fluorescence of the copolymer (which contains a single recognition element) prepared in this example by glucose and lactate was determined. Figure 1 shows the normalized fluorescence emission (I/Io @ 420 nm) of 0.5 mg/mL solutions of the copolymer (1:20 molar ratio) in PBS containing a) 0-20 mM glucose; b) 0-20 mM lactate. Spectra were recorded using a Shimadzu RF-5301 spectrafluorometer with excitation @365 nm; excitation slits at 1.5 nm; emission slits at 5 nm; ambient temperature. Error bars are standard deviation with duplicate values for each data point. The fluorescence of the copolymer was affected by the presence of glucose and lactate. Example 2 Modulation of bis-boronate-indicator covalently attached to water-soluble polymer by glucose and potential physiological interferences. A. 9,10-bis[[2-(2-hydroxyethoxy)ethylamino]methyl]- anthracene. I. Synthesis of single-)methacrylate monomer of bis-boronate-anthracene indicator To a solution of 2-(2-aminoethoxy) ethanol (31.4 g, 30.0 mL, 299 mmole, 20.9 equiv.) in 40 mL CHCl3 at 23°C was added 9,10-bis (chloromethyl) anthracene (3.94 g, 14.3 mmole). The solution was stirred in the dark for 67 hours. At this time, added 100 mL CH2Cl2 and washed with 1 x 50 mL and 2 x 100 mL portions of NaHCO3 (saturated aqueous solution). The organic extract was dried over anhydrous Na2SO4, filtered and concentrated to yield 4.67 g (79%) of a yellow powder. Product (~85 % pure by RP-HPLC) was carried on as is. HPLC conditions: HP 1100 HPLC chromatograph, Vydac 20lTP 10 x 250 mm column, 0.10) mL injection, 2 mL/min, 370 run detection, A = water (0. 1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 run, 10-80% B over 18 min, 80-100% B over 2 min, 10) %B 2 min, retention time 15.6 min. B. 9,10-bis [N- [2- (5,5-dimethylborinan-2-yl) benzyl] -N- [2- (2-hydroxyethoxy)ethylamino]methyl] anthracene. A solution of 9,10-bis [ [2-(2-hydroxyethoxy) - ethylamino]methyl]anthracene (4.02 g, 9.75 mmole), DIEA (12.6 g, 17.0 mL, 97.5 mmole, 10.0 equiv.) and (2-bromomethylphenyl)boronic acid neopentyl ester (13.7 g, 48 mmole, 4.9 equiv.) ;.n 125 mL CHCl3 at 23°C was stirred in the dark for 4 6 hours. At this time, the reaction mixture was concentrated initially by rotary evaporation, then using a vacuum pump to remove the DIEA. The residue was purified by alumina column chromatography (150 g activated neutra alumina, 0-3% CH3OH/CH2Cl2) to yield 5.67 g (70%) of a viscous oil which solidified upon standing. Product (~85 % pure by RP-HPLC) was carried on as is. TLC: Merck basic alumina plates, Rf 0.33 with 95/5 CH2Cl2/CH3OH, see with U\ (254/366). HPLC conditions: HP HOC HPLC chromatograph, Vydac 201TP 10 x 250 mm column, 0.100 mL injection, 2 mL/min, 370 run detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 rain, 10-80% B over 18 min, 80-100% B over 2 min, 1C0% B 2 min, retention time 18.8 min. C. 9-[N-[2-(5,5-dimethy Lborinan-2-yl)benzyl]-N- [2- (2-methacroyloxyethoxY) ethylamino]methyl] -10- [N- [2- (5,5-dimethylborinan-2-yl) benzyl] -N- [2- (2-hydroxyethoxy) ethylamino] -methyl] anthracene . (Single- methacrylate monomer) A solution of 9,10-b..s[N-[2-(5, 5-dimethyl- borinan-2-yl)benzyl]-N-[2-(2-hydroxyethoxy)ethylamino]- methyl]anthracene (0.298 g, 0.359 mmole), methacrylic acid (0.304 g, 0.300 mL, 3.53 mmole, 9.84 equiv.), DCC (0.965 g, 4.68 mmole, 13 0 equiv.) and N,N-dimethyl- aminopyridine (0.020 g, ),16 mmole, 0.46 equiv.) in 15 mL CH2Cl2 at 23°C was stirred in the dark for 4 hours. At this time, the reaction mixture was filtered and concentrated by rotary evaporation. The residue was purified by alumina column chromatography (50 g activated neutral alumina, 0-4% CH2CH/CH2Cl2) to yield 0.150 g (47%) of a yellow solid. FAB MS: Calc=d for C52H66E2N209 [M]+ 88 5; Found [M + 1] + 886. TLC: Merck basic alumina plates, Rf 0.45 with 95/5 CH2Cl2/CH3OH, see with UV .254/366). HPLC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm column, 0.100 mL injection, 2 mL/min, 370 nm detection, A = water (0.1% HFBA) and It = MeCN (0.1% HFBA) , gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 21 min. D. Water soluble copolymer of 9-[N-[2-(5,5-dimethyl- borinan-2-yl)benzyl] -N- [2 -(2-methacroyloxyethoxy) ethyl- amino] methyl] -10- [N- [2- (5-, 5-dimethylborinan-2-yl) benzyl] - N- [2- (2-hydroxyethoxy) ethylamino] -methyl] anthracene and TMAMA (1:50 molar ratio) To a solution of [2-(methacryloxy)ethyl]trimethyl- ammonium chloride (TMAMA, 70 wt% aqueous solution, 0.344 g monomer, 1.66 mmole, 5( equiv.) in 0.600 mL water was added a solution of 9-[N-[2-(5,5-dimethylborinan-2-yl)- benzyl]-N-[2-(2-methacroyloxyethoxy)ethylamino]methyl]- 10- [N-[2-(5,5-dimethylborinan-2-yl)benzyl]-N-[2-(2- hydroxyethoxy)ethylaminc]methyl]anthracene (0.0024 g, 0.0033 mmole) in 3.00 ml MeOH. To this mixture was added 4,4'-azobis(4-cyanovaleric acid) (0.0075 g, 0.027 mmole, 1.6 mole % of total monomer). The solution was filtered through a 0.45μ membrane filter, was purged with nitrogen gas and then heated in the dark at 55°C for 16 hours. At this time, the viscous solution was cooled to 25°C and concentrated in vacuo. The residue was diluted with 20 mL water and filtered through a 0.2μ . membrane filter. The polymer solution was dialyzed through a cellulose acetate membrane (MWCO 3500} against 2 x 4 L of water. From the dialysis was obtained 38.5 mL of polymer solution. Concentratior of a portion of this solution to dryness indicated 0.0075g polymer per 1.0 mL solution. Overall 0.289g (77%) yield of polymer. II. Modulation of Fluorescence With Glucose, Lactate and Acetoacetate The modulation of the fluorescence of the copolymer (which contains two recognition elements) prepared in this example by glucose, lactate and acetoacetate was determined. Figure 2 shows the normalized fluorescence emission (I/Io @ 428 nm) of a 1.5 mg/mL solution of anthracene bis boronate-TMAMA (1:50 mole ratio) copolymer in PBS containing a) 0-20 mM glucose; b) 0-20 mM lactate; c) 0-20 mM lithium acetcacetate. Spectra were recorded using a Shimadzu RF-530 spectrafluorometer with excitation @365 nm; excitation slits at 1.5 nm; emission slits at 1.5 nm; ambient temperature. The fluorescence of the copolymer was affected by the presence of glucose, but not by the presence of lactate or acetoacetate. Example 3 Effect of lactate in solation on the dose response effect of glucose on the fluorescence of bis-boronate-anthracene indicator A. 9,10-bis[[2-(tert-butoxycarbonyl)ethylamino]methyl]- anthracene. A solution of β-alanine tert-butyl ester hydrochloride (3.06 g, 16.8 mmole, 5.09 equiv.), DIEA (4.27 g, 5.75 mL, 33.0 mmole, 10.00 equiv.) and 9,10- bis (chloromethyl) anthrac ene (0.910 g, 3.31 mmole) in 75 mL CHCl3 at 23°C was stirred in the dark for 93 hours. At this time, the solution was filtered and washed with 1 x 40 mL and 2 x 60 mL portions of NaHCO3 (saturated aqueous solution). The organic extract was dried over anhydrous Na2SO4, filtered and concentrated to yield a crude yellow solid. The residue was purified by silica gel column chromatography (30 g gravity grade gel, 0-3% CH3OH/CH2Cl2) to yield 1.06 g (65%) of a viscous yellow-orange. Product was carried on as is. TLC: Merck silica gel 6( plates, Rf 0.33 with 95/5 CH2Cl2/CH3OH, see with W (254/366) . B. 9,10-bis [N- [2- (5,5 -dimethylborinan-2-yl)benzyl] -N- [2-(tert-butoxycarbonyl)ethylamino]methyl]anthracene. A solution of 9,10-bis[[2-(tert-butoxycarbonyl)- ethylamino]methyl]anthracene (1.60 g, 3.25 mmole), DIEA (4.45 g, 6.00 mL, 34.4 mmole, 10.6 equiv.) and (2- bromomethylphenyl)boronic acid neopentyl ester (4.80 g, 17.0 mmole, 5.22 equiv. in 30 mL CHCl3 at 23°C was stirred in the dark for 4.5 days. At this time, 45 mL CHCl3 were added to ,tne mixture and the mixture was washed with 2 x 25' mL portions of NaHCO3 (saturated aqueous solution). The organic extract was dried over anhydrous Na2SO4, filtered and concentrated to yield crude reddish oil. The residue was purified by alumina column chromatography (100 g activated neutral alumina, 0-3% CH3OH/CH2Cl2) to yield ~ 3.5 g of an orange solid. The product was dissolved, followed by the formation of a white precipitate (DIEA-HBr salt). The solution was filtered and the filtrate concentrated to yield 2.72 g (93%) of an orange solid, Product (>80 % pure by RP- HPLC) was carried on as is. TLC: Merck basic alumina plates, Rf 0.66 with 95/5 CH2Cl2/CH3OH, see with UV (254/366). HELC conditions: HP 110) HPLC chromatograph, Vydac 201TP 10 x 250 mm column, 0.1)0 mL injection, 2 mL/min, 370 nm detection, A = water (0 1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80- 100% B over 2 min, 100% 3 2 min, retention time 23.9 min. C. 9,10-bis [N- (2-boron abenzyl) -N- [2-- (carboxyethyl)amino]-methyl]anthracene. A solution of 9,10-bis [N-[2-(5, 5--dimethylborinan-2- yl)benzyl]-N-[2-(tert-bu :oxycarbonyl)ethylamino]methyl]- anthracene (0.556 g, 0.620 mmole) in 5 mL 20% TFA/CH2Cl2 at 23°C was stirred in the dark for 25 hours. At this time, the reaction mixture was concentrated under a stream of N2 gas. The residue was triturated with 3 x 10 mL portions of ether. The residual solid was dried in vacuo to yield 0.351g (87%) of a fluffy yellow powder. FAB MS: Glycerol matrix; 3alc=d for C42H46B2N20010 (bis glycerol adduct) [M]+ 76), Found [M]+ 760. HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.325 mL injection, 0.75 mL/min, 1.5 mL injection loop, 363 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA) , gradient 10% B 2 min, 10- 80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 16.7 min. D. Modulation of Fluorescence With Glucose and Lactate The modulation of the fluorescence of the indicator compound (which contains two recognition elements) prepared in this example by glucose and lactate was determined. Figure 3 s lows the fluorescence (at 428 ran) of 75 pM solutions of bis carboxylate bis-boronate- anthracene indicator in PBS containing a) 0-10 mM glucose, 0 mM lactate; b) 0-10 mM glucose, 2 mM lactate; c) 0-10 mM glucose, 5 ml! lactate. Spectra were recorded using a Shimadzu RF-530 . spectrafluorometer with excitation @365 nm; excitation slits at 1.5 nm; emission slits at 1.5 nm; ambient temperature. All points measured in triplicate, with ±1 SD error bars included. The presence of lactate did not substantially affect the fluorescence modulation of the indicator by glucose. Example 4 Selectivity of Bis-Bororate Glucose Indicator for Glucose vs. Lactate and Acetoace tate When Indicator Covalently Immobilized in the Hydrogel I. Preparation of Dual-Methacrylamide Monomer A. 9,10-bis[3-(methacrylamido)propylamino]- methylanthracene. A suspension of 9,1 )-bis(chloromethyl)anthracene (1.5 g, 5.45 mmole), DIEA (28.17 g, 38.00 mL, 218 mmole, 40 equiv.), N-(3-aminopr)pyl)methacrylamide hydrochloride salt (9.76 g, 54.5 mmole 10.0 equiv.), and ~ 5 mg of BHT in 200 mL CHCl3 at 23°C was stirred in the dark for 4 days at 40°C. At this time, the temperature was increased to 45°C and the mixture was stirred for 3 days longer. At this time, a precipitate had formed. The mixture was filtered, and the solid product dissolved in the minimum amount of CH2Cl2. A yellow crystalline solid, the bis hydrochloride salt of the desired product, formed overnight (3.15 g, quantitative). TLC: Merck basic alumina plates, Rf 0.31 with 90/10 CH2Cl2/CH3OH, see with UV (254/366). HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.100 mL injection, 0.75 mL/min, 360 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 10D% B 2 min, retention time 15.0 min. B. 9,10-bis [N- [2- (5,5- limethylborinan-2-yl)benzyl] -N- [3-(methacrylamido)propylamino]methylanthracene. (Dual- methacrylamide monomer) A solution of 9,10-bis [3-(methacrylamido)- propylamino]methylanthra.:ene (0.0.650 g, 1.34 mmole of the free amine), DIEA (3.612 g, 0.825 mL, 4.74 mmole, 3.55 equiv.), (2-bromomethylphenyl)boronic acid neopentyl ester (1.34 g, 4.74 mmole, 3.55 equiv.) and BHT (5 mg as inhibitor) in 20 mL CHC, at 23°C was stirred in the dark for 5 days. At this tine, the reaction mixture was concentrated in vacuo a;id the residue was purified by alumina chromatography !200 g activated neutral alumina, 0-2% CH3OH/CH2Cl2) to yield 0.465 g (39%) of a very viscous yellow oil. TLC: Merck basic alumina plates, Rf 0.59 with 90/10 CH2Cl2/CH3OH, see with UV (254/366). HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, (.050 mL injection, 0.75 mL/'min, 360 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 1C % B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 1C0% B 2 min, retention time 16.9 min. C. Preparation of N,N-dimethylacrylamide hydrogel with glucose indicator: A solution of N,N-dimethylacrylamide (40% wt.) and N,N=-methylenebisacrylamide (0.8% wt.) in ethylene glycol was prepared. 9,10-bis[N-[2-(5,5-dimethylborinan-2-yl)- benzyl]-N-[3-(methacrylauido)propylamino]methylanthracene (17.8 mg, 2xl0-5 mole) and 40 μL of aqueous ammonium persulfate (5% wt) were combined with 1 mL of ethylene glycol monomer solution. The resulting solution was placed in a glove box purged with nitrogen. An aqueous solution of N,N,N=,N=-tetramethylethylenediamine (80 uL, .5% wt.) was added to the nonomer formulation to accelerate polymerization. The resulting formulation was poured in a mold constructed from microscope slides and 100 micron stainless steel spacer. After being kept for 8 hours in nitrogen atmosphere the mold was placed in phosphate buffered saline (PBS) (10 mM PBS, pH=7.4), the microscope slides were separated, and the hydrogel was removed. The hydrogel was washed with 100 mL of PBS containing 1 mM lauryl sulfate sodium salt and 1 mM EDTA sodium salt for 3 days, 1 he solution being changed every day, followed by washing with DMF/PBS (10/90 by vol., 3 x 100 mL), and finally with PBS (pH=7.4, 3 x 100 mL). The resulting hydrogel polymer was stored in PBS (10 mM PBS, pH=7.4) containing 0.2% wt. sodium azide and 1 mM EDTA sodium salt. II. Modulation of Fluorescence With Glucose, Lactate and Acetoacetate The modulation of the fluorescence of the indicator compound (which contains two recognition elements) prepared in this example by glucose, lactate and acetoacetate was determined. Figure 4 shows the normalized fluorescence emission (I/Io @ 427 nm) of a hydrogel containing the glucose recognition molecule of this example in 10 mM PB! , pH 7.4 containing 0.2% NaN3 and 1 mM EDTA containing various amounts of sodium-L-lactate, lithium acetoacetate or c-D-glucose. Data were recorded using a Shimadzu RF-5301 spectrofluorometer with excitation @365 nm (slit - 3 nm) and emission at 427 nm (slit = 3 nm) at low sensitivity at 37°C using a temperature controlled sample holder. The cuvettes containing 3 mL of the de sired solution were equilibrated at 37°C for 15 minutes before measurement. Each hydrogel sample was measured in four independent samples. Error bars are standard deviation with quadruplicate values for each data point. The hygrogels containing a glucose recognition molecule were prepared as previously described. The hydrogels were mounted on glass slides and covered with polyester mesh in PMMA cuvettes at 4 5D to the incident light. Solutions of 1, 5, 10 and 20 mM sodium L-lactate [Aldrich], 5, 10 and 20 mM lithium acetoacetate [Aldrich], and 1, 2, 4, 5, 10, and 20 mM α-D-glucose were prepared in 10 mM PBS, pH 7.4 containing 0.2% NaN3 and 1 mM EDTA. The fluorescence of the copolymer was affected by the presence of glucose, but not by the presence of lactate or acetoacetate. Example 5 Glucose selectivity vs. lactate using bis-boronate recognition and proximity quenching signal generation A. N- (2 ,2-diethoxyethyl) -4-bromo-l, 8-naphthalimide. A suspension of 4-brorno-1, 8-naphthalic anhydride (10.0 g, 36.1 mmol) and aminoacetaldehyde diethyl acetal (4.81 g, 5.26 mL, 36.1 mmol, 1 equiv. ] in 45 mL EtOH was stirred at 45°C for 3 days. At this time, the resulting suspension was filtered, washing with EtOH and the residue was dried to yieLd 13.3 g (94%) of a light brown solid product. TLC: Merck silica gel 60 plates plates, Rf 0.17 with 98/2 CH2Cl2/CH30H, see with UV (254/366) . HPLC: HP 1100 HPLC chromotograph, Waters 5 x 100 mm NovaPak HR C18 column, 0 050 mL injection, 0.75 mL/min, 1.5 mL injection loop, 350 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 24.2 min. B. N-(2,2-diethoxyethyl)-4-butylamino-1,8-naphthalimide. A solution of N-(2,2 -diethoxyethyl) -4-bromo-1, 8- naphthalimide (0.797 g, 2.03 mmol) and n-butylamine (1.48 g, 2.00 mL, 20.2 mmol,0.96 equiv.) in 8 mL NMP was heated at 45°C for 66 hours. At this time, the resulting suspension was allowed to cool to 25°C, followed by filtration. The residue was dissolved with 50 mL ether ' and extracted 3 x 50 mL water. The organic extract was dried over anhydrous Na2SO4, filtered and concentrated to yield a crude yellow povder. The crude material was purified by silica gel chromatography (25 g gravity grade gel, 0-1% CH3OH/CH2Cl2) to yield 0.639 g (82%) of a yellow powder. TLC: Merck silica gel 60 plates, Rf 0.71 with 95/5 CH2Cl2/CH3OH, see with UV (254/366) . HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.D50 mL injection, 0.75 mL/min, 1.5 mL injection loop, 4 30 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 23.5 min. C. N- (2-oxoethyl) -4-butylamino-1, 8naphthalimide. A solution of N-(2,2-diethoxyethyl)-4-butylamino- 1,8-naphthalimide (0.622 g, 1.62 mmol) and p-toluene- sulfonic acid mono hydrate (0.010 g, 0.053 mmol, 0.032 equiv.) in 25 mL acetone was stirred at 25°C for 18 hours. At this time, the solution was concentrated and the residue purified by silica gel chromatography (25 g gravity grade gel, 0-1% CH3OH/CH2CL2) to yield 0.470 g (94%) of an orange solid TLC: Merck silica gel 60 plates, Rf 0.61 with 95/5 CH2Cl2/CH3OH, see with UV (254/366). HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 3.050 mL injection, 0.75 mL/min, 1.5 mL injection loop, 3 50 run detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 8 3-100% B over 2 min, 100% B 2 min, retention time 19.6 min. D. N- (4-dimethylaminobenzyl) -1, 6-diaminohexane. A suspension of 4-limethylaminobenzaldehyde (1.00 g, 6.70 mmol), Na2SO4 (6.70 g, 47.2 mmol, 7.04 equiv.) and 1, 6-diaminohexane (3.89 g, 33.5 mmol, 5.00 equiv.) in 20 mL anhydrous EtOH was stirred in the dark at 25°C under an atmosphere of nitrogen gas for 18 hours. At this time, the solution was filtered and NaBH4 (1.73 g, 45.8 mmol, 6.84 equiv.) was added to the filtrate. The suspension was stirred at 25°C for 5 hours. At this time, the reaction mixture was concentrated and the residue dissolved in 50 mL water and extracted 3 x 50 mL ether. The combined organic extracts were washed 2 x 50 mL water. The combined aqueous extracts were extracted 2 x 50 mL ether. The combined organic extracts were dried over Na2SO4, filtered and concentrated to yield 1.35 g (81%) of a viscous oil. TLC: Merck silica gel 6( plates plates, Rf 0.58 with 80/15/5 CH2Cl2/CH3OH/iPrNH2, see with ninhydrin stain, UV (254/366) . HPLC: HP 1100 HPLC chromatography Waters 5 x 100 nun NovaPak HR C18 column, 0.350 mL injection, 0.75 mL/min, 1.5 mL injection loop, 230 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 8C-100% B over 2 min, 100% B 2 min, retention time 13.3 min. E. N-2- [6-N (H-4-dimethylaminobenzyl) aminohexyl] amino- ethyl) -4-butylamino-1, 8- naphthalimide. To a suspension of N-(2-oxoethyl)-4-butylamino-l,8- naphthalimide (0.34 6 g, 1.11 mmol) in 25 mL anhydrous MeOH was added a solution of N-(4-dimethylamino- benzyl)-l, 6-diaminohexane (0.554 g, 2.22 mmol, 2.00 equiv.) and acetic acid (0.067 g, 1.1 mmol, 1.0 equiv.) in 20 mL anhydrous MeOH To this mixture was added a solution of NaCNBH3 (0.(70 g, 1.1 mmol, 1.0 equiv.) in 5 mL anhydrous MeOH. The reaction mixture was stirred at 25°C for 15 hours. At this time, the MeOH was removed by rotary evaporation and the residue was dissolved in 30 mL water. The solution was adjusted to pH 2 with 1 N HCl and then stirred for 1 hour at 25°C. At this time, the solution was adjusted to pH 12 with 1 N NaOH and subsequently extracted 3 x 50 mL CH2Cl2. The combined organic extracts were washed 3 x 50 mL water, dried over anhydrous Na2SO4, filtered and concentrated to yield a crude brown oil. The crude material was purified by silica gel chromatography (35 g flash grade gel, 0-50% CH3OH/CH2Cl2, then 4 5/5C/5 CH3OH/CH2Cl2/iPrNH2) to yield 0.190 g (32%) of diamire product. FAB MS: Calc=d for C33H25N5O2 [M]+ 54 4; Found [M]+ 54 4. TLC: Merck silica gel 60 plates, Rf 0.42 with 80/20 CH2Cl2/CH3OH, see with rinhydrin stain and UV (254/366). HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.050.mL injection, 0.75 mL/min, 1.5 mL injection loop, 3 50 nm detection, A = water (0.1% HFBA) and B = MeCN {0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 8 )--100% B over 2 min, 100% B 2 min-, retention time 17.6 min F. N-2-[6-N-(N-4-dimetliylaminobenzyl)-6-N-[2-(5,5- dimethylborinan-2-yl)benzyl] aminohexyl] - [2- (5,5-dimethyl- boxinan-2-yl)benzyl] aminoethyl-4-butylamino-1, 8- naphthalimide. To a solution of N- 2-[6-N-(N-4-dimethylaminobenzyl)- aminohexyl]aminoethyl)-4-butylamino-1,8-naphthalimide (0.150 g, 0.276 mmole) and DIEA (0.355 g, 0.478 mL, 2.81 mmole, 10.0 equiv.) in 5 mL CHCl3 was added a solution of (2-bromomethylphenyl)boronic acid neopentyl ester (0.390 g, 1.38 mmole, 5.00 equiv.) in 2 mL CHCl3. The solution was subsequently stirred at 25°C for 27 hours. At this time, the mixture was contentrated and the residue was purified by alumina colunn chromatography (100 g activated neutral alumina, 0-5% CH3OH/CH2Cl2) to yield 0.024 g (19%) of a visco is brown oil. FAB MS (glycerol matrix) Calc'd for C53H67B2N50O8 [M]+ 924 (bis glycerol adduct in phace of bis neopentyl ester of boronic acids); Found [M + 924. TLC: Merck neutral alumina plates, Rf 0.62 with 80/20 CH2Cl2/CH3OH, see with UV (254/366*). HPLC: HP 1100 HPLC chrometograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.C50 mL injection, 0.75 mL/min, 1.5 mL injection loop, 450 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HF3A), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 20.7 min. G. N-2- [6-N- (N-4-dimethylaminobenzyl) -6-N- [2 - (borono) benzyl] aminohitxyl ]-[2- (borono) benzyl] amino- ethyl-4-butylamino-1, 8-naphthalimide (nBuF-hexa-Q bis-boronate). The free bis boronic acid product used in glucose studies results from dissolution of N-2-[6-N-(N-4- dimethyl-aminobenzyl) -6- N- [2- (5, 5-dimethylborinan-2- yl)benzyl]amino-hexyl]-[2-(5,5-dimethylborinan-2- yl)benzyl]aminoethyl-4- butylamino-1,8-naphthalimide in the MeOH/PBS buffer system. H. Modulation of fluorescence with glucose and lactate. The modulation of the fluorescence of the indicator compound (which contains two recognition elements) prepared in this sample oy glucose and lactate was determined. Figure 5 stows the normalized fluorescence emission (I/Io @ 535 ran) of 0.015 mM solutions of the indicator compund in 70/30 MeOH/PBS containing a) 0-20 mM glucose; b) 0-20 mM lactate. Spectra were recorded using a Shimadzu RF-5301 spectrafluorometer with excitation @ 450 nm; excitation shitf at 1.5 rm; emission slits at 1.5 nm; ambient temperature. Error bars are standard deviation with triplicate values for each data point. The fluorescence of the indicator was affected by the presence of glucose, but not substantially affected by the presence of lactate Example 6 Effect of glucose or lactate on acrylamide gel containing H-[3- (methacrylamido) propyl] -3,4-dihydroacy-9, lO-dioxo-2- anthracenesulfonamide (Alizarin Red S monomer) and α,α'-bis [N- [2- {5,5-dimethylborinan-2-yl)benzyl] -N- [3- (methacrylamido)propyl amino] ~1,4--xylene (bis boronic acid monomer): A. 3,4-Dihydroxy-9,1( -dioxo-2~anthracenesnlfonyl chloride: 3, 4~dihydroxy-9, 0-dioxo~2-anthracenesulfonic acid sodium salt (1,4 g, 3 9 mmoles) was combined with 30 mL of chlorosulfonic acid and heated to 90°C for 5 hours, after which the solution was cooled to 0°C and poured into 100 g of ice. After the ice melted the solution was extracted with CH2Cl2 (3 x 100 mL) , methylene chloride extracts were combined, dried with Na2SO4 and evaporated to produce 0.87 g of solid (Yield 66%). B. N- [3- (methacrylamido) propyl] -3,4-dibydroxy-9,10- dioxo-2-anthracenesulfonamide: 3,4~dihydroxy~9( 10-dioxo-2-anthracenesulfonyl chloride (96 mg, 0.28 mmoles) and N- (3-aminopropyl) methacrylamide hydrochloride (108 mg, 0.6 mmoles) were combined with 20 mL of CH2Cl2. To this suspension Et3N (303 mg, 3 mmoles) was added. The mixture was stirred at room temperature for 24 hours, filtered, and solvent was evaporated. The resulting solid was subjected to column chomatography on SiC, (10 g) with CH2Cl2/MeOH (90/10) as an eluent. The product was obtained as a red solid {80 mg, 64% yield). FAB MS: Calculated for C21H20N2O7S M+ 4 45; Found M+ 445. HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 0 100 mL injection, ,0.75 mL/min, 2 mL injection loop, 370 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 8C-100% B over 2 min, 100% B 2 min, retention time 17.67 min . C. α,α' -bis [3-(methacrylamido)propylamino] -1,4-xylene. A solution of N- (3-aminopropyl)methacrylamide hydrochloride salt (3.00 g, 16.8 mmole, 2.21 equiv.), DIEA (6.5 g, 8.8 mL, 5C mmole, 6.6 equiv.), terephthaldicarboxaldel yde (1.02 g, 7.60 mmole) and Na2SO4 (10.7 g, 75.3 mmole, 9 91 equiv.) in 75 mL anhydrous MeOH was stirred in the dark at 25DC for 18 hours. At this time, more Na2SO4 (10.7g, 75.3 mmole, 9.91 equiv.) was added and stirring continued for 6 hours longer. At this time, the solution was filtered and NaBH4 (1.73 g, 45.7 mmole, 6.01 equiv.) was added to the filtrate in portions and subsequently stirred at 25°C for 21 hours. The suspension was filtred through Celite and the filtrate was concentrated. The residue was dissolved in 100 mL CH2Cl2 and washed 1 x 25 mL saturated aqueous NaHCO3. The organic extract was cried over anhydrous Na2SO4, filtered and concentrated to yield a viscous oil. The product was carried on as is. HPLC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm column, 0.100 mL injection, 2.00 mL/min, 260 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 15.8 min. D. α,α=-bis[N-[2-(5,5-dimethylborinan-2-yl)benzyl]- N- [3- (methacrylamido) propylamino] -1,4-xylene. A solution of α,α=-bis[3-(methacrylamido)- propylamino]-1,4-xylene (2.94 g, 7.61 mmole), DIEA (2.97 g, 4.00 mL, 23.0 mmoles, 3.02 equiv.), (2-bromomethyl~ phenyl)boronic acid neopentyl ester (6.50 g, 23.0 mmole, 3.02 equiv.) and BHT ( 5 mg as inhibitor) in 75 mL CH2Cl2 at 25°C was stirred in the dark for 28 hours. At this time, the mixture was washed 1 x 25 mL saturated aqueous NaHCCb. The organic extract was dried over anhydrous Na2SO4, filtered and concentrated. To the residue was added 200 mL ether and the suspension was stirred for 18 hours. The suspensior was filtered and the residue dissolved in CH2Cl2, fitered and the filtrate concentrated. To the solid residue was added 150 mL ether and the suspension was stirred for 18 hours. At this time, the suspension was filtered yielding 1.98 g (33%) of a fluffy pin) powder. FAB MS: Calc=d for C46H64B2N4O6 [M]+ 790; Found [M + 1] + 791. HPLC: HP 1100 HPLC cinematograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.050 mL injection, 0.75 mL/min, 280 nm detection, A = water (0.1% HFBA) and.B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 13.4 min. E. Preparation of acrylamide gel containing N-[3-(methacrylamido)propyl]-3,4-dihydroxy-9,10-dioxo-2- anthracenesulfonamide (Alizarin Red S monomer) and α,α'-bis[N-[2-(5,5-dimethylborinan-2-yl)benzyl]-N-[s- (mathacrylamido) propyl amino] -1,4-xylene: Ethylene glycol solution containing 30% wt. acrylamide and 0.8% wt. N,N'-methylenebisacrylamide was prepared. N- [3- (methacrylamido)propyl]-3,4-dihydroxy-9,10-dioxo-2-a nthracenesulfonamide (1.5 mg, 3.38 x 10-6 mole) and α,α'-bis[N-[2-(5,5-dimethyl- borinan-2-yl)benzyl]-N- [3- (meth-acrylamido) propylamine-] -1, 4-xylene (28 mg, 3.54 x 10-5 mole) were combined with 800 uL of ethylene glycol monomer solution and 40 uL of 5% wt. aqueous ammonium persulfate. This formulation was placed in a glove box purged with nitrogen along with a mold constructed from class microscope slides and 100 micron stainless steel spacer. An aqueous solution of N,N,N',N'-tetramethylethylenediamine (40 μL, 5% wt.) was added to the monomer solution to accelerate polymerization and the final formulation was poured into a glass mold. The mold was left under nitrogen atmosphere for 16 hours, after which it was immersed in PBS (pH=7.4) and the glass slides were separated to afford a hydrogel polymer in a form of a thin film. The resulting hydrogel thin film was washed with 100 mL of phosphate buffered saline containing 1 mM lauryl sulfate sodium salt for 3 days the solution being changed every day, followed by washing with MeOH/PBS (20/80 by vol., 3 x 100 mL) , and finally with PBS (pH=7.4, 3 x 100 mL) . Hydrogel polymer was stored in PBS (10 mM PBS, pH=7.4) containing 0.2% wt. sodium azide and 1 mM EDTA sodium salt. F. Modulation of Absorbance With Glucose and Lactate The modulation of the absorbance of the indicator hydrogel (which contains two recognition elements) prepared in this example by glucose and lactate was determined. The acrylamide gel was mounted in PMMA cell in the same way as described in Example 4. Phosphate buffered saline (PBS), pH=7.4 containing desired amount of glucose or sodium lactate was heated to 37°C in a water bath and placed in the PMMA cell containing the gel after which the PMMA c ell was allowed to equilibrate for 15 min at 37°C. Absorbance measurement for each glucose or lactate concentration was conducted in triplicate. For each measurement, absorbance at 650 nm was used as a blank, A(650 nm) was subtracted from all values of A(450nm) and A(530 nm). Figure 6 shows the absorbance spectra for acrylamide gel (30%) containing 4 mM Alizarin Red S monomer and 44 mM bis boronic acid monomer with and without glucose. Figure 7 shows the effect of glucose on absorbance of acrylamide gel (30%) containing 4 mM Alizarin Red S monomer and 4 4 mM bis boronic acid monomer. Figure 8 shows the effect of sodium lactate on absorbance of acrylamide gel (30%) containing 4 mM Alizarin,Red S monomer and 4 4 mM bis boronic acid monomer. The absorbance of the indicator was affected by the presence of glucose, but not substantially affected by the presence of lactate. G. Modulation of Fluorescence With Glucose and Lactate The modulation of the fluorescence of an acrylamide gel synthesized substantially in accordance with this Example 6 (except that 1.9 mg of N-[3-(methacrylamido)- propyl]-3,4-dihydroxy-9,10-dioxo-2-anthracenesulfonamide and 35 mg of α,α'-bis [N-[2-(5,5-dimethylborinan-2-yl)- benzyl]-N-[3-(methacrylamido)propylamino]-1,4-xylene were used) was determined. The experiment was conducted in a Shimadzu RF-5301 PC spectrofluorimeter equipped with a variable temperature attachment (excitation at 470 nm, slits 3/10 nm, high sensitivity). The acrylamide gel was attached to a piece of a glass slide which was glued in a PMMA fluorescence cell at a 5° angle. The cell was filled with 2.5 ml of PBS (pH=7.4) and heated to 37°C. Stock solutions of glucose (1)0 mM and 500 mM) in PBS (pH=7.4) were prepared and heated to 37°C in a water bath. An aliquot of heated glucose stock solution was added to the PMMA cell periodically while the fluorescence intensity at 550 nm was monitored as a function of time (1 measurement every 2 minutes). Glucose concentration in the PMMA cell was measured using a YSI Model 2300 STAT plus glucose analyzer. The results, shown in Figure 9, show that the addition of glucose reduces the fluorescent intensity of the indicator hydrogel. The same effect is seen in Figure 10, which shows the effect of glucose on the fluorescence spectrum of the same type of gel. That effect is beJieved to occur because of the following considerations. The methacrylamide monomer of Alizarin Red S (reporter molecule) contains a vicinal diol functionality and monomer functionality (see structure below). In i.queous solution and in organic solvents, the Alizarin Red S and bis-boronate recognition element monomers (see structure below) are capable of reversible reaction with each other to form a boronate ester. The boronate ester molecule formed in this reversible reaction is fluorescent, while the Alizarin Red S monomer by itself displays virtually no fluorescence emission in aqueous solution and in organic solvents, such as MeOH. Thus upon binding to the glucose recognition element, Alizarin Red S changes its optical properties, such as absorbance and quantum yield of fluorescence, for example. A solution of Alizarin Red S with monomer functionality and glucose recognition element with monomer functionality can be prepared together with a hydrogel monomer and a crosslinker. Copolymerization of this mixture produces a hydrogel material which is diffusable to various small and medium size molecules; thus it is capable of analyte detection and quantitation. An analyte, such as glucose for example, would diffuse inside the hydrogel matrix and displace the reporter molecule previously bound to the recognition element. This event causes a change in the optical properties of the hydrogel film since it now contains a greater number of reporter molecules unbound to the recognition element. The modulation of the fluorescence of the indicator compound (which contains two recognition elements) prepared in this example by glucose and lactate was also determined. The experiment was conducted in a Shimadzu RF-5301 PC spectrofluorimeter equipped with a variable temperature attachment (excitation at 470 nm, slits 5/10 nm, low sensitivity). The acrylamide gel was attached to a piece of a glass slide which was glued in a PMMA fluorescence cell at a 45° angle. The cell was filled with 2.5 ml of PBS (pH=7.4) and heated to 37°C in a water bath. A stock solution of sodium lactate (100 mM) in PBS (pH=7.4) was prepared and heated to 37 °C in a water bath. Stock solutions of glucose (100 mM and 500 mM) in PBS (pH=7.4) were prepared and heated to 37°C in a water bath. An aliquot of heated lactate stock solution was added to the PMMA cell periodically while the fluorescence intensity at 550 ran was monitored as a function of time (1 measurement every 2 minutes), until the lactate concentration reached 8 mM. Then, an aliquot of heated glucose stock solution was added to the PMMA cell periodically while the fluorescence intensity at 550 nm was monitored as a function of time (1 measurement every 2 minutes). Glucose concentration in the PMMA cell was measured using a YSI Model 2300 STAT plus glucose analyzer. The results shown in Figure 11, show that the addition of lactate had no significant effect on the fluorescent intensity of the indicator hydrogel, and the subsequent addition of glucose reduced the fluorescent intensity of the indicator hydrogel. Example 7 Single-methacrylamide monomer of bis-boronate-anthracene: A. 9-chloromethyl-10-[ [2- (2-hydroxyethoxy) ethylamino] - methyl]anthracene hydrochloride salt. To a suspension of 9,10-bis(chloromethyl)anthracene (5.18 g, 18.8 mmole, ,.99 equiv. ) in 200 mL of NMP was added 2-(2-aminoethoxy)ethanol (0.495 g, 0.475 mL, 4.71 mmole) . The mixture was stirred in the dark for 17 hours. At this time, the reaction mixture was concentrated to ~ 50 nL under vacuum at 50°C. The residue was purified by silica gel chromatography (150 g gravity grade silica gel, 0-10% CH3OH/CH2Cl2) to yield 0.425 g (24%) of a yellow/orange solid. TLC: Merck silica gel 60 plates, Rf 0.72 with 70/30 CH2Cl2/CH3OH, see with UV (254/366), ninhydrin stain. HPLC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm column, 0.100 mL injection, 2 mL/min, 370 nm detection, A - water (0.1% HFBA) and B = MeCN (0.1% HFBA) , gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention, time 16.1 min. B. 9-[[2-(2-hydroxyethoxy)ethylamino]methyl]-10-[[(3- methacrylamido) propylamino] methyl] -anthracene. To a suspension of N-(3-aminopropyl)methacrylamide hydrochloride salt (3.33 g, 17.2 mmole, 4.2 equiv.), DIEA (5.19 g, 7.00 mL, 40.1 mmole, 9.8 equiv.) and - 3 mg of BHT in 125 mL CHCl3 at 23°C was added dropwise a solution of 9-chloromethyl-10-[[2-(2-hydroxyethoxy)ethylamino]- methyl]anthracene hydrochloride salt (1.56 g, 4.10 mmole) in 25 mL of CHCl3. The mixture was subsequently stirred in the dark for 92 hours. At this time, the reaction mixture was filtered and washed with 2 x 40 mL of NaHCO3 (saturated aqueous solution). The organic extract was dried over anhydrous Na2SO4, filtered and concentrated to yield a sticky orange solid which was purified by alumina chromatography (50 g activated neutral alumina, 0-5% CH3OH/CH2Cl2) to yield C.364 g (20%) of an orange solid. TLC: Merck silica gel 60 plates, Rf 0.16 with 70/30 CH2Cl2/CH3OH, see with UV (254/366), ninhydrin stain HPLC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm column, 0.100 mL inject ion, 2 mL/min, 370 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B ever 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 16.85 min. C. 9-[N-[2-(5,5-dimethylborinan-2-yl)benzyl]-N-[3- (methacrylamido) propyl amino] methyl] -10- [N- [2- (5,5- dimethylborinan-2-yl)fcenzyl] -N- [2- (2-hydroxyethoxy) - ethylamino] methyl] anti racene. (Single-me thacrylamide monomer) A solution of 9-\|[2-(2-hydroxyethoxy)ethylamino]- methyl]-10-[[(3-methac xylamido)propylamino]methyl]- anthracene (0.343 g, (.763 mmole), DIEA' (0.965 g, 1.30 mL, 9.8 equiv.) and C-bromomethylphenyl)boronic acid neopentyl ester (1.09 g, 3.85 mmole, 5.0 equiv.) in 20 mL CHCl3 at 23°C was stirred in the dark for 25 hours. At this time, the reaction mixture was concentrated initially by rotary evaporation, then using a vacuum pump to remove DIEA. The residue was purified by alumina column chromatography 40 g activated neutral alumina, 0- 10% CH3OH/CH2Cl2) to yield 0.299 g (46%) of a yellow orange solid. This compound may be co-polymerized with a suitable monomer as described previously, deprotected, and used to detect glucose. FAB MS: Calc=d for C51H65B2N3O7 [M]+ 854; Found [M + 1] + 855. TLC: Merck basic alumina plates, Rf 0.35 with 95/5 CH2Cl2/CH3OH, see with UV (254/366) . . HPXC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm column, 0.100 mL injection, 2 mL/min, 370 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 19.7 min. Example 8 Dual-methacrylate monomer of bis-boronate-anthracene A. 9,10-bis [N- [2- (5, 5-dimethylborinan-2-yl)benzyl] -N- [2- (2-methacroyloxyethoxy) ethylamino]methyl] anthracene. A solution of 9,13-bis[N-[2-(5,5-dimethylborinan-2- yl)benzyl]-N-[2-(2-hydroxyethoxy)ethylamino]methyl]- anthracene (0.100 g, 0.120 mmole; see Example 2), methacrylic acid (0.112 g, 0.110 mL, 1.30 mmole, 10.8 equiv.), DCC (0.316 g, 1.53 mmole, 12.8 equiv.) and N,N- dimethylamino-pyridine (0.014 g, 0.11 mmole, 0.92 equiv.) in 5 mL CH2Cl2 was stirred at 0°C fcr 1 hour, then 23°C for 22 hours. At this time, the reaction mixture was filtered and concentre ted by rotary evaporation. The residue was purified by alumina column chromatography (30 g activated neutral alumina, 0-2% CH3OH/CH2Cl2) to yield 0.030 g (26%) of a yellow solid. This compound may be co-polymerized with a suitable monomer as described previously, deprotectetd, and used to detect glucose. FAB MS: Calc=d for C56H70B2N2010 [M]+ 953; Found [M]+ 951 (weak molecular ion peak). TLC: Merck basic alumina plates, Rf 0.67 with 95/5 CH2Cl2/CH3OH, see with UV (254/366). HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column 0.100 mL injection, 0.75 mL/min, 2 mL injection loop, 37) nm detection, A = water (0.1% HFBA) and B = MeCN (0 1.% HFBA) , gradient 10% B 2 min, 10- 80% B over 18 min, 80 -100% B over 2 min, 100% B 2 min, retention time 19.6 min. Example 9 Dual 5-aminopentyl bis-boronate-anthracene A. 9,10-bis [ [5- (t-BOC)-aminopentylamino]methyl]- anthracene. A suspension of 9,10-bis(chloromethyl)anthracene (0.28 g, 1 mmole), DIEA (7.0 mL, 40 mmole), mono-t- butoxycarbonyl 1,5-diaminopentane (3.75 g, 10 mmole), and 50 ml of CHCl3 was stirred in the dark for 2 days at 45°C. The solution was washed with saturated H2O/NaHCO3, the organic phase was dried (Na2SO4), and the solvent was evaporated. The residue was purified by alumina chromatography (40 g activated neutral alumina, 95/5 % vol. CH2Cl2/MeOH) to yield 0.55 g of viscous oil. This material was used as is for the next step. B. 9,10-bis [N- [2- (5,5--dimethylborinan-2-yl)benzyl] -N- [5-(t-BOC)-aminopentylamino]methyl]anthracene. A solution of 9,1)-bis[ [5-(t-BOC)-aminopentylamino]- methyl]anthracene (0.3 g, 0.49 mmole), DIEA (0.35 mL, 2 mmole), and (2-bromome;hylphenyl)boronic acid neopentyl ester (0.566 g, 2.0 mmole) in 20 mL CH2Cl2 was stirred in the dark for 2 days at 25°C. At this time, the reaction mixture was concentrated in vacuo and the residue was purified by alumina chromatography (60 g of activated neutral alumina, 98/2 % vol. CH2Cl2/MeOH) to yield 0.401 g of yellow oil. This material was used as is for the next step. C. 9,10-bis[N-(2-boronobenzyl)-N-[5-aminopentylamino]- methyl]anthracene trifluoroacetic acid salt. 9,10-bis[N-[2- (5, 5-dimethylborinan-2-yl)benzyl]-N- [5-(t-BOC)-aminopentylamino]methyl]anthracene (0.4 g, 0.39 mmole) was dissolved in 20 ml of CH2Cl2/TFA (80/20 % vol.). The solution was stirred for 12 hours, the solvent was evaporated, and the residue was washed with 10 ml of ether. A total of 373 mg of solid was obtained (72% yield). Product was ~80% pure by RP-HPLC. This compound may be co-polymerized with a suitable monomer as described previously, deprotected, and used to detect glucose. HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.050 mL injection, 0.75 mL/min, 360 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 16.0 min. Example 10 A. N-2-(tert-butoxycarbonyl)aminoethyl-4- bromonaphthalene-1,8-dicarboximide: N-t-Boc-ethylened lamine (Fluka, 1.6 g, 10 mmole) and 4-bromo-l,8-naphthalic anhydride (Aldrich, 2.77 g, 10 mmole) were combined with 60 ml of anhydrous ethanol, the suspension was stirred at 60°C for 20 hours, cooled to room temperature, and filtered. The obtained solid was washed with 30 ml of cold EtOH and dried under vacuum. Yield 3.84 g (91%). NMF (CDCl3): 1.28 (9H, s) ; 3.52 (2H, t); 4.35 (2H, t); 4.92 (1H, s);7.84 (1H, t); 8.04 (1H, d) ; 8.42 (1H, d); 8.58 (1H, d); 8.67 (1H, d). B. N-2- (tert-butoxycarbonyl) aminoethyl-4- (N' - methylaminoethylamino)naphthalene-1,8-dicarboximide: N-Methylethylenedlamine (1.48 g, 20 mmole) was combined with 2 ml of --methyl-2-pyrrolidinone (NMP) followed by addition o: N-2-(tert- butoxycarbonyl)aminoethyl-4-bromonaphthalene-l,8- dicarboximide (0.35 g, 0.845 mmole). The resulting solution was stirred at 45°C for 40 hours after which NMP and N-methylethylenediamine were evaporated under vacuum. The obtained residue was subjected to column chromatography (20 g of silica gel, initially CH2Cl2/MeOH (90/10), then CH2Cl2/MeCH/Et3N (75/20/5)). A yellow solid was obtained (0.311 g, 89 % yield). Purity was checked by RP-HPLC. C. N-aminoethyl-4-(N -aminoethylene-N'- [2- (borono)benzyl]methylamino)naphthalene-l, 8- dicarboximide trifluoroacetic acid salt: N-2- (tert-butoxycarbonyl)aminoethyl-4-(N'- methylaminoethylamino; naphthalene-1, 8-dicarboximide (0.3 g, 0.73 mmole), 2-broromethylphenyl boronic acid, pinacol ester (0.6 g, 2 mmole), N,N-diisopropyl-N-ethylamine (1.3 ml, 8 mmole), and 10 nl of CH2Cl2 were combined. The solution was stirred for 20 hours, followed by addition of 2 g of PS-Trisamine resin (Argonaut Technologies, 3.38 mmol/g). The reaction mixture and resin were agitated for 10 hours after which the resin was removed by filtration and washed with CH2Cl2 (2X20 ml) . Combined CH2Cl2 solutions were evaporated and dried under vacuum. Methylene chloride solution containing 20% vol. TFA and 5% vol. triisopropyl silane was added to the resulting orange residue. The resulting solution was stirred at room temperature for 10 hours, after which the solvent was evaporated and the residue triturated with ether to yield a yellow solid. The solid was filtered and dried in vacuum (yield 580 mg). Purity of the material was checked by RP-HPLC. The solid was used as is in the next step. D. N-(3-Borono-5-nitrobenzamido)ethyl-4-(N'- aminoethylene-N' - [2 - (borono)benzyl]methy lamino) naphthalene-1, 8- dicarboximide: N-aminoethyl-4-(N'-aminoethylene-N'- [2-(borono)benzyl]methylamino)naphthalene-1,8- dicarboximide trifluoroacetic acid salt (0.225 g, 0.4 mmole), 3-carboxy-5-nitrophenylboronic acid (0.085 g, 0.4 mmole), diphenylphosphoryl azide (0.13 ml, 0.6 mmole), and 2 ml of anhydrous [MF were combined. N,N- diisopropyl-N-ethyl amine (0.7 ml, 4 mmole) was added and the solution was stirred for 20 hours. Ether (10 ml) was added to the reaction nixture and the insoluble residue was separated and sonicated with 5 ml of CH2Cl2 to yield an orange solid which was filtered and dried under vacuum (38 mg, 15% yield) . Purity of the solid was checked by RP-HPLC. NMR (dmso-d6/020, 90/10): 6 2.32 (3H, s); 2.82 (2H, t); 3.58 (2H, t); 3.65 (2H, t), 3.70 (2H, s); 6.65 (1H, d) ; 7.0-7.3 (4H, m ; 7.68 (1H, t) ; 8.18 (1H, d) ; 8.42 (1H, d); 8.47 (1H, d); 8.1-8.35 (3H, m) . E. Test of N- (3-borono-5-nitrobenzamido) ethyl-4-(N' - aminoethylene-N' ' - [2- (borono)benzyl]mettylamino) naphthalene-1,8- dicarboximide for interaction with glucose as monitored by fluorescence This experiment was conducted in MeOH/phosphate buffered saline, (PBS, 10 mM, pH=7.4). The concentration of N-(3-borono-5-nitrobenzamido)ethyl-4- (N' - aminoethylene-N'- [2- (borono) benzyl]methylaimino) naphthalene-1, 8-dicarboximide in MeOH/PBS, (50/50 vol. %) was 15 M. The glucose concentration was vared from 0 mM to 50 mM, and the L- sodium lactate concentration was varied from 0 mM to 7 mM. The experiment was conducted in a Shimadzu RF-5301 PC spectrofluorimeter excitation wavelength was set at 430 nm, emission was monitored in the 480-650 nm range, slit width 3/1.5 nm, high sensitivity of PMT. The results are shown in Figures 12 and 13, which show that the fluorescence of the indicator of this example was affected by the presence of glucose, but not by the presence of lactate. Example 11 6-(Cyclohexanecarboxamido)hexylamine indicator monomer A. 9- [N- [3- (methacrylamido)propylamino]methyl] -10-N- [(6-aminohexylamino)methyl]anthracene. To a solution of 3-aminopropylmethacrylamide (0.775 g, 5.45 mmol, 10.0 equiv.) and tert-butyl N-(6-aminohexyl)carbamate (1.18 g, 5.45 mmol, 10.0 equiv.) and several crystals of BHT in 200 mL CHCl3 was added 9,10-bis(chloromethyl)anthracene (0.150 g, 0.545 mmol). The reaction mixture was subsequently stirred in the dark at ambient temperature for 4 days. At this time, the CHCl3 was evaporated and the residue was dissolved in 100 mL ether. The organic layer was extracted w: th 8 x 125 mL sat'd aqueous NaHCO3 • and 5 x 200 mL phosphite buffer (0.4 M, pH 7.0). The pH of the combined phosphate buffer washes was adjusted to pH 11 by addition of Na2CO3 (sat'd aqueous solution), followed by extraction with 5 x 300 mL CH2Cl2. The combined organic layers were concentrated and the residue dissolved in 5 mL of 1 20% solution of TFA in CH2Cl2. The mixture was stirred at ambient temperature for 2 hours. At this time, the reaction mixture was extracted with 4 x 10 mL sat'd aqueous NaHCO3. The pH of the combined aqueous layers was adjusted to pH 11 by addition of Na2CO3 (sat'd aqueous solution), followed by extraction with 4 x 75 mL CH2Cl2. The combined organic extracts were dried over anhydrous Na2SO4, filtered and concentrated in vacuo to yield 0.068 g (27%) of product. TLC: a) Merck Silica Gel 60 plates, Rf 0.16 with 70/30 CH2Cl3/CH3OH, see with UV (254/366), prior to deprotection; Rf 0.27 with 85/14.5/0.5 CH2Cl2/CH3OH/iPrNH2, see with UV (254/366), final product. HPLC: HP 1100 HI L.C chromatograph, Waters 8 x 100 mm NovaPak HR C18 column, 0.100 mL injection, 0.75 mL/min, 0.400 ml injection loop, 360 nm detection, A = water (0.1% HNBA) and B = MeCN (0.1% HFBA) , gradient 10% B : min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 15.5 min. B. 9- [N- [3- (methacrylamido)propylamino]methyl] -10- [N- [6- (cyclohexanecarboxamido) hexylamino]methyl] anthracene. To a solution of 9-[N-[3- (methacrylamido)propylamino]methyl]-10-N-[6- aminohexylamino)methyl]anthracene (1.68 g, 3.63 mmol) and a few crystals of EHT in 20 mL CH2Cl2 at ambient temperature was adc ed dropwise a solution of cyclohexanecarboxy.'.ic acid N-hydroxysuccinimide ester (0.845 g, 3.76 mmo., 1.03 equiv.) over a 1 hour period. The reaction was subsequently stirred in the dark at ambient temperature for 16 hours. At this time, the reaction mixture was concentrated in vacuo and the residue dissolved in 105 mL of a solution of 90/15 ether/ CH2Cl2. The organiC layer was extracted with 4 x 225 mL phosphate buffer ,0.4 M, pH 7.0). The pH of the combined phosphate buffer washes was adjusted to pH 11 by addition of Na2CO3 (sat'd aqueous solution), followed by extraction with 6 x 500 mL CH2Cl2. The combined organic layers were dried over anhydicus Na2SO4, filtered and concentrated in vacuo to yield 1 2 g (60%) of product. TLC: Merck Silica Gel 60 plates, Rf 0.30 with 85/14.5/0.5 CH2Cl2/CH3OH/iPrNH2, see with UV (254/366) HPLC: HP 11)0 HPLC chromatograph, Waters 8 x 100 mm NovaPak HR 318 column, 0.100 mL injection, 0.75 mL/min, 0.4 30 mL injection loop, 360 nm detection, A - water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% C. 9-[N-(2-boronobenzy][-N-[3- (methacrylamido) propylamine]methyl] -10- [N- (2- boronobenzyl) -N- [6-(cyclohexanecarboxamido) hexylamino] - methyl] anthracene. A solution of 9-[N-[3- (methacrylamido)propylamino]methyl] -10-[N-[6- (cyclohexanecarboxamido)hexylamino]methyl]-anthracene . (1.0 g , 1.8 mmol), DIEA (1.81 g, 2.44 mL, 14.0 mmol, 7.8 equiv.), 2-bromomethylphenylboronic acid pinacol ester (2.14 g, 7.20 mmol, 4.( equiv.) and a few crystals of BHT in 30 mL CHCl3 was stirred in the dark at ambient temperature for 60 hours. At this time, the reaction mixture was concentrated and the residue (9-[N-[2- (4,4,5,5,-tetramethyl-: ,3,2-dioxaborolano)benzyl]-N-[3- (methacrylamido)propylamino] methyl] -10-[N-[2-(4,4,5,5,- tetramethyl-1, 3, 2-dioxaborolano) benzyl] -N- [ 6- (cyclohexanecarboxamide) hexylamino]methyl]anthracene) suspended in 150 mL ether. The organic layer was washed with 4 x 50 mL phosphate buffer (0.4 M, pH 7.0). The organic layer was concentrated and the residue dissolved in ether in 200 mL 0.1 N aqueous HCl. The aqueous layer was washed with 3 x 50 ml. 1:1; ether: ethyl acetate and the pH was adjusted to pK 11 by addition of Na2CO3 (sat'd aqueous solution), followed by extraction with 3 x 150 mL CH2Cl2. The combined organic layers were dried over anhydrous Na2SO4, filtered and concentrated in vacuo to yield a red oily compound. The residue was dissolved in ether and concentrateD in vacuo to yield 1.17 g (85%) of a yellow solid product, D. N,N-dimethylacrylamide hydrogel with 9-[N-(2- boronobenzyl) -N- [3- (methacrylamido) propylamino]methyl] - 10- [N- (2-boronobenzyl)- N- [6- (cyclohexanecarboxamide)hexylamino] methyl]anthracene. A solution of N,N-dimethylacrylamide (40% wt.) and N,N'- methylenebisacrylamide (0.8% wt.) in phosphate buffer, pH=7.4, 200 mM was prepared. 9-[N-(2-Boronobenzyl)-N-[3- (methacrylamido) propylamino]methyl] -10- [N- (2- boronobenzyl)-N-[6-(cyclohexanecarboxamido)hexylamino] methyl] anthracene (18 mg, 2.15X10-5 mole) and 60 mg of fructose were combined with 2 mL of MeOH. This solution was sonicated until all of the fructose dissolved and was subsequently evaporatec to yield a solid. To this solid, 1 mL of phosphate buffer solution containing monomers was added. After sonicaticn for 10 min this solution was filtered through a 0.2 uM PTFE membrane filter. Aqueous ammonium persulfate (2C μL, 5% wt.) was combined with the formulation. The resulting solution was placed in glove box purged with nitrogen. An aqueous solution of N,N,N',N'-tetramethylethylenediamine (40 μL, 5% wt.) was added to the monomer formulation to accelerate polymerization. The resulting formulation was poured into a mold constructec from glass microscope slides and a 100 uM stainless steel spacer. After being kept for 8 hours in a nitrogen atmosphere, the mold was placed in phosphate buffered saline (pH=7.4), the microscope slides were separated, and the hydrogel was removed. The hydrogel was washed with 100 mL of phosphate buffered saline (PBS) containing 1 mM lauryl sulfate sodium salt and 1 mM EDTA tetrasodium salt for 3 days, the solution being changed every day, followed by washing with EtOH/PBS (20/80 by vol , 3 x 100 mL), and finally with PBS (H=7.4, 3 x 100 mL. The resulting hydrogel film was stored in PBS (pH=7.4) containing 0.02% wt. sodium azide and 1 mM EDTA tetrasod: um salt. E. Modulation of Fluorescence with Glucose. The modulation of the fluorescence of the 6- (cyclohexanecarboxamido)hexylamine indicator/DMA hydrogel film prepared in this example by glucose and lactate was determined. Figure 14 shows the relative fluorescence emission (I @ 430 nm) of the hydrogel film in PBS (pH 7.4 containing 0.02% NaN3 and 1 mM EDTA) containing 0 to 20 mM α-D-glucose, 0 to 10 mM I-sodium lactate, and 0-20 mM α- D-glucose in the presence of 4 mM L-sodium lactate. The hydrogel film (100 μM thickness, 8 mm diameter disk) was mounted in a PMMA cuvette at a 45° angle. All measurements were made at 37°C in a Shimadzu RF-5301 spectrofluorometer with excitation at 370 nm (slit = 3 nm) and emission at 4 30 nm (slit = 3 nm) at low PMT sensitivity. Glucose and L-sodium lactate concentrations were checked using the YSI Model 2300 STAT plus glucose analyzer. Error bars are standard deviation with triplicate values for each data point. The fluorescence was affected by the presence of glucose, but not by the presence of lactate. Moreover, the presence of lactate (4 mM) had no significant effect on the 0-20 mM glucose calibration curve. EXAMPLE 12 2-(carboxyethyl)amine indicator monomer Chemical Name: 9- N-(2-boronobenzyl)-N-[3- (methacrylamido)propylamino]methyl]-10-[N-(2- boronobenzyl)-N-[2 - (carboxyethyl)amiro]methyl]anthracene (uncapped) Chemical Formula: C40H45B2N3O7 MW: 701.4 Physical appearance: faint yellow powder Solubility: PBS/methanol, methanol, ethanol, chloroform, dichloromethane Capped Indicator: 9-[N-[2-(4,4,5,5,-tetramethyl- 1, 3, 2-dioxaborolano)benzyl]-N-[3- (methacrylamido)propylamino]methyl] -10-[N-[2- (4,4,5,5,-tetramethyl-1,3,2-dioxaborolano)benzyl]-N- [2-(carboxyethyl)amino]methyl]anthracene. I. Synthesis A. 9-[N-[3-(methacrylamido)propylamino]methyl]-10-[N- [2- (tert-butoxycarbonyl)ethylamino]methyl]anthracene. To a solution of 3-aminopropylmethacrylamide (12.9 g, 90.7 mmol, 4.99 equiv.), β-alanine tert-butyl ester (13.2 g, 90.9 mmol, 5.00 equiv.] and several crystals of BHT in 700 mL CHCl3 was added 9, 10-bis(chloromethyl)anthracene (5.00 g, 18.2 mmol). The reaction mixture was subsequently stirred in the dark at 30 °C for 88 hours. At this time, the CHCl2 was evaporated and the residue was dissolved in 500 mL ether. The solution was stirred for 1 hour at which time salts had precipitated from solution. The ether solution was filtered and subsequently extracted with 10 x 350 mL sat'd aqueous NaHCO3. The ether layer was further extracted with 6 x 350 mL phosphate buffer (0.2 M, pH 6.5). The pH of the combined phosphate buffer washes was adjusted to pH 11-12 by addition of Na2CO3 (sat'd aqueous solution), followed by extraction with 6 x 500 mL CH2Cl2. The combined organic layers were dried over anhydrous Na2SO4, filtered and concentrated in vacuo to yield an oily crude product. The crude product was purified by silica gel chromatography (50 g flash grade silica gel, 0-5% MeOH/CH2Cl2 step gradient) to yield 2.04 g of a sticky yellow solid (23%). TLC: Merck Silica Gel 60 plates, Rf 0.29 with 90/10 CH2Cl2/CH3OH, see with UV (254/366) and ninhydrin stain. HPLC: HP 1100 HPIC chromatography Waters 5 x 100 mm NovaPak HR C18 column, 0.100 mL injection, 0.75 mL/min, 1.500 ml injection loop, 280 nm detection, A - water (0.1% HEBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100 % B 2 min, retention time 17.0 min. B. 9-[N-[2-(4,4,5,5 -tetramethyl-1,3,2- dioxaborolano)benzyl] • N-[3- (methacrylamido)propy: amino] methyl] -10-[N-[2- (4,4,5,5,- tetramethyl-1,3,2-dioxaborolano) benzyl] -N- [2- (tert- butoxycarbonyl) ethylamino]methyl] anthracene. A solution of 9-[N-[3- (methacrylamido)propyl amino] methyl]--10-[N-[2-(tert- butoxycarbonyl)ethylamino)methyl]anthracene (1.5 g , 3.1 mmol), DIEA (3.16 g, 4.26 mL, 24.4 mmol, 7.9 equiv.), 2- bromomethylphenylboronic acid pinacol ester (3.64 g, 12.2 mmol, 3.9 equiv.) and a few crystals of BHT in 50 mL CHCl3 was stirred in the dark at ambient temperature for 16 hours. At this time, the reaction mixture was concentrated and the residue suspended in 200 mL ether. The ether layer was extracted with 3 x 125 mL phosphate buffer (0.2 M, pH 7.0) dried over anhydrous Na2SO4, filtered and concentrated in vacuo to yield a crude product.The residue was triturated with hexanes to yield 2.14 g (76%) of a white solid. HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.200 mL injection, 0.75 mL/min, 1.500 mL injection loop, 280 nm detection, A = water (0.1% HFBA)- and B = MeCN (0.1% HFBA) , gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 10C% B 2 min, retention time 19.2 min. C. 9-[N-(2-boronobenzyl)-N-[3- (methacrylamido) propylamino] methyl] -10- [N- (2- boronobenzyl) -N- [2- (curboxyethyl) amino]methyl] anthracene. A solution of 9-[N-[2 -(4,4,5,5,-tetramethyl-1,3, 2- dioxaborolano)benzyl] -N-[3- (methacrylamido)propylamino]methyl]-10-[N-[2- (4,4,5,5,- tetramethyl-1,3,2-dioxaborolano)benzyl]-N-[2-(tert- butoxycarbonyl)ethylamino]methyl]anthracene (0.294 g, 0.319 mmol) in 5 mL of 20% TFA/CH2Cl2 was stirred in the dark at ambient temperature for 22 hours. At this time, the reaction mixture was concentrated and the residue triturated with ether. The residue was dissolved in 5 mL 90:10 acetone/water and stirred for 2 hours. At this time, the reaction mixture was concentrated and the residue triturated with water and PBS (pH 7.4 containing 0.02% NaN3 and 1 mM EDTA) resulting in the recovery of 0.062 g (28%) of a light yellow solid. HPLC: HP 1100 HFLC chromatography Waters 5 x 100 mm NovaPak HR C18 column, 0.100 mL injection, 0.75 mL/min, 1.500 mL injection loop, 280 nm detection, A = water (0.1% HF3A) and B = MeCN (0.1% HFBA) , gradient 10% B 2 rain, 10-80% B over 18 min, 80-100% B over 2 min, 10) % B 2 min, retention time 17.4 min. FAB MS: Glycerol matrix; Calc'd for C46H53B2N3O7 (bis glycerol adduct) [M] + 813; Found [M + 2]+ 815. D. N,N-dimethylacrylamide hydrogel with 9-[N-(2- boronobenzyl) -N- [3- (methacrylamido)propylamines] methyl] - 10- [N- (2-boronobenzyl; -N- [2- (carboxyethyl)amino]methyl]anthracene. A solution of N,N-dimethylacrylamide (40% wt.) and N,N'- methylenebisacrylamide (0.8% wt.) in phosphate buffer, pH=7.4, 200 mM was prepared. 9-[N-(2-boronobenzyl)-N-[3- (methacrylamido)propyl amino]methyl]-10-[N-(2- boronobenzyl)-N-[2-(carboxyethyl)amino]methyl]anthracene (14 mg, 2.0 x 10-5 mole ) and 60 mg of fructose were combined with 2 ml of MeOH. This solution was sonicated until all fructose disolved and evaporated to yield a solid. To this solid . ml of phosphate buffer solution containing monomers was added. After sonication for 10 minutes this solution was filtered through 0.2 μM PTFE filter. Aqueous ammonium persulfate (20 μL, 5% wt.) was combined with the formaLation. The resulting solution was placed in a glove box purged with nitrogen. An aqueous solution of N,N,N',N'-tetrametylethylenediamine (40 μL, 5% wt.) was adied to the monomer formulation to accelerate polymerization. The resulted formulation was poured in a mold constructed from microscope slides and 100 μM stainless steel spacer. After being kept for 8 hours in nitrogen atmosphere the mold was placed in phosphate buffered sa]ine (10 mM, pH=7.4), the microscope slides were separated, and the hydrogel was removed. The hydrogel was washed with 100 ml of phosphate buffered saline (PBS) containing 1 mM lauryl sulfate sodium salt and 1 mM EDTA tetrasodium salt for 3 days, the solution being changed every day, followed by washing with EtOH/PBS (20/80 by vol ., 3 x 100 ml), and finally with PBS (pH=7.4, 3 x 100 ml). The resulting hydrogel film was stored in PBS (10 mM, pH=7.4) containing 0.02% wt. sodium azide and 1 mM EDTA tetrasodium salt. II. Modulation of Fluorescence with Glucose. The modulation of the fluorescence of the 2- (carboxyethyl)amine indicator/DMA hydrogel film prepared in this example by glucose and lactate was determined. Figure 15 shows the relative fluorescence emission (I @ 430 ran) of the hydrogel film in P3S (pH 7.4 containing 0.02% NaN3 and 1 mM EDTA) containing 0 to 20 mM α-D-glucose, 0 to 10 mM L- sodium lactate, and 0-20 mM glucose in the presence of 3 mM L-sodium lactate. The hydrogel film (100 μm thickness, 8 mm diameter disk) was mounted in a PMMA cuvette at a 4 5° angle. All measurements were made at 37°C in a Shimadzu RF- 5301 spectrofluorometer with excitation at 370 nm (slit = 3 nm) and emission at 430 nm (slit = 3 nm) at low PMT sensitivity. Glucose and L-sodium lactate concentrations were checked using the YSI Model 2300 STAT plus glucose analyzer. The data is plotted as the average of triplicate values for each data point. The fluorescence was affected by the presence of glucose, but not by the presence of lactate. Moreover, the presence of lactate (4 mM) had no significant effect or the 0-20 mM glucose calibration curve. EXAMPLE 13 Fluorescent glucose indicator containing two detectable moieties: Chemical Name: 9-[N-( 2-boronobenzyl)-N-[3- (methacrylamido)propylamino]methyl]-10-[N-(2- boronobenzyl)-N-[3-(N-6-(9- anthracenecarboxamido hexylamino carbonyl) ethylamino]methyl] anthracene (uncapped) Chemical Formula: C73H17B2N507 MW: 1168 Physical appearance: Paint yellow powder Solubility: PBS/methanol, methanol, ethanol, chloroform, dichloromethane Pinacol capped compound: 9-[N-[2- (4,4,5,5,-tetramethyl-1,3,2- dioxaborolano)benzyl] - N-[3- (methacrylamido)propyl amino]methyl]-10-[N-[2-(4,4,5,5,- tetramethyl-l,3,2-dioxaborolano)benzyl]-N-[3-(N-6-(9- anthracenecarboxamido)hexylamino carbonylethylaminomethyl]anthracene. A. 9-Anthracencyl Chloride: Anthracene-9- carboxylic acid (1.2 g, 5.4xl0~3 mole) was combined with 15 ml of thionyl chloride. The solution was refluxed for 2 hours followed by evaporation of the volatile components. The obtained solid was dried under high vacuum for 24 hours yielding 1.3 g of material (quantitative yield). This material was used as is in the next step. B. N- (6-Aminohexyl) -anthracene-9-carboxamide hydrochloric acid salt: 9-Anthracenoyl chloride (1.3 g, 5.4 mmole) in 50 ml cf anhydrous CH2Cl2 was added dropwise to 11.6 g of hexamethylenediamine (100 mmole) in 100 ml of CH2Cl2 at 0°C. The solution was stirred at 0°C for 1 hour then allowed tc warm to room temperature and stirred overnight. The solvent was evaporated and 200 ml of water was added to the residue. This mixture was sonicated and stirred for 1 hour then filtered. The filtered solid was cried under vacuum for 24 hours. MeOH (50 ml) and 2 ml of conc. HC1 was added to the solid, followed by evaporation of MeOH. The resulting solid was washed with hot CH2Cl2/MeOH (90/10 vol. %) and recrystallized from MeOH, yielding 0.51 g of the product (26%). The purity of the product was checked by HPLC. HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm NovaPak HR C18 colunr, 0.1 mL injection, 0.75 mL/min flowrate, 2 mL injection loop, 280 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA) , gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100 % B 2 min, retention time 16.5 min. C. 9-[N-[2-(4,4,5,5,-tetramethyl-1,3,2- dioxaborolano)benzyl] -N- [3- (methacrylamido)propylamino]methyl] -10- [N-[2- (4,4,5,5,- tetramethyl-1,3,2-dioxaborolano) benzyl] -N-[3- (N-6- (9- an thracenecarboxamido) hexylamino caxbonylethylaminomethjl]anthracene : 9-[N-[2-(4,4,5,5,-tetramethyl-1,3,2- dioxaborolano) benzyl] -N-[3- (methacrylamido) propylamino] methyl] -10-[N-[2-(4,4,5,5,- tetramethyl-1,3,2-dioxaborolano) benzyl] -N- [2- carboxyethylamino]methyl]anthracene (40 mg, 4.5xl0-5 mole) was combined with N-(6-aminohexyl)-anthracene-9- carboxamide hydrochloric acid salt (20 mg, 5.6xl0-5 mole), diphenylphosphoryl azide (15.4 mg, 5.6xl0-5 mole), and 2 ml of DMF. Diisopropylethylamine(39 20 μL, 2.44xl0-4 mole) was added to the mixture and the solution was stirred at room temperature for 24 hours. The DMF was evaporated under high vacuum, the residue was dissolved in 50 ml of EtOAc and washed with water (3x10 ml). The EtOAc solution was separated, dried (Na2SO4) , and evaporated producing 6 mg of solid (87 % yield). Purity of the material was checked by HPLC. HPLC: HP 1100 HP] C chromatograph, Waters 5 x 100 mm NovaPak HR C18 column, 0.1 mL injection, 0.75 mL/min flowrate, 2 mL injection loop, 280 nm detection, A = water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min, retention time 20.42 min. FAB mass-spectrum, glycerol matrix: calculated for C67H75B2N509 (bis glycerol adduct) [M]+=1116, found [M+l]+=1117. II . Effect of glucose on fluorescence of indicator immobilized in hydroge.. film Preparation of HEMA/Methacrylic acid hydrogel with glucose indicator: A 50 % wt. solution of 2-hydroxyethylmethacrylate(4.75 g) and methacrylic acid ((.25 g) in phosphate buffer, pH=7.4, 200 mM was prepared. Glucose indicator (11 mg, 1.0 x 10-5 mole) and 60 rag of fructose were combined with 2 ml of MeOH. This solution was sonicated until all fructose dissolved and evaporated to yield a solid. To this solid 1 ml of phosphate buffer solution containing monomers was added. After sonication for 10 minutes this solution was filtered through 0.2 μM PTFE filter. Aqueous ammonium persulfate (20 μL, 5% wt.) was combined with the formulation. The resulting solution was placed in a glove box purged with nitrogen. An aqueous solution of N,N,N',N'-tetramethylethylenediamine (40 μL, 5% wt.) was added to the monomer formulation to accelerate polymerization. The resulting formulation was poured in a mold constructed from microscope slides and a 100 μM stainless steel spacer. After being kept for 8 hours in a nitrogen atmosphere the mold was placed in phosphate buffered saline (10 mM, pH=7.4), the microscope slides were separated, and the hydrogel was removed. The hydrogel was washed with 100 ml of phosphate buffered saline (PBS) containirg 1 mM lauryl sulfate sodium salt and 1 mM EDTA tetrasocium salt for 3 days, the solution being changed every day, followed by washing with EtOH/PBS (20/80 by vol., 3 x 100 ml), and finally with PBS (pH=7.4, 3 x 100 ml). The resulting hydrogel film was stored in PBS (10 mM, pH=7.4) containing 0.02% wt. sodium azide and 1 mM EDTA tetrasodium salt. Effect of glucose and L-sodium lactate on hydrogel film containing glucose indicator. The experiment was conducted in a Shimadzu RF-5301 PC spectrofluorimeter equipped with a variable temperature attachment. Excitation wavelength was set at 370 nm,slits 3/3 nm, low PMT sensitivity, emission was scanned from 400 to 600 nm. Glucose and L-sodium lactate concentrations were checked using YSI Model 2300 STAT plus glucose analyzer. The hydrogel filn (100 μm thickness, round shape - 8 mm diameter) was mounted in a PMMA cuvette at 45° angle. Phosphate buffered saline (PBS), pH=7.4 containing the desired amount of glucose, L-sodium lactate, and glucose with L-sodium lactate were heated to 37 °C in a water bath and placed in the PMMA cell containing the mounted hydrogel. After each addition the PMMA cell was allowed to equilibrate for 45 min at 37°C. Fluorescence intensity measurements for each glucose/lactate concentration were conducted on two different samples and an average value was used in the calibiation curve. Calibration curves (Fluorescence Intensity at 430 nm vs. concentration) were obtained for glucose L-sodium lactate, and glucose in the presence of 3 mM L-sodium lactate. The results are shown in Figure 16. EXAMPLE 14 6-(3-carboxypropiolamido)hoxylamino indicator monomer Pinacol capped compound: 9- [N-[2- (4,4,5,5,-tetramethyl-1,3,2- dioxaborolano)benzyl] -N-[3- (methacrylamido)propylamino]methyl]-10-[N-[2-(4,4,5,5,- tetramethyl-1,3,2-dioxaborolano)benzyl]-N-[6-(3- carboxypropionamido)hexylamino]methyl]anthracene. Uncapped compound: 9-[N-(2-boronobenzyl)-N-[3- (methacrylamido) propylamino]methyl] --10- [N- (2- boronobenzyl)-N-[6-(3- carboxypropionamido)hexylamino]methyl]anthracene. Synthesis: The synthesis may be carried out in an analogous fashion to Example 11 using 9-[N-[3- (methacrylamido)propylamino]methyl]-10-N-[6- (hexylamino)methyl]anthracene as the starting material. In contrast, the amine starting material is reacted with the N-hydroxysuccinimide (NHS) ester of the mono methyl ester of succinic acic in place of the NHS ester of cyclohexanecarboxylic acid used in Example 11. An additional base hydrolysis step is required to complete the synthesis. Chemical Name: N-(3-Methacrylamidopropyl)-4-[2-N-[[2- (borono)benzyl]-[6-(N- [2-(borono)benzyl]-6-N- (3- carboxypropanamidoethyl)aminohexyl]]aminoethylamino]napht halene-1,8-dicarboximide Chemical Formula: C47H60B2N6O10 M. W.: 890 The compound may be synthesized as shown below: EXAMPLE 16 Alternate glucose indicator/monomer excited with visible light Chemical Name: N-Butyl -4-- [2-N- [ [2- (borono) benzyl] - [ 6- (N- [2-(borono)benzyl]-6-N- (2- methacrylamidoethyl)aminohexyl]] aminoethylamino] naphthale ne-1,8-dicarboximide Chemical Formula: C44H51B2N5O7 M. W. : 789.5 The compound may be synthesized as shown below: WE CLAIM: 1. A method for detecting the presence or concentration of glucose in a sample which may also contain an alpha-hydroxy acid or a beta-diketone, which comprises: a) exposing the sample tc a compound having at least two recognition elements for glucose, oriented such that the interaction between the compound and glucose is more stable than the interaction between the compound and the alpha-hydroxy acid or beta-diketone, said con pound also containing a detectable moiety having a detectable quality that changes in a concentration-dependent manner when said compound is exposed to glucose in said sample; and b) measuring any change in said detectable quality to thereby determine the presence or concentration of glucose in said sample, wherein the preserce of the alpha-hydroxy acid or the beta-diketone does not substantially interfere with said determination, wherein the compound is selected from the group consisting of: 9-[N-(2-boronobenzyl) -M-[3-(methacrylamido) propyl amino ] methyl] -10-\|N-(2-boronobenzyl)-N-[6-(cyclohexanecarboxamido) hexylamino]methylanthracene; 9-[N-(2-boronobenzyl) -N-[3-(methacrylamido)propyl ami no ] - methyl ] -10- [ N- (2-boronobenzyl ) -N- [2- (carboxyethyl ) amino ) methyl ] - anthracene; 9-[N-(2-boronobenxyl) -N-[3-(methacrylamido)propyl amino]- methyl ]-10-[N-(2-boronobenzyl)-N-[3-(N-6-(9-anthracenecarbox- amido)hexylamino carbonyl) ethylamino]methyl ] anthracene; 9-[N-(2-boronobenzyl) -M-[3-(methacrylamido)propylamino]- methyl ]-10-[N-(2-boronobenzyl)-N-[6-(3-carboxypropionamido)- hexylamino ] methyl ] anthracene ; N-(3-Methacrylamidoprocpyl)-4-[2-N-[[2-(borono)benzyl]-[6- (N-\|2-(borono)benzyl]-6-N- (3-carboxypropanamidoethyl) aminohexyl ] ]-aminoethylamino ] naphthalene-1, 8-dicarboximide; N-Butyl-4-[2-N-[[ 2- (borono) benzyl]- [-6- (N-[2- (borono) benzyl]-6-N-(2-methacrylaridoethyl)aminohexyl]]aminoethylamino]- naphthalene-1 , 8-dicarboximide; and salts thereof. 2. The method as claimed in claim 1,. wherein the sample is a physiological fluid . 3. The method as claimed in claim 2, wherein the physiological fluid is selected from the group consisting of blood, plasma, serum, interstitial fluid, cerebrospinal fluid, urine, saliva, intraocular fluid, lymph, tears, sweat, and physiological buffers. 4. The method as claimed in claim 1, wherein the compound is exposed to the sample in solution. 5. The method as claimed in claim 1, wherein the compound is immobilized on or within a solid support. 6. The method as claimed in claim 5, wherein the solid support is a polymeric matrix. 7. A compound selected from the group consisting of: 9- [N- (2-boronobonzyl) -N- [3 - methacrylamido) propylamine-] methyl] - 1 0- [N- (2-boronobenzyl ) -N- [ 6- (cyclohexanecarboxamido) hexylamino] methyl ] anthracene; 9-[N-(2-boronobenzyl -N-[3-(methacrylamido)propylamino]- methyl ]- 10-\|N-(2-boronobenzyl)-N-[2-(carboxyethyl)amino]methyl]- anthracene; 9-[N- (2-boronobenzyl)-N-[3-(methacrylamido)propylamino]- methyl]-10-[N-(2-boronobenzyl)-N-[3-(N-6-(9-anthracenecarbox- amido) hoxylamino carbonyl) ethyl amino] methyl] anthracene; 9- ( N- (2-boronobenzyl) -N-- [3- (methacrylamido) propylamino] - methyl ]-10-[N- (2-boronobenzyl)-N-[ 6-(3-carboxypropionamido)- hexylamino ] methyl] anthracene; N-(3-Methacrylamidopropoyl)-4-[2-N-[ 2-(borono)benzyl]-[6- (N-[2-(borono)benzyl]-6-N-(3-carboxypropanamidoethyl) aminohexy 1 \| ] -aminoethylamino] naphthalene-1, 8-dicarboximide; N-Butyl-4-[2-N-[[2-(borono)benzyl]-\|6-(N-[2-(borono) benzy 1 ) -6-N- (2-methacrylamidioethyl) aminohexyl] ] aminoethyl amino] - naphthalene-1,8-dicarboximide; and salts thereof. Compositions and methods for determining the presence or concentration of glucose in a sample which may also contain an alpha-hydroxy acid or a beta-diketone.The method uses a compound having at least two recognition elements for glucose, oriented such that the interaction between the compound and glucose is more stable than the interaction between the compound and the alpha-hydroxy acid or beta-diketone, such that the presence of the alpha-hydroxy acid or the beta-diketone does not substantially interfere with said determination.

Full Text

TITLE CF THE INVENTION
DETECTION OF GLUCOSE IN SOLUTIONS ALSO CONTAINING
AN ALPHA-HYDROXY ACID OR A BETA-DIKETONE
CROSS-REFERENCE TO RELATED APPLICATIONS
The present application is a continuation-in-part of
application Serial No. ]0/029,184 filed December 28,
2001, which is a contimation-in-part of application
Serial No. 09/754,217 filed January 5, 2001 and claims
the benefit of application Serial No. 60/363,885 filed
March 14, 2002, application Serial No. 60/329,746 filed
October 18, 2001 and application Serial No. 60/269,887
filed February 21, 2001.
STATEMENT REGARDING FEDERALLY SPONSORED
RESEARCH OR DEVELOPMENT
Not applicable.
BACKGROUND D OF THE INVENTION
1. Field of the Invention
The present invention relates to the detection of
glucose in samples which ray also contain potential
interfering compounds, Such as α-hydroxy acids or (3-
diketones.
2. Description of the Related Art
The complexation of carbohydrates, including glucose,
with phenylboronic acid las been known for a long time
and the reversibility of that interaction has served as a
basis for the chromatographic separation of sugars.

Specifically, in 1959, Iorand and Edwards reported
association constants fcr aqueous associations of
phenylboronic acid with many saturated polyols; binding
interactions ranged fron very weak (e.g., ethylene
glycol, Kd=360 mM) to moderately strong (e.g., glucose,
Kd=9.1 mM) . See J. Yoon, et al., Bioorganic and Medicinal
Chemistry 1(4):267-71 (3993). The binding mechanism is
believed to occur throuch bonding of adjacent hydroxyl
groups on glucose to hycroxyl groups on a boronate
moiety.
U.S. Patent '5,503,773 (James, et al.) describes a
fluorescent boronic acid-containing compound that emits
fluorescence of a high intensity upon binding to
saccharides, including glucose. The fluorescent compound
has a molecular structure comprising a fluorophore, at
least one phenylboronic acid moiety and at least one
amine-providinig nitrogex atom where the nitrogen atom is
disposed in the vicinity of the phenylboronic acid moiety
so as to interact intramolecularly with the boronic acid.
Such interaction thereby causes the compound to emit
fluorescence upon saccharide binding. See also T. James,
et al., J. Am. Chem. Soc. 117(35):8982-87 (1995).
Additionally, fluorescent sensors using an
anthrylboronic acid-containing compound for detecting
blood glucose are known in the art. For example, J.
Yoon, et al., J. Am. Chum. Soc. 114:5874-5875 (1992)
describe that anthrylboronic acid can be used as a
fluorescent chemosensor for signaling carbohydrate
binding, including binding of glucose and fructose.
Unfortunately, compounds which interact with glucose
in the manner described above also have a tendency to
interact with other compounds having hydroxyl groups,
thus reducing the specilicity of a glucose assay,
especially when assaying physiological samples which may

contain interfering amounts of lactate, acetoacetate,
etc. For example, some diabetic patients also develop
lactic acidosis, in which blood lactate levels are
greater than 5 mmol/liter. Thus, there remains a great
need for glucose assays which are relatively insensitive
to potentially interfering hydroxyl compounds, such as.
lactate.
BRIEF SUMMARY OF THE INVENTION
In one aspect, the present invention is directed to a
method for detecting the presence or concentration of
glucose in a sample which may also contain an α-hydroxy
acid or a β-diketone, which comprises:
a) exposing the sample to a compound having at least
two recognition elements for glucose, oriented such that
the interaction between the compound and glucose is more
stable than the interaction between the compound and the
a-hydroxy acid or β-diketone, said compound also
containing a detectable moiety having a detectable
quality that changes in a concentration-dependent manner
when said compound is exposed to glucose in said sample;
and
b) measuring any change in said detectable quality
to thereby determine the presence or concentration of
glucose in said sample, wherein the presence of the α-
hydroxy acid or the β-diketone does not substantially
interfere with said determination.
In another aspect, the present invention is directed
to a compound having the following structure

wherein:
-R1 and R2 are the sane or different and are selected
from the following: ) hydrogen; ii) a substituent to
modify the pKa and hydrolytic stability of the R8
moiety, iii) a detectable moiety, or iv) a linking
group capable of attachment to a solid support or a
polymeric matrix, said support or matrix optionally
containing a detectable moiety;
-R3 is hydrogen or a linking group capable of
attachment to a solid support or a polymeric matrix,
said support or matrix optionally containing a
detectable moiety;
-R4 and R5 are the same or different and are selected
from the following: ) hydrogen, ii) a substituent to
modify the pKa and hydrolytic stability of the R8
moiety, iii) a detectable moiety, or iv) a linking
group capable of attachment to a solid support or a
polymeric matrix, said support or matrix optionally
containing a detectable moiety;
-each Z is independently carbon or nitrogen;
-R``6 and R7 are the sane or different and are
i) linking groups having from zero to ten contiguous
or branched carbon said/or heteroatoms, or ii) a
linking group capable of attachment to a solid

support or a polymeric matrix, said support or matrix
optionally containing a detectable moiety;
-R is selected from the following: i) an aliphatic
and/or aromatic spacer containing from 1 to 10
contiguous atoms selected from the group consisting
of carbon, oxygen, nitrogen, sulfur and phosphorus,
ii) a detectable moiety, of iii) a linking group
capable of attachment to a solid support or a
polymeric matrix, said support or matrix optionally
containing a detectable moiety;
-each R8 is the same or different and is an optionally
protected moiety which when unprotected is capable of
interaction with the vicinal diol groups present in
glucose; and
-R9 and R10 are the same or different, and are i)
hydrogen, ii) a detectable moiety, iii) a group
which is a) a linking group capable of attachment
to a solid support of a polymeric matrix, said
support or matrix optionally containing a
detectable moiety, and/or b) includes a functional
group capable of altering the physical properties
of the compound;
with the proviso that the indicator compound contains at
least one detectable moiety associated therewith, either
directly or as part of the solid support or polymeric
matrix.
In another aspect, the present invention is directed
to a detection system which comprises a compound
described above.
BRIEF DESCRIPTION OF THE DRAWINGS
Figure 1 illustrates the normalized fluorescence
emission (I/Io @ 420 nm) of an indicator as described in
Example 1.

Figure 2 illustrates the normalized fluorescence
emission (I/I0 @ 428 nm) of an indicator as described in
Example 2.
Figure 3 illustrates the normalized fluorescence
emission (I/I0 @ 428 nm) of an indicator as described in
Example 3.
Figure 4 illustrates the normalized fluorescence
emission (I/I0 @ 427 nm) of an indicator as described in
Example 4.
Figure 5 illustrates the normalized fluorescence
emission (I/I0 @ 540 nm) of an indicator as described in
Example 5.
Figure 6 illustrates the absorbance spectra of an
indicator as described in Example 6.
Figures 7-8 illustrate the ratio of the absorbance
(450 nm/530 nm) of an indicator as described in Example
6.
Figure 9 illustrates the normalized fluorescence
emission (I/I0 at 550 nm) of an indicator as described in
Example 6.
Figure 10 illustrates the fluorescence spectrum, in
the absence of glucose and in the presence of 100 mM
glucose, of an indicator as described in Example 6.
Figure 11 illustrates the normalized fluorescence
emission (I/I0 at 550 nm) , in the presence of glucose and
lactate, of an indicator as described in Example 6.
Figure 12 illustrates the normalized fluorescence
emission (I/I0 at 525 nm) of an indicator exposed to
glucose as described in Example 10.
Figure 13 illustrates the normalized fluorescence
emission (I/I0 at 530 nm) of an indicator exposed to
lactate as described in Example 10.

Figure 14 shows the relative fluorescence emission (I
@ 430 rm) of an indicat or exposed to glucose and lactate
as described in Example 11.
Figure 15 shows the relative fluorescence emission (I
@ 4 30 nm) of an indicator exposed to glucose and lactate
as described in Example 12.
Figure 16 illustrates the fluorescence of an
indicator exposed to glucose and lactate as described in
Example 13.
DETAILED DESCRIPTION OF THE INVENTION
In one aspect, the present invention provides a way
to detect the presence or concentration of glucose in a
sample which may also contain interfering compounds, such
as α-hydroxy acids or β-diketones. Such potentially
interfering compounds incude lactate, acetoacetate, (3-
hydroxy butyric acid, etc.
The present invention is carried out using an
indicator compound which is capable of recognizing
glucose in a sample, but which is less likely to
recognize interfering conpounds in the sample. The
indicator compound has a least two recognition elements
for glucose, oriented such that the interaction between
the indicator compound and glucose is more stable than
the interaction between the indicator compound and the
interfering compounds.
Suitable recognition elements include moieties which
are capable of a preferaily reversible interaction with
glucose, especially with the diol groups present in
glucose. Several such recognition elements are known,
and preferably include boronic acid, boronate ion,
arsenious acid, arsenite ion, telluric acid, tellurate
ion, germanic acid, germanate ion, etc. Most preferred
are recognition elements containing boron. It will be

understood that until use, the recognition elements may
be capped with a protecting group. Such groups are well
known, and include neoper:yl glycol, pinacol, etc. In
certain embodiments, the capped recognition element is
decapped in the medium in which the compound is to be
used (see, e.g., Example 5).
The recognition elements are preferably spaced on the
indicator compound a sui :able distance from each other so
as to allow at least two of the recognition elements to
interact with a glucose nolecule, resulting in increased
specificity. In general the recognition elements may
have a spacer of up to about 30 atoms between them.
Preferably, the recognition elements are oriented such
that they are capable of being about 6Å apart when
interacting with glucose
The indicator compourds of the present invention have
a detectable quality that changes in a concentration-
dependent manner when the compound is exposed to a sample
containing glucose. Many such qualities are known and
may be used xn the present invention. For example, the
indicator compound may include a luminescent (fluorescent
or phosphorescent) or chemiluminescent moiety, an
absorbance based moiety, etc. The indicator compound may
include an energy donor noiety and an energy acceptor
moiety, each spaced such that there is a detectable
change when the indicator compound interacts with
glucose. The indicator compound may include a
fluorophore and a quencher, configured such that the
fluorophore is quenched by the quencher when glucose is
absent. In that situation, when glucose is present, the
indicator undergoes a configurational change which causes
the quencher to move sufficiently distant from the
fluorophore so that fluorescence is emitted. Conversely,
the fluorophore and quencher may be configured such that

in the absence of glucose, they are sufficiently
separated and the fluorophore emits fluorescence; upon
interaction with glucose, the fluorophore and quencher
are moved in sufficient proximity to cause quenching.
The configurational change concept is described in more
detail in our co-pending application Serial No.
09/754,219, filed January 5, 2001, entitled "Detection of
Analytes", incorporated herein by reference.
Alternatively, the indicator may include a moiety
such as a fluorophore capable of interacting with the
recognition element or another moiety spatially disposed
with respect to the reccgnition element such that in the
absence of glucose, the fluorophore emits fluorescence.
Upon addition of glucose, the glucose competes with the
interaction between the fluorophore and the recognition
element, or the interaction between the fluorophore and
the other moiety spatially disposed with respect to the
recognition element, causing a reduction in fluorescence.
An example of that concept is illustrated in Example 6.
It will also be recognized that the indicator may be
chosen such that the fluorophore emits no fluorescence,
or a relatively low leveL of fluorescence, when the
fluorophore interacts wi ;h the recognition element or
another moiety spatially disposed with respect to the
recognition element in tie absence of glucose. Upon
addition of glucose, the glucose competes with the
interaction between the fluorophore and the recognition
element, or the interact .on between the fluorophore and
the other moiety spatially disposed with respect to the
recognition element, causing an increase in fluorescence.
Other detectable moieties include those whose
fluorescence is affected by glucose interaction via
photoinduced electron transfer or inductive effects.
These include the lantharide chelates disclosed in

copending U.S. Application Serial No. 09/265,979 filed
March 11, 1999 (and published as PCT International
Application WO 99/46600 on September 16, 1999),
incorporated herein by reference; polyaromatic
hydrocarbons and their derivatives; coumarins; BoDiPy;
dansyl; catechols; etc. Another class of moieties
include those whose abso::bance spectrum changes upon
interaction of the indicator compound with glucose,
including Alizarin Red, etc. Another class of moieties
include those whose fluorescence is modulated by
proximity effects, e.g., energy donor/acceptor pairs such
as dansyl/dabsyl, etc.
Preferably, the detectable quality is a detectable
spectral change, such as changes in absorptive
characteristics (e.g., absorbtivity and/or spectral
shift), in fluorescent decay time (determined by time
domain or frequency domain measurement), fluorescent
intensity, fluorescent ahasotropy or polarization; a
spectral shift of the emission spectrum; a change in
time-resolved anisotropy decay (determined by time domain
or frequency domain measurement) , etc.
The indicator compounds of the present invention, if
soluble, may be used directly in solution if so desired.
On the other hand, if the desired application so
requires, the indicator compounds may be immobilized
(such as by mechanical entrapment or covalent or ionic
attachment) onto or within an insoluble surface or matrix
such as glass, plastic, polymeric materials, etc. When
the indicator compound i 3 entrapped within, for example,
another polymer, the entrapping material preferably
should be sufficiently permeable to glucose to allow
suitable interaction between glucose and the indicator
compound.

If the indicator compounds are sparingly soluble or
insoluble in water, yet detection in an aqueous medium is
desired, the indicator compound may be co-polymerized
with a hydrophilic mononer to form a hydrophilic
macromolecule as described in co-pending U.S. application
Serial No. 09/632,624, filed August 4, 2000, the contents
of which are incorporated herein by reference.
Preferred indicator compounds have the following
structure:

wherein:
-R1 and R2 are the same or different and are selected
from the following: hydrogen; ii) a substituent to
modify the pKa and hydrolytic stability of the R8
moiety, iii) a detectable moiety, or iv) a linking
group capable of attachment to a solid support or a
polymeric matrix, sa..d support or matrix optionally
containing a detectable moiety;
-R3 is hydrogen or a linking group capable of
attachment to a solid support or a polymeric matrix,
said support or matrix optionally containing a
detectable moiety;
-R4 and R5 are the sane or different and are selected
from the following: i) hydrogen, ii) a substituent to
modify the pKa and hydrolytic stability of the R8
moiety, iii) a detectable moiety, or iv) a linking
group capable of attachment to a solid support or a

polymeric matrix, said support or matrix optionally
containing a detectable moiety;
-each Z is independently carbon or nitrogen;
-R6 and R7 are the same or different and are
i) linking groups havnig from zero to ten contiguous
or branched carbon and/or heteroatoms, or ii) a
linking group capable of attachment to a solid
support or a polymeric matrix, said support or matrix
optionally containing a detectable moiety;
-R is selected from the following: i) an aliphatic
and/or aromatic spacer containing from 1 to 10
contiguous atoms selected from the group consisting
of carbon, oxygen, nitrogen, sulfur and phosphorus,
ii) a detectable moiety, or iii) a linking group
capable of attachment to a solid support or a
polymeric matrix, said support or matrix optionally
containing a detectable moiety;
-each R8 is the same or different and is an optionally
protected moiety whicn when unprotected is capable of
interaction with the vicinal diol groups present in
glucose; and
-R9 and R10 are the sane or different, and are i)
hydrogen, ii) a detectable moiety, iii) a group
which is a) a linking group capable of attachment
to a solid support or a polymeric matrix, said
support or matrix optionally containing a
detectable moiety, ard/or b) includes a functional
group capable of altering the physical properties
of the compound;
with the proviso that the indicator compound contains at
least one detectable moiety associated therewith, either
directly or as part of the solid support or polymeric
matrix.

Suitable groups for modifying the: pKa and hydrolytic
stability of the R8 moities would be readily apparent to
one of ordinary skill, and include groups such as
halogen; nitro; amino; halogen substituted alkyl;
optionally substituted carboxyl; acyl; keto; nitrile;
amide; ester; alkoxy; etc..
Suitable linking groups for any substituent may
include groups from about 1 to about 20 contiguous atoms,
which may be branched or substituted and which may
include one or more hetreroatoms, which terminate in a
functional group capable of further reaction or
attachment to a polymer or support. Examples of suitable
linking groups include alkyl; aryl; acyl; polyamide;
polyether; all optionally substituted, and combinations
thereof.
R9 and R10 may further include functional groups
capable of altering the physical properties of the
compound, such as solubility, pKa, etc. For example,
these include optionally substituted carboxylates, amino
groups, quartenary ammonium groups, sulfonates, PEG, etc.
It will be understood that when any of the
substituents is a detecable moiety, that could also
include suitable linking groups which link the detectable
moiety to the rest of the indicator compound. Suitable
linking groups include those listed above. Suitable
detectable moieties include those defined above.
R8 is preferably selected from the group consisting of
boronic acid, boronate ion, arsenious acid, arsenite ion,
telluric acid, tellurate ion, germanic acid, germanate
ion, and combinations thereof.
It will also be understood from the above definition
that the present compounds and detection systems may be
in polymeric form. Thus, an integral compound
(containing recognition elements and detectable moiety)

could be linked to an existing polymer, or the integral
compound in monomeric form could be polymerized or co-
polymerized with another suitable monomer to form a
polymer. Alternatively, two separate monomeric
components (e.g., one containing the recognition
elements, and one containing a detectable moiety) could
be co-polymerized so that the resulting polymer contains
all necessary elements of the system (see Example 6).
Many uses exist for the indicator compounds of the
present invention, including uses as indicators in the
fields of energy, medicine and agriculture. For example,
the indicator compounds can be used to detect sub-levels
or supra-levels of gluccse in physiological buffers or
fluids, such as blood, plasma, serum, interstitial fluid,
cerebrospinal fluid, urine, saliva, intraocular fluid,
lymph, tears, or sweat, thus providing valuable
information for diagnosing or monitoring such diseases as
diabetes and adrenal insufficiency.
Medical/pharmaceutical production of glucose for
human therapeutic application requires monitoring and
control.
Uses for the present invention in agriculture include
detecting levels of gluccse in soybeans and other
agricultural products. Glucose must be carefully
monitored in critical harvest decisions for such high
value products as wine crapes. As glucose is the most
expensive carbon source and feedstock in fermentation
processes, glucose monitoring for optimum reactor feed
rate control is importart in power alcohol production.
Reactor mixing and control of glucose concentration also
is critical to quality control during production of soft
drinks and fermented beverages, which consumes the
largest amounts of glucose and fermentable (vicinal diol)
sugars internationally.

When the indicator compounds incorporate fluorescent
indicator substituents, various detection techniques also
are known in the art. For example, the compounds of the
invention can be used ir fluorescent sensing devices
(e.g., U.S. Patent No. 5,517,313) or can be bound to
polymeric material such as test paper for visual
inspection. This latter technique would permit, for
example, glucose measurement in a manner analogous to
determining pH with a strip of litmus paper. The
compounds described herein may also be utilized as simple
reagents with standard benchtop analytical
instrumentation such as spectrofluorometers or clinical
analyzers as made by Shimadzu, Hitachi, Jasco, Beckman
and others. These molecules would also provide analyte
specific chemical/optica . signal transduction for fiber
optic-based sensors and analytical fluorometers as made
by Ocean Optics (Dunedin Florida), or Oriel Optics.
U.S. Patent 5,517,311, the disclosure of which is
incorporated herein by reference, describes a
fluorescence sensing device in which the compounds of the
present invention can be used to determine the presence
or concentration of glucose in a liquid medium. The
sensing device comprises a layered array of a fluorescent
indicator molecule-contaning matrix (hereafter
"fluorescent matrix"), a high-pass filter and a
photodetector. In this device, a light source,
preferably a light-emitting diode ("LED"), is located at
least partially within the indicator material, or in a
waveguide upon which the indicator matrix is disposed,
such that incident light from the light source causes the
indicator molecules to fluoresce. The high-pass filter
allows emitted light to reach the photodetector, while
filtering out scattered incident light from the light
source. The fluorescence of the indicator molecules

employed in the device described in U.S. Patent 5,517,313
is modulated, e.g., attenuated or enhanced, by the local
presence of glucose.
In the sensor described in U.S. Patent 5,517,313, the
material which contains the indicator molecule is
permeable to the analyte. Thus, the analyte can diffuse
into the material from the surrounding test medium,
thereby affecting the fluorescence emitted by the
indicator compounds. The light source, indicator
compound-containing material, high-pass filter and
photodetector are configured such that at least a portion
of the fluorescence emitted by the indicator compounds
impacts the photodetector, generating an electrical
signal which is indicative of the concentration of
glucose in the surrounding medium.
In accordance with other possible embodiments for
using the indicator compounds of the present invention,
sensing devices also are described in U.S. Patent Nos.
5,910,661, 5,917,605 and 5,894,351, all incorporated
herein by reference.
The compounds of the present invention can also be
used in an implantable device, for example to
continuously monitor blood glucose levels in vivo.
Suitable devices are described in, for example, co-
pending U.S. Patent Appllication Serial No. 09/383,148
filed August 26, 1999, as well as U.S. Patent Nos.
5,833,603, 6,002,954 and 6,011,984, all incorporated
herein by reference.
The compounds of the present invention can be
prepared by persons skilled in the art without an undue
amount of experimentation using readily known reaction
mechanisms and reagents, for example including reaction
mechanisms which are consistent with the general
procedures described below.

Example 1
Water soluble copolymer of anthracene derivative and
MAPTAC
I. Synthesis of mono-boronate-anthracene indicator
co-polymerized in water-soluble polymer:
A. 9-[3-(methacrylamido)propylamine]methylanthracene
To a suspension of N-(3-aminopropyl)methacrylamide
hydrochloride salt (11.82g, 66.0 mmole, 3.0 equiv.) and
DBMP (10mg as inhibitor; in 250 mL CHCl3 at 0°C was added
dropwise DIEA (18.5 g, :5.0 mL, 144 mmole, 6.5 equiv.)
over a 20 min period. The mixture was allowed to warm to
25°C and then recooled to 0°C. To the cooled mixture was
added dropwise a solution of 9-chloromethylanthracene
(5.0 g, 22 mmole) in CHCl3 (100 mL) over a 1 hour period.
The mixture was subsequently stirred at 25°C for 1 hour,
50°C for 12 hours and then 70°C for 2 hours. At this
time, the mixture was washed with 4 x 60 mL portions of
water, and the combined aqueous layers were extracted
with CH2Cl2. The combined organic extracts were dried
over anhydrous Na2SO4, decanted and concentrated in vacuo.
The crude material was purified by silica gel
chromatography (flash silica gel, 2-5% CH3OH/CH2Cl2) to
yield 2.44 g (33%) of a solid product.
TLC: Merck silica gel 6( plates, Rf 0.39 with 90/10
CH2Cl2/CH3OH, see with UV (254/366), ninhydrin stain.
B. 9-[N-[2-(5,5-dimethylborinan-2-yl)benzyl]-N-[3-
(methacrylamido) propylan ino ] methylanthracene.
To a solution of 9-[3-(methacrylamido)propylamino]-
methylanthracene (2.44 c, 7.34 mmole) and DBMP (10 mg as
inhibitor) in 200 ml CHCl3 at 0°C was added DIEA (2.85 g,

3.84 mL, 22.0 mmole, 3.C equiv.) in portions over a 10
rain period, followed by the dropwise addition of a
solution of (2-bromometh/lphenyl)boronic acid neopentyl
ester (2.4 9 g, 8.81 mmols, 1.2 equiv.; over a 30 min
period. The mixture was subsequently stirred at 25°C for
20 hours. At this time, the mixture was washed with
water, and the combined aqueous layers were extracted
with CH2Cl2. The combined organic extracts were dried
over anhydrous Na2SO4, decanted and concentrated in vacuo.
The crude material was purified by silica gel
chromatography (flash silica gel, 2-5% CH3OH/CH2Cl2) to
yield 2.50 g (76%) of a lightly yellow crystalline solid.
Mp: 72-73°C.
TLC: Merck silica gel 60 plates,Rf 0.36 with 90/10
CH2Cl2/CH3OH, see with UV '254/366), ninhydrin stain.
C. Water soluble copolymer of 9- [N- [2- (5 ,5-dimethyl-
boxinan-2-yl)benzyl] -N- [3- (methacrylamido)propylamino] -
methylanthracene and MAPTAC (1:20 molar ratio) .
To a solution of 9-[N - [2- (5,5-dimethylborinan-2-yl) -
benzyl] -N- [3- (methacrylamido) propylaraino]methylanthracene
(0.0490 g, 0.105 mmole) e.rtd [3-(methacrylamido)propyl]-
trimethylammonium chloride (MAPTAC, 50 wt % aqueous
solution, 0.48 g, 0.90 mL, 2.1 mmole, 20 equiv.) in 1.5
mL ethylene glycol was added 4 , 4 '-azobis (cyanovaleric
acid) (0.008 g, 0.03 mmole, 1.4 mole % of total
monomer). The solution was purged with argon gas for 5
minutes and then heated to 60°C in the dark for 18 hours.
At this time, the viscous solution was cooled to 25°C,
diluted with 5 mL water and dialyzed through a cellulose
acetate membrane (MWCO 3500) against 3 x 4 L of water.

The dialyzed material was concentrated to dryness to
yield 0.339 g (68%) of a yellow glassy solid.
II. Modulation of Fluorescence With Glucose and Lactate.
The modulation of the fluorescence of the copolymer
(which contains a single recognition element) prepared in
this example by glucose and lactate was determined.
Figure 1 shows the normalized fluorescence emission (I/Io
@ 420 nm) of 0.5 mg/mL solutions of the copolymer (1:20
molar ratio) in PBS containing a) 0-20 mM glucose; b)
0-20 mM lactate. Spectra were recorded using a Shimadzu
RF-5301 spectrafluorometer with excitation @365 nm;
excitation slits at 1.5 nm; emission slits at 5 nm;
ambient temperature. Error bars are standard deviation
with duplicate values for each data point. The
fluorescence of the copolymer was affected by the
presence of glucose and lactate.
Example 2
Modulation of bis-boronate-indicator covalently attached
to water-soluble polymer by glucose and potential
physiological interferences.
A. 9,10-bis[[2-(2-hydroxyethoxy)ethylamino]methyl]-
anthracene.

I. Synthesis of single-)methacrylate monomer of
bis-boronate-anthracene indicator

To a solution of 2-(2-aminoethoxy) ethanol (31.4 g,
30.0 mL, 299 mmole, 20.9 equiv.) in 40 mL CHCl3 at 23°C
was added 9,10-bis (chloromethyl) anthracene (3.94 g, 14.3
mmole). The solution was stirred in the dark for 67
hours. At this time, added 100 mL CH2Cl2 and washed with
1 x 50 mL and 2 x 100 mL portions of NaHCO3 (saturated
aqueous solution). The organic extract was dried over
anhydrous Na2SO4, filtered and concentrated to yield 4.67
g (79%) of a yellow powder. Product (~85 % pure by
RP-HPLC) was carried on as is.
HPLC conditions: HP 1100 HPLC chromatograph, Vydac 20lTP
10 x 250 mm column, 0.10) mL injection, 2 mL/min, 370 run
detection, A = water (0. 1% HFBA) and B = MeCN (0.1%
HFBA), gradient 10% B 2 run, 10-80% B over 18 min,
80-100% B over 2 min, 10) %B 2 min, retention time 15.6
min.

B. 9,10-bis [N- [2- (5,5-dimethylborinan-2-yl) benzyl] -N-
[2- (2-hydroxyethoxy)ethylamino]methyl] anthracene.
A solution of 9,10-bis [ [2-(2-hydroxyethoxy) -
ethylamino]methyl]anthracene (4.02 g, 9.75 mmole), DIEA
(12.6 g, 17.0 mL, 97.5 mmole, 10.0 equiv.) and
(2-bromomethylphenyl)boronic acid neopentyl ester (13.7
g, 48 mmole, 4.9 equiv.) ;.n 125 mL CHCl3 at 23°C was

stirred in the dark for 4 6 hours. At this time, the
reaction mixture was concentrated initially by rotary
evaporation, then using a vacuum pump to remove the DIEA.
The residue was purified by alumina column chromatography
(150 g activated neutra alumina, 0-3% CH3OH/CH2Cl2) to
yield 5.67 g (70%) of a viscous oil which solidified upon
standing. Product (~85 % pure by RP-HPLC) was carried on
as is.
TLC: Merck basic alumina plates, Rf 0.33 with 95/5
CH2Cl2/CH3OH, see with U\ (254/366).
HPLC conditions: HP HOC HPLC chromatograph, Vydac 201TP
10 x 250 mm column, 0.100 mL injection, 2 mL/min, 370 run
detection, A = water (0.1% HFBA) and B = MeCN (0.1%
HFBA), gradient 10% B 2 rain, 10-80% B over 18 min,
80-100% B over 2 min, 1C0% B 2 min, retention time 18.8
min.

C. 9-[N-[2-(5,5-dimethy Lborinan-2-yl)benzyl]-N-
[2- (2-methacroyloxyethoxY) ethylamino]methyl] -10-
[N- [2- (5,5-dimethylborinan-2-yl) benzyl] -N- [2-
(2-hydroxyethoxy) ethylamino] -methyl] anthracene . (Single-
methacrylate monomer)

A solution of 9,10-b..s[N-[2-(5, 5-dimethyl-
borinan-2-yl)benzyl]-N-[2-(2-hydroxyethoxy)ethylamino]-
methyl]anthracene (0.298 g, 0.359 mmole), methacrylic
acid (0.304 g, 0.300 mL, 3.53 mmole, 9.84 equiv.), DCC
(0.965 g, 4.68 mmole, 13 0 equiv.) and N,N-dimethyl-
aminopyridine (0.020 g, ),16 mmole, 0.46 equiv.) in 15 mL
CH2Cl2 at 23°C was stirred in the dark for 4 hours. At
this time, the reaction mixture was filtered and
concentrated by rotary evaporation. The residue was
purified by alumina column chromatography (50 g activated
neutral alumina, 0-4% CH2CH/CH2Cl2) to yield 0.150 g (47%)
of a yellow solid.
FAB MS: Calc=d for C52H66E2N209 [M]+ 88 5; Found [M + 1] +
886.
TLC: Merck basic alumina plates, Rf 0.45 with 95/5
CH2Cl2/CH3OH, see with UV .254/366).
HPLC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm
column, 0.100 mL injection, 2 mL/min, 370 nm detection, A
= water (0.1% HFBA) and It = MeCN (0.1% HFBA) , gradient
10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min,
100% B 2 min, retention time 21 min.
D. Water soluble copolymer of 9-[N-[2-(5,5-dimethyl-
borinan-2-yl)benzyl] -N- [2 -(2-methacroyloxyethoxy) ethyl-
amino] methyl] -10- [N- [2- (5-, 5-dimethylborinan-2-yl) benzyl] -
N- [2- (2-hydroxyethoxy) ethylamino] -methyl] anthracene and
TMAMA (1:50 molar ratio)
To a solution of [2-(methacryloxy)ethyl]trimethyl-
ammonium chloride (TMAMA, 70 wt% aqueous solution, 0.344
g monomer, 1.66 mmole, 5( equiv.) in 0.600 mL water was

added a solution of 9-[N-[2-(5,5-dimethylborinan-2-yl)-
benzyl]-N-[2-(2-methacroyloxyethoxy)ethylamino]methyl]-
10- [N-[2-(5,5-dimethylborinan-2-yl)benzyl]-N-[2-(2-
hydroxyethoxy)ethylaminc]methyl]anthracene (0.0024 g,
0.0033 mmole) in 3.00 ml MeOH. To this mixture was added
4,4'-azobis(4-cyanovaleric acid) (0.0075 g, 0.027 mmole,
1.6 mole % of total monomer). The solution was filtered
through a 0.45μ membrane filter, was purged with nitrogen
gas and then heated in the dark at 55°C for 16 hours. At
this time, the viscous solution was cooled to 25°C and
concentrated in vacuo. The residue was diluted with 20
mL water and filtered through a 0.2μ . membrane filter.
The polymer solution was dialyzed through a cellulose
acetate membrane (MWCO 3500} against 2 x 4 L of water.
From the dialysis was obtained 38.5 mL of polymer
solution. Concentratior of a portion of this solution to
dryness indicated 0.0075g polymer per 1.0 mL solution.
Overall 0.289g (77%) yield of polymer.
II. Modulation of Fluorescence With Glucose, Lactate and
Acetoacetate
The modulation of the fluorescence of the copolymer
(which contains two recognition elements) prepared in
this example by glucose, lactate and acetoacetate was
determined. Figure 2 shows the normalized fluorescence
emission (I/Io @ 428 nm) of a 1.5 mg/mL solution of
anthracene bis boronate-TMAMA (1:50 mole ratio) copolymer
in PBS containing a) 0-20 mM glucose; b) 0-20 mM lactate;
c) 0-20 mM lithium acetcacetate. Spectra were recorded
using a Shimadzu RF-530 spectrafluorometer with
excitation @365 nm; excitation slits at 1.5 nm; emission
slits at 1.5 nm; ambient temperature. The fluorescence
of the copolymer was affected by the presence of glucose,
but not by the presence of lactate or acetoacetate.

Example 3
Effect of lactate in solation on the dose response effect
of glucose on the fluorescence of bis-boronate-anthracene
indicator

A. 9,10-bis[[2-(tert-butoxycarbonyl)ethylamino]methyl]-
anthracene.
A solution of β-alanine tert-butyl ester
hydrochloride (3.06 g, 16.8 mmole, 5.09 equiv.), DIEA
(4.27 g, 5.75 mL, 33.0 mmole, 10.00 equiv.) and 9,10-
bis (chloromethyl) anthrac ene (0.910 g, 3.31 mmole) in 75
mL CHCl3 at 23°C was stirred in the dark for 93 hours. At
this time, the solution was filtered and washed with 1 x
40 mL and 2 x 60 mL portions of NaHCO3 (saturated aqueous
solution). The organic extract was dried over anhydrous
Na2SO4, filtered and concentrated to yield a crude yellow
solid. The residue was purified by silica gel column
chromatography (30 g gravity grade gel, 0-3% CH3OH/CH2Cl2)
to yield 1.06 g (65%) of a viscous yellow-orange.
Product was carried on as is.
TLC: Merck silica gel 6( plates, Rf 0.33 with 95/5
CH2Cl2/CH3OH, see with W (254/366) .

B. 9,10-bis [N- [2- (5,5 -dimethylborinan-2-yl)benzyl] -N-
[2-(tert-butoxycarbonyl)ethylamino]methyl]anthracene.
A solution of 9,10-bis[[2-(tert-butoxycarbonyl)-
ethylamino]methyl]anthracene (1.60 g, 3.25 mmole), DIEA
(4.45 g, 6.00 mL, 34.4 mmole, 10.6 equiv.) and (2-
bromomethylphenyl)boronic acid neopentyl ester (4.80 g,
17.0 mmole, 5.22 equiv. in 30 mL CHCl3 at 23°C was
stirred in the dark for 4.5 days. At this time, 45 mL
CHCl3 were added to ,tne mixture and the mixture was washed
with 2 x 25' mL portions of NaHCO3 (saturated aqueous
solution). The organic extract was dried over anhydrous
Na2SO4, filtered and concentrated to yield crude reddish
oil. The residue was purified by alumina column
chromatography (100 g activated neutral alumina, 0-3%
CH3OH/CH2Cl2) to yield ~ 3.5 g of an orange solid. The
product was dissolved, followed by the formation of a
white precipitate (DIEA-HBr salt). The solution was
filtered and the filtrate concentrated to yield 2.72 g
(93%) of an orange solid, Product (>80 % pure by RP-
HPLC) was carried on as is.
TLC: Merck basic alumina plates, Rf 0.66 with 95/5
CH2Cl2/CH3OH, see with UV (254/366).
HELC conditions: HP 110) HPLC chromatograph, Vydac 201TP
10 x 250 mm column, 0.1)0 mL injection, 2 mL/min, 370 nm
detection, A = water (0 1% HFBA) and B = MeCN (0.1%

HFBA), gradient 10% B 2 min, 10-80% B over 18 min, 80-
100% B over 2 min, 100% 3 2 min, retention time 23.9 min.
C. 9,10-bis [N- (2-boron abenzyl) -N- [2--
(carboxyethyl)amino]-methyl]anthracene.
A solution of 9,10-bis [N-[2-(5, 5--dimethylborinan-2-
yl)benzyl]-N-[2-(tert-bu :oxycarbonyl)ethylamino]methyl]-
anthracene (0.556 g, 0.620 mmole) in 5 mL 20% TFA/CH2Cl2
at 23°C was stirred in the dark for 25 hours. At this
time, the reaction mixture was concentrated under a
stream of N2 gas. The residue was triturated with 3 x 10
mL portions of ether. The residual solid was dried in
vacuo to yield 0.351g (87%) of a fluffy yellow powder.
FAB MS: Glycerol matrix; 3alc=d for C42H46B2N20010 (bis
glycerol adduct) [M]+ 76), Found [M]+ 760.
HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.325 mL injection, 0.75 mL/min,
1.5 mL injection loop, 363 nm detection, A = water (0.1%
HFBA) and B = MeCN (0.1% HFBA) , gradient 10% B 2 min, 10-
80% B over 18 min, 80-100% B over 2 min, 100% B 2 min,
retention time 16.7 min.
D. Modulation of Fluorescence With Glucose and Lactate
The modulation of the fluorescence of the indicator
compound (which contains two recognition elements)

prepared in this example by glucose and lactate was
determined. Figure 3 s lows the fluorescence (at 428 ran)
of 75 pM solutions of bis carboxylate bis-boronate-
anthracene indicator in PBS containing a) 0-10 mM
glucose, 0 mM lactate; b) 0-10 mM glucose, 2 mM lactate;
c) 0-10 mM glucose, 5 ml! lactate. Spectra were recorded
using a Shimadzu RF-530 . spectrafluorometer with
excitation @365 nm; excitation slits at 1.5 nm; emission
slits at 1.5 nm; ambient temperature. All points
measured in triplicate, with ±1 SD error bars included.
The presence of lactate did not substantially affect the
fluorescence modulation of the indicator by glucose.
Example 4
Selectivity of Bis-Bororate Glucose Indicator for Glucose
vs. Lactate and Acetoace tate When Indicator Covalently
Immobilized in the Hydrogel
I. Preparation of Dual-Methacrylamide Monomer

A. 9,10-bis[3-(methacrylamido)propylamino]-
methylanthracene.
A suspension of 9,1 )-bis(chloromethyl)anthracene
(1.5 g, 5.45 mmole), DIEA (28.17 g, 38.00 mL, 218 mmole,
40 equiv.), N-(3-aminopr)pyl)methacrylamide hydrochloride
salt (9.76 g, 54.5 mmole 10.0 equiv.), and ~ 5 mg of BHT

in 200 mL CHCl3 at 23°C was stirred in the dark for 4 days
at 40°C. At this time, the temperature was increased to
45°C and the mixture was stirred for 3 days longer. At
this time, a precipitate had formed. The mixture was
filtered, and the solid product dissolved in the minimum
amount of CH2Cl2. A yellow crystalline solid, the bis
hydrochloride salt of the desired product, formed
overnight (3.15 g, quantitative).
TLC: Merck basic alumina plates, Rf 0.31 with 90/10
CH2Cl2/CH3OH, see with UV (254/366).
HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.100 mL injection, 0.75 mL/min,
360 nm detection, A = water (0.1% HFBA) and B = MeCN
(0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min,
80-100% B over 2 min, 10D% B 2 min, retention time 15.0
min.

B. 9,10-bis [N- [2- (5,5- limethylborinan-2-yl)benzyl] -N-
[3-(methacrylamido)propylamino]methylanthracene. (Dual-
methacrylamide monomer)
A solution of 9,10-bis [3-(methacrylamido)-
propylamino]methylanthra.:ene (0.0.650 g, 1.34 mmole of

the free amine), DIEA (3.612 g, 0.825 mL, 4.74 mmole,
3.55 equiv.), (2-bromomethylphenyl)boronic acid neopentyl
ester (1.34 g, 4.74 mmole, 3.55 equiv.) and BHT (5 mg as
inhibitor) in 20 mL CHC, at 23°C was stirred in the dark
for 5 days. At this tine, the reaction mixture was
concentrated in vacuo a;id the residue was purified by
alumina chromatography !200 g activated neutral alumina,
0-2% CH3OH/CH2Cl2) to yield 0.465 g (39%) of a very
viscous yellow oil.
TLC: Merck basic alumina plates, Rf 0.59 with 90/10
CH2Cl2/CH3OH, see with UV (254/366).
HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, (.050 mL injection, 0.75 mL/'min,
360 nm detection, A = water (0.1% HFBA) and B = MeCN
(0.1% HFBA), gradient 1C % B 2 min, 10-80% B over 18 min,
80-100% B over 2 min, 1C0% B 2 min, retention time 16.9
min.
C. Preparation of N,N-dimethylacrylamide hydrogel with
glucose indicator:
A solution of N,N-dimethylacrylamide (40% wt.) and
N,N=-methylenebisacrylamide (0.8% wt.) in ethylene glycol
was prepared. 9,10-bis[N-[2-(5,5-dimethylborinan-2-yl)-
benzyl]-N-[3-(methacrylauido)propylamino]methylanthracene
(17.8 mg, 2xl0-5 mole) and 40 μL of aqueous ammonium
persulfate (5% wt) were combined with 1 mL of ethylene
glycol monomer solution. The resulting solution was
placed in a glove box purged with nitrogen. An aqueous
solution of N,N,N=,N=-tetramethylethylenediamine (80 uL,
.5% wt.) was added to the nonomer formulation to
accelerate polymerization. The resulting formulation was
poured in a mold constructed from microscope slides and

100 micron stainless steel spacer. After being kept for
8 hours in nitrogen atmosphere the mold was placed in
phosphate buffered saline (PBS) (10 mM PBS, pH=7.4), the
microscope slides were separated, and the hydrogel was
removed. The hydrogel was washed with 100 mL of PBS
containing 1 mM lauryl sulfate sodium salt and 1 mM EDTA
sodium salt for 3 days, 1 he solution being changed every
day, followed by washing with DMF/PBS (10/90 by vol., 3 x
100 mL), and finally with PBS (pH=7.4, 3 x 100 mL). The
resulting hydrogel polymer was stored in PBS (10 mM PBS,
pH=7.4) containing 0.2% wt. sodium azide and 1 mM EDTA
sodium salt.
II. Modulation of Fluorescence With Glucose, Lactate and
Acetoacetate
The modulation of the fluorescence of the indicator
compound (which contains two recognition elements)
prepared in this example by glucose, lactate and
acetoacetate was determined. Figure 4 shows the
normalized fluorescence emission (I/Io @ 427 nm) of a
hydrogel containing the glucose recognition molecule of
this example in 10 mM PB! , pH 7.4 containing 0.2% NaN3 and
1 mM EDTA containing various amounts of sodium-L-lactate,
lithium acetoacetate or c-D-glucose. Data were recorded
using a Shimadzu RF-5301 spectrofluorometer with
excitation @365 nm (slit - 3 nm) and emission at 427 nm
(slit = 3 nm) at low sensitivity at 37°C using a
temperature controlled sample holder. The cuvettes
containing 3 mL of the de sired solution were equilibrated
at 37°C for 15 minutes before measurement. Each hydrogel
sample was measured in four independent samples. Error
bars are standard deviation with quadruplicate values for
each data point. The hygrogels containing a glucose
recognition molecule were prepared as previously
described. The hydrogels were mounted on glass slides

and covered with polyester mesh in PMMA cuvettes at 4 5D
to the incident light. Solutions of 1, 5, 10 and 20 mM
sodium L-lactate [Aldrich], 5, 10 and 20 mM lithium
acetoacetate [Aldrich], and 1, 2, 4, 5, 10, and 20 mM
α-D-glucose were prepared in 10 mM PBS, pH 7.4 containing
0.2% NaN3 and 1 mM EDTA. The fluorescence of the
copolymer was affected by the presence of glucose, but
not by the presence of lactate or acetoacetate.
Example 5
Glucose selectivity vs. lactate using bis-boronate
recognition and proximity quenching signal generation
A. N- (2 ,2-diethoxyethyl) -4-bromo-l, 8-naphthalimide.
A suspension of 4-brorno-1, 8-naphthalic anhydride
(10.0 g, 36.1 mmol) and aminoacetaldehyde diethyl acetal
(4.81 g, 5.26 mL, 36.1 mmol, 1 equiv. ] in 45 mL EtOH was
stirred at 45°C for 3 days. At this time, the resulting
suspension was filtered, washing with EtOH and the
residue was dried to yieLd 13.3 g (94%) of a light brown
solid product.
TLC: Merck silica gel 60 plates plates, Rf 0.17 with 98/2
CH2Cl2/CH30H, see with UV (254/366) .
HPLC: HP 1100 HPLC chromotograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0 050 mL injection, 0.75 mL/min,
1.5 mL injection loop, 350 nm detection, A = water (0.1%
HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min,
10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min,
retention time 24.2 min.
B. N-(2,2-diethoxyethyl)-4-butylamino-1,8-naphthalimide.
A solution of N-(2,2 -diethoxyethyl) -4-bromo-1, 8-

naphthalimide (0.797 g, 2.03 mmol) and n-butylamine (1.48
g, 2.00 mL, 20.2 mmol,0.96 equiv.) in 8 mL NMP was
heated at 45°C for 66 hours. At this time, the resulting
suspension was allowed to cool to 25°C, followed by
filtration. The residue was dissolved with 50 mL ether '
and extracted 3 x 50 mL water. The organic extract was
dried over anhydrous Na2SO4, filtered and concentrated to
yield a crude yellow povder. The crude material was
purified by silica gel chromatography (25 g gravity grade
gel, 0-1% CH3OH/CH2Cl2) to yield 0.639 g (82%) of a yellow
powder.
TLC: Merck silica gel 60 plates, Rf 0.71 with 95/5
CH2Cl2/CH3OH, see with UV (254/366) .
HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.D50 mL injection, 0.75 mL/min,
1.5 mL injection loop, 4 30 nm detection, A = water (0.1%
HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min,
10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min,
retention time 23.5 min.
C. N- (2-oxoethyl) -4-butylamino-1, 8naphthalimide.
A solution of N-(2,2-diethoxyethyl)-4-butylamino-
1,8-naphthalimide (0.622 g, 1.62 mmol) and p-toluene-
sulfonic acid mono hydrate (0.010 g, 0.053 mmol, 0.032
equiv.) in 25 mL acetone was stirred at 25°C for 18
hours. At this time, the solution was concentrated and
the residue purified by silica gel chromatography (25 g
gravity grade gel, 0-1% CH3OH/CH2CL2) to yield 0.470 g
(94%) of an orange solid
TLC: Merck silica gel 60 plates, Rf 0.61 with 95/5
CH2Cl2/CH3OH, see with UV (254/366).

HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 3.050 mL injection, 0.75 mL/min,
1.5 mL injection loop, 3 50 run detection, A = water (0.1%
HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min,
10-80% B over 18 min, 8 3-100% B over 2 min, 100% B 2 min,
retention time 19.6 min.
D. N- (4-dimethylaminobenzyl) -1, 6-diaminohexane.
A suspension of 4-limethylaminobenzaldehyde (1.00 g,
6.70 mmol), Na2SO4 (6.70 g, 47.2 mmol, 7.04 equiv.) and
1, 6-diaminohexane (3.89 g, 33.5 mmol, 5.00 equiv.) in 20
mL anhydrous EtOH was stirred in the dark at 25°C under
an atmosphere of nitrogen gas for 18 hours. At this
time, the solution was filtered and NaBH4 (1.73 g, 45.8
mmol, 6.84 equiv.) was added to the filtrate. The
suspension was stirred at 25°C for 5 hours. At this
time, the reaction mixture was concentrated and the
residue dissolved in 50 mL water and extracted 3 x 50 mL
ether. The combined organic extracts were washed 2 x 50
mL water. The combined aqueous extracts were extracted 2
x 50 mL ether. The combined organic extracts were dried
over Na2SO4, filtered and concentrated to yield 1.35 g
(81%) of a viscous oil.
TLC: Merck silica gel 6( plates plates, Rf 0.58 with
80/15/5 CH2Cl2/CH3OH/iPrNH2, see with ninhydrin stain, UV
(254/366) .

HPLC: HP 1100 HPLC chromatography Waters 5 x 100 nun
NovaPak HR C18 column, 0.350 mL injection, 0.75 mL/min,
1.5 mL injection loop, 230 nm detection, A = water (0.1%
HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min,
10-80% B over 18 min, 8C-100% B over 2 min, 100% B 2 min,
retention time 13.3 min.
E. N-2- [6-N (H-4-dimethylaminobenzyl) aminohexyl] amino-
ethyl) -4-butylamino-1, 8- naphthalimide.
To a suspension of N-(2-oxoethyl)-4-butylamino-l,8-
naphthalimide (0.34 6 g, 1.11 mmol) in 25 mL anhydrous
MeOH was added a solution of N-(4-dimethylamino-
benzyl)-l, 6-diaminohexane (0.554 g, 2.22 mmol, 2.00
equiv.) and acetic acid (0.067 g, 1.1 mmol, 1.0 equiv.)
in 20 mL anhydrous MeOH To this mixture was added a
solution of NaCNBH3 (0.(70 g, 1.1 mmol, 1.0 equiv.) in 5
mL anhydrous MeOH. The reaction mixture was stirred at
25°C for 15 hours. At this time, the MeOH was removed by
rotary evaporation and the residue was dissolved in 30 mL
water. The solution was adjusted to pH 2 with 1 N HCl
and then stirred for 1 hour at 25°C. At this time, the
solution was adjusted to pH 12 with 1 N NaOH and
subsequently extracted 3 x 50 mL CH2Cl2. The combined
organic extracts were washed 3 x 50 mL water, dried over
anhydrous Na2SO4, filtered and concentrated to yield a
crude brown oil. The crude material was purified by
silica gel chromatography (35 g flash grade gel, 0-50%
CH3OH/CH2Cl2, then 4 5/5C/5 CH3OH/CH2Cl2/iPrNH2) to yield
0.190 g (32%) of diamire product.
FAB MS: Calc=d for C33H25N5O2 [M]+ 54 4; Found [M]+ 54 4.
TLC: Merck silica gel 60 plates, Rf 0.42 with 80/20
CH2Cl2/CH3OH, see with rinhydrin stain and UV (254/366).

HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.050.mL injection, 0.75 mL/min,
1.5 mL injection loop, 3 50 nm detection, A = water (0.1%
HFBA) and B = MeCN {0.1% HFBA), gradient 10% B 2 min,
10-80% B over 18 min, 8 )--100% B over 2 min, 100% B 2 min-,
retention time 17.6 min
F. N-2-[6-N-(N-4-dimetliylaminobenzyl)-6-N-[2-(5,5-
dimethylborinan-2-yl)benzyl] aminohexyl] - [2- (5,5-dimethyl-
boxinan-2-yl)benzyl] aminoethyl-4-butylamino-1, 8-
naphthalimide.
To a solution of N- 2-[6-N-(N-4-dimethylaminobenzyl)-
aminohexyl]aminoethyl)-4-butylamino-1,8-naphthalimide
(0.150 g, 0.276 mmole) and DIEA (0.355 g, 0.478 mL, 2.81
mmole, 10.0 equiv.) in 5 mL CHCl3 was added a solution of
(2-bromomethylphenyl)boronic acid neopentyl ester (0.390
g, 1.38 mmole, 5.00 equiv.) in 2 mL CHCl3. The solution
was subsequently stirred at 25°C for 27 hours. At this
time, the mixture was contentrated and the residue was
purified by alumina colunn chromatography (100 g
activated neutral alumina, 0-5% CH3OH/CH2Cl2) to yield
0.024 g (19%) of a visco is brown oil.
FAB MS (glycerol matrix) Calc'd for C53H67B2N50O8 [M]+ 924
(bis glycerol adduct in phace of bis neopentyl ester of
boronic acids); Found [M + 924.
TLC: Merck neutral alumina plates, Rf 0.62 with 80/20
CH2Cl2/CH3OH, see with UV (254/366*).
HPLC: HP 1100 HPLC chrometograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.C50 mL injection, 0.75 mL/min,
1.5 mL injection loop, 450 nm detection, A = water (0.1%
HFBA) and B = MeCN (0.1% HF3A), gradient 10% B 2 min,

10-80% B over 18 min, 80-100% B over 2 min, 100% B 2 min,
retention time 20.7 min.
G. N-2- [6-N- (N-4-dimethylaminobenzyl) -6-N-
[2 - (borono) benzyl] aminohitxyl ]-[2- (borono) benzyl] amino-
ethyl-4-butylamino-1, 8-naphthalimide (nBuF-hexa-Q
bis-boronate).
The free bis boronic acid product used in glucose
studies results from dissolution of N-2-[6-N-(N-4-
dimethyl-aminobenzyl) -6- N- [2- (5, 5-dimethylborinan-2-
yl)benzyl]amino-hexyl]-[2-(5,5-dimethylborinan-2-
yl)benzyl]aminoethyl-4-
butylamino-1,8-naphthalimide in the MeOH/PBS buffer
system.
H. Modulation of fluorescence with glucose and lactate.
The modulation of the fluorescence of the indicator
compound (which contains two recognition elements)
prepared in this sample oy glucose and lactate was
determined. Figure 5 stows the normalized fluorescence
emission (I/Io @ 535 ran) of 0.015 mM solutions of the
indicator compund in 70/30 MeOH/PBS containing a) 0-20 mM
glucose; b) 0-20 mM lactate. Spectra were recorded using
a Shimadzu RF-5301 spectrafluorometer with excitation @
450 nm; excitation shitf at 1.5 rm; emission slits at 1.5
nm; ambient temperature. Error bars are standard
deviation with triplicate values for each data point.
The fluorescence of the indicator was affected by the
presence of glucose, but not substantially affected by
the presence of lactate

Example 6
Effect of glucose or lactate on acrylamide gel containing
H-[3- (methacrylamido) propyl] -3,4-dihydroacy-9, lO-dioxo-2-
anthracenesulfonamide (Alizarin Red S monomer) and
α,α'-bis [N- [2- {5,5-dimethylborinan-2-yl)benzyl] -N- [3-
(methacrylamido)propyl amino] ~1,4--xylene (bis boronic acid
monomer):
A. 3,4-Dihydroxy-9,1( -dioxo-2~anthracenesnlfonyl
chloride:
3, 4~dihydroxy-9, 0-dioxo~2-anthracenesulfonic acid
sodium salt (1,4 g, 3 9 mmoles) was combined with 30 mL
of chlorosulfonic acid and heated to 90°C for 5 hours,
after which the solution was cooled to 0°C and poured
into 100 g of ice. After the ice melted the solution was
extracted with CH2Cl2 (3 x 100 mL) , methylene chloride
extracts were combined, dried with Na2SO4 and evaporated
to produce 0.87 g of solid (Yield 66%).
B. N- [3- (methacrylamido) propyl] -3,4-dibydroxy-9,10-
dioxo-2-anthracenesulfonamide:
3,4~dihydroxy~9( 10-dioxo-2-anthracenesulfonyl
chloride (96 mg, 0.28 mmoles) and N- (3-aminopropyl)
methacrylamide hydrochloride (108 mg, 0.6 mmoles) were
combined with 20 mL of CH2Cl2. To this suspension Et3N
(303 mg, 3 mmoles) was added. The mixture was stirred at
room temperature for 24 hours, filtered, and solvent was
evaporated. The resulting solid was subjected to column
chomatography on SiC, (10 g) with CH2Cl2/MeOH (90/10) as
an eluent. The product was obtained as a red solid {80
mg, 64% yield).
FAB MS: Calculated for C21H20N2O7S M+ 4 45; Found M+ 445.

HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0 100 mL injection, ,0.75 mL/min, 2
mL injection loop, 370 nm detection, A = water (0.1%
HFBA) and B = MeCN (0.1% HFBA), gradient 10% B 2 min,
10-80% B over 18 min, 8C-100% B over 2 min, 100% B 2 min,
retention time 17.67 min .
C. α,α' -bis [3-(methacrylamido)propylamino] -1,4-xylene.
A solution of N- (3-aminopropyl)methacrylamide
hydrochloride salt (3.00 g, 16.8 mmole, 2.21 equiv.),
DIEA (6.5 g, 8.8 mL, 5C mmole, 6.6 equiv.),
terephthaldicarboxaldel yde (1.02 g, 7.60 mmole) and Na2SO4
(10.7 g, 75.3 mmole, 9 91 equiv.) in 75 mL anhydrous MeOH
was stirred in the dark at 25DC for 18 hours. At this
time, more Na2SO4 (10.7g, 75.3 mmole, 9.91 equiv.) was
added and stirring continued for 6 hours longer. At this
time, the solution was filtered and NaBH4 (1.73 g, 45.7
mmole, 6.01 equiv.) was added to the filtrate in portions
and subsequently stirred at 25°C for 21 hours. The
suspension was filtred through Celite and the filtrate
was concentrated. The residue was dissolved in 100 mL
CH2Cl2 and washed 1 x 25 mL saturated aqueous NaHCO3. The
organic extract was cried over anhydrous Na2SO4, filtered
and concentrated to yield a viscous oil. The product was
carried on as is.
HPLC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm
column, 0.100 mL injection, 2.00 mL/min, 260 nm
detection, A = water (0.1% HFBA) and B = MeCN (0.1%
HFBA), gradient 10% B 2 min, 10-80% B over 18 min,
80-100% B over 2 min, 100% B 2 min, retention time 15.8
min.

D. α,α=-bis[N-[2-(5,5-dimethylborinan-2-yl)benzyl]-
N- [3- (methacrylamido) propylamino] -1,4-xylene.
A solution of α,α=-bis[3-(methacrylamido)-
propylamino]-1,4-xylene (2.94 g, 7.61 mmole), DIEA (2.97
g, 4.00 mL, 23.0 mmoles, 3.02 equiv.), (2-bromomethyl~
phenyl)boronic acid neopentyl ester (6.50 g, 23.0 mmole,
3.02 equiv.) and BHT ( 5 mg as inhibitor) in 75 mL CH2Cl2
at 25°C was stirred in the dark for 28 hours. At this
time, the mixture was washed 1 x 25 mL saturated aqueous
NaHCCb. The organic extract was dried over anhydrous
Na2SO4, filtered and concentrated. To the residue was
added 200 mL ether and the suspension was stirred for 18
hours. The suspensior was filtered and the residue
dissolved in CH2Cl2, fitered and the filtrate
concentrated. To the solid residue was added 150 mL
ether and the suspension was stirred for 18 hours. At
this time, the suspension was filtered yielding 1.98 g
(33%) of a fluffy pin) powder.
FAB MS: Calc=d for C46H64B2N4O6 [M]+ 790; Found [M + 1] +
791.
HPLC: HP 1100 HPLC cinematograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.050 mL injection, 0.75 mL/min,
280 nm detection, A = water (0.1% HFBA) and.B = MeCN
(0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min,
80-100% B over 2 min, 100% B 2 min, retention time 13.4
min.
E. Preparation of acrylamide gel containing
N-[3-(methacrylamido)propyl]-3,4-dihydroxy-9,10-dioxo-2-
anthracenesulfonamide (Alizarin Red S monomer) and
α,α'-bis[N-[2-(5,5-dimethylborinan-2-yl)benzyl]-N-[s-
(mathacrylamido) propyl amino] -1,4-xylene:

Ethylene glycol solution containing 30% wt.
acrylamide and 0.8% wt. N,N'-methylenebisacrylamide was
prepared.
N- [3- (methacrylamido)propyl]-3,4-dihydroxy-9,10-dioxo-2-a
nthracenesulfonamide (1.5 mg, 3.38 x 10-6 mole) and
α,α'-bis[N-[2-(5,5-dimethyl-
borinan-2-yl)benzyl]-N- [3- (meth-acrylamido) propylamine-] -1,
4-xylene (28 mg, 3.54 x 10-5 mole) were combined with 800
uL of ethylene glycol monomer solution and 40 uL of 5%
wt. aqueous ammonium persulfate. This formulation was
placed in a glove box purged with nitrogen along with a
mold constructed from class microscope slides and 100
micron stainless steel spacer. An aqueous solution of
N,N,N',N'-tetramethylethylenediamine (40 μL, 5% wt.) was
added to the monomer solution to accelerate
polymerization and the final formulation was poured into
a glass mold. The mold was left under nitrogen
atmosphere for 16 hours, after which it was immersed in
PBS (pH=7.4) and the glass slides were separated to
afford a hydrogel polymer in a form of a thin film. The
resulting hydrogel thin film was washed with 100 mL of
phosphate buffered saline containing 1 mM lauryl sulfate
sodium salt for 3 days the solution being changed every
day, followed by washing with MeOH/PBS (20/80 by vol., 3
x 100 mL) , and finally with PBS (pH=7.4, 3 x 100 mL) .
Hydrogel polymer was stored in PBS (10 mM PBS, pH=7.4)
containing 0.2% wt. sodium azide and 1 mM EDTA sodium
salt.
F. Modulation of Absorbance With Glucose and Lactate
The modulation of the absorbance of the indicator
hydrogel (which contains two recognition elements)
prepared in this example by glucose and lactate was
determined. The acrylamide gel was mounted in PMMA cell
in the same way as described in Example 4. Phosphate

buffered saline (PBS), pH=7.4 containing desired amount
of glucose or sodium lactate was heated to 37°C in a
water bath and placed in the PMMA cell containing the gel
after which the PMMA c ell was allowed to equilibrate for
15 min at 37°C. Absorbance measurement for each glucose
or lactate concentration was conducted in triplicate.
For each measurement, absorbance at 650 nm was used as a
blank, A(650 nm) was subtracted from all values of
A(450nm) and A(530 nm).
Figure 6 shows the absorbance spectra for acrylamide
gel (30%) containing 4 mM Alizarin Red S monomer and 44
mM bis boronic acid monomer with and without glucose.
Figure 7 shows the effect of glucose on absorbance of
acrylamide gel (30%) containing 4 mM Alizarin Red S
monomer and 4 4 mM bis boronic acid monomer. Figure 8
shows the effect of sodium lactate on absorbance of
acrylamide gel (30%) containing 4 mM Alizarin,Red S
monomer and 4 4 mM bis boronic acid monomer. The
absorbance of the indicator was affected by the presence
of glucose, but not substantially affected by the
presence of lactate.
G. Modulation of Fluorescence With Glucose and Lactate
The modulation of the fluorescence of an acrylamide
gel synthesized substantially in accordance with this
Example 6 (except that 1.9 mg of N-[3-(methacrylamido)-
propyl]-3,4-dihydroxy-9,10-dioxo-2-anthracenesulfonamide
and 35 mg of α,α'-bis [N-[2-(5,5-dimethylborinan-2-yl)-
benzyl]-N-[3-(methacrylamido)propylamino]-1,4-xylene were
used) was determined.
The experiment was conducted in a Shimadzu RF-5301
PC spectrofluorimeter equipped with a variable
temperature attachment (excitation at 470 nm, slits 3/10
nm, high sensitivity). The acrylamide gel was attached
to a piece of a glass slide which was glued in a PMMA

fluorescence cell at a 5° angle. The cell was filled
with 2.5 ml of PBS (pH=7.4) and heated to 37°C. Stock
solutions of glucose (1)0 mM and 500 mM) in PBS (pH=7.4)
were prepared and heated to 37°C in a water bath. An
aliquot of heated glucose stock solution was added to the
PMMA cell periodically while the fluorescence intensity
at 550 nm was monitored as a function of time (1
measurement every 2 minutes). Glucose concentration in
the PMMA cell was measured using a YSI Model 2300 STAT
plus glucose analyzer. The results, shown in Figure 9,
show that the addition of glucose reduces the fluorescent
intensity of the indicator hydrogel. The same effect is
seen in Figure 10, which shows the effect of glucose on
the fluorescence spectrum of the same type of gel.
That effect is beJieved to occur because of the
following considerations. The methacrylamide monomer of
Alizarin Red S (reporter molecule) contains a vicinal
diol functionality and monomer functionality (see
structure below). In i.queous solution and in organic
solvents, the Alizarin Red S and bis-boronate recognition
element monomers (see structure below) are capable of
reversible reaction with each other to form a boronate
ester. The boronate ester molecule formed in this
reversible reaction is fluorescent, while the Alizarin
Red S monomer by itself displays virtually no
fluorescence emission in aqueous solution and in organic
solvents, such as MeOH. Thus upon binding to the glucose
recognition element, Alizarin Red S changes its optical
properties, such as absorbance and quantum yield of
fluorescence, for example.

A solution of Alizarin Red S with monomer
functionality and glucose recognition element with
monomer functionality can be prepared together with a
hydrogel monomer and a crosslinker. Copolymerization of
this mixture produces a hydrogel material which is
diffusable to various small and medium size molecules;
thus it is capable of analyte detection and quantitation.
An analyte, such as glucose for example, would diffuse
inside the hydrogel matrix and displace the reporter
molecule previously bound to the recognition element.
This event causes a change in the optical properties of
the hydrogel film since it now contains a greater number
of reporter molecules unbound to the recognition element.
The modulation of the fluorescence of the indicator
compound (which contains two recognition elements)
prepared in this example by glucose and lactate was also
determined. The experiment was conducted in a Shimadzu
RF-5301 PC spectrofluorimeter equipped with a variable
temperature attachment (excitation at 470 nm, slits 5/10
nm, low sensitivity). The acrylamide gel was attached to
a piece of a glass slide which was glued in a PMMA
fluorescence cell at a 45° angle. The cell was filled
with 2.5 ml of PBS (pH=7.4) and heated to 37°C in a water

bath. A stock solution of sodium lactate (100 mM) in PBS
(pH=7.4) was prepared and heated to 37 °C in a water bath.
Stock solutions of glucose (100 mM and 500 mM) in PBS
(pH=7.4) were prepared and heated to 37°C in a water
bath. An aliquot of heated lactate stock solution was
added to the PMMA cell periodically while the
fluorescence intensity at 550 ran was monitored as a
function of time (1 measurement every 2 minutes), until
the lactate concentration reached 8 mM. Then, an aliquot
of heated glucose stock solution was added to the PMMA
cell periodically while the fluorescence intensity at 550
nm was monitored as a function of time (1 measurement
every 2 minutes). Glucose concentration in the PMMA cell
was measured using a YSI Model 2300 STAT plus glucose
analyzer. The results shown in Figure 11, show that the
addition of lactate had no significant effect on the
fluorescent intensity of the indicator hydrogel, and the
subsequent addition of glucose reduced the fluorescent
intensity of the indicator hydrogel.
Example 7
Single-methacrylamide monomer of bis-boronate-anthracene:

A. 9-chloromethyl-10-[ [2- (2-hydroxyethoxy) ethylamino] -
methyl]anthracene hydrochloride salt.
To a suspension of 9,10-bis(chloromethyl)anthracene
(5.18 g, 18.8 mmole, ,.99 equiv. ) in 200 mL of NMP was

added 2-(2-aminoethoxy)ethanol (0.495 g, 0.475 mL, 4.71
mmole) . The mixture was stirred in the dark for 17
hours. At this time, the reaction mixture was
concentrated to ~ 50 nL under vacuum at 50°C. The
residue was purified by silica gel chromatography (150 g
gravity grade silica gel, 0-10% CH3OH/CH2Cl2) to yield
0.425 g (24%) of a yellow/orange solid.
TLC: Merck silica gel 60 plates, Rf 0.72 with 70/30
CH2Cl2/CH3OH, see with UV (254/366), ninhydrin stain.
HPLC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm
column, 0.100 mL injection, 2 mL/min, 370 nm detection, A
- water (0.1% HFBA) and B = MeCN (0.1% HFBA) , gradient
10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min,
100% B 2 min, retention, time 16.1 min.

B. 9-[[2-(2-hydroxyethoxy)ethylamino]methyl]-10-[[(3-
methacrylamido) propylamino] methyl] -anthracene.
To a suspension of N-(3-aminopropyl)methacrylamide
hydrochloride salt (3.33 g, 17.2 mmole, 4.2 equiv.), DIEA
(5.19 g, 7.00 mL, 40.1 mmole, 9.8 equiv.) and - 3 mg of
BHT in 125 mL CHCl3 at 23°C was added dropwise a solution
of 9-chloromethyl-10-[[2-(2-hydroxyethoxy)ethylamino]-
methyl]anthracene hydrochloride salt (1.56 g, 4.10 mmole)
in 25 mL of CHCl3. The mixture was subsequently stirred
in the dark for 92 hours. At this time, the reaction
mixture was filtered and washed with 2 x 40 mL of NaHCO3

(saturated aqueous solution). The organic extract was
dried over anhydrous Na2SO4, filtered and concentrated to
yield a sticky orange solid which was purified by alumina
chromatography (50 g activated neutral alumina, 0-5%
CH3OH/CH2Cl2) to yield C.364 g (20%) of an orange solid.
TLC: Merck silica gel 60 plates, Rf 0.16 with 70/30
CH2Cl2/CH3OH, see with UV (254/366), ninhydrin stain
HPLC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm
column, 0.100 mL inject ion, 2 mL/min, 370 nm detection, A
= water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient
10% B 2 min, 10-80% B ever 18 min, 80-100% B over 2 min,
100% B 2 min, retention time 16.85 min.

C. 9-[N-[2-(5,5-dimethylborinan-2-yl)benzyl]-N-[3-
(methacrylamido) propyl amino] methyl] -10- [N- [2- (5,5-
dimethylborinan-2-yl)fcenzyl] -N- [2- (2-hydroxyethoxy) -
ethylamino] methyl] anti racene. (Single-me thacrylamide
monomer)
A solution of 9-|[2-(2-hydroxyethoxy)ethylamino]-
methyl]-10-[[(3-methac xylamido)propylamino]methyl]-
anthracene (0.343 g, (.763 mmole), DIEA' (0.965 g, 1.30
mL, 9.8 equiv.) and C-bromomethylphenyl)boronic acid

neopentyl ester (1.09 g, 3.85 mmole, 5.0 equiv.) in 20 mL
CHCl3 at 23°C was stirred in the dark for 25 hours. At
this time, the reaction mixture was concentrated
initially by rotary evaporation, then using a vacuum pump
to remove DIEA. The residue was purified by alumina
column chromatography 40 g activated neutral alumina, 0-
10% CH3OH/CH2Cl2) to yield 0.299 g (46%) of a yellow
orange solid. This compound may be co-polymerized with a
suitable monomer as described previously, deprotected,
and used to detect glucose.
FAB MS: Calc=d for C51H65B2N3O7 [M]+ 854; Found [M + 1] +
855.
TLC: Merck basic alumina plates, Rf 0.35 with 95/5
CH2Cl2/CH3OH, see with UV (254/366) . .
HPXC: HP 1100 HPLC chromatograph, Vydac 201TP 10 x 250 mm
column, 0.100 mL injection, 2 mL/min, 370 nm detection, A
= water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient
10% B 2 min, 10-80% B over 18 min, 80-100% B over 2 min,
100% B 2 min, retention time 19.7 min.

Example 8
Dual-methacrylate monomer of bis-boronate-anthracene

A. 9,10-bis [N- [2- (5, 5-dimethylborinan-2-yl)benzyl] -N-
[2- (2-methacroyloxyethoxy) ethylamino]methyl] anthracene.
A solution of 9,13-bis[N-[2-(5,5-dimethylborinan-2-
yl)benzyl]-N-[2-(2-hydroxyethoxy)ethylamino]methyl]-
anthracene (0.100 g, 0.120 mmole; see Example 2),
methacrylic acid (0.112 g, 0.110 mL, 1.30 mmole, 10.8
equiv.), DCC (0.316 g, 1.53 mmole, 12.8 equiv.) and N,N-
dimethylamino-pyridine (0.014 g, 0.11 mmole, 0.92 equiv.)
in 5 mL CH2Cl2 was stirred at 0°C fcr 1 hour, then 23°C
for 22 hours. At this time, the reaction mixture was
filtered and concentre ted by rotary evaporation. The
residue was purified by alumina column chromatography (30
g activated neutral alumina, 0-2% CH3OH/CH2Cl2) to yield
0.030 g (26%) of a yellow solid. This compound may be
co-polymerized with a suitable monomer as described
previously, deprotectetd, and used to detect glucose.
FAB MS: Calc=d for C56H70B2N2010 [M]+ 953; Found [M]+ 951
(weak molecular ion peak).

TLC: Merck basic alumina plates, Rf 0.67 with 95/5
CH2Cl2/CH3OH, see with UV (254/366).
HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column 0.100 mL injection, 0.75 mL/min, 2
mL injection loop, 37) nm detection, A = water (0.1%
HFBA) and B = MeCN (0 1.% HFBA) , gradient 10% B 2 min, 10-
80% B over 18 min, 80 -100% B over 2 min, 100% B 2 min,
retention time 19.6 min.
Example 9
Dual 5-aminopentyl bis-boronate-anthracene

A. 9,10-bis [ [5- (t-BOC)-aminopentylamino]methyl]-
anthracene.
A suspension of 9,10-bis(chloromethyl)anthracene
(0.28 g, 1 mmole), DIEA (7.0 mL, 40 mmole), mono-t-
butoxycarbonyl 1,5-diaminopentane (3.75 g, 10 mmole), and
50 ml of CHCl3 was stirred in the dark for 2 days at 45°C.
The solution was washed with saturated H2O/NaHCO3, the
organic phase was dried (Na2SO4), and the solvent was
evaporated. The residue was purified by alumina
chromatography (40 g activated neutral alumina, 95/5 %
vol. CH2Cl2/MeOH) to yield 0.55 g of viscous oil. This
material was used as is for the next step.

B. 9,10-bis [N- [2- (5,5--dimethylborinan-2-yl)benzyl] -N-
[5-(t-BOC)-aminopentylamino]methyl]anthracene.
A solution of 9,1)-bis[ [5-(t-BOC)-aminopentylamino]-
methyl]anthracene (0.3 g, 0.49 mmole), DIEA (0.35 mL, 2
mmole), and (2-bromome;hylphenyl)boronic acid neopentyl
ester (0.566 g, 2.0 mmole) in 20 mL CH2Cl2 was stirred in
the dark for 2 days at 25°C. At this time, the reaction
mixture was concentrated in vacuo and the residue was
purified by alumina chromatography (60 g of activated
neutral alumina, 98/2 % vol. CH2Cl2/MeOH) to yield 0.401 g
of yellow oil. This material was used as is for the next
step.

C. 9,10-bis[N-(2-boronobenzyl)-N-[5-aminopentylamino]-
methyl]anthracene trifluoroacetic acid salt.

9,10-bis[N-[2- (5, 5-dimethylborinan-2-yl)benzyl]-N-
[5-(t-BOC)-aminopentylamino]methyl]anthracene (0.4 g,
0.39 mmole) was dissolved in 20 ml of CH2Cl2/TFA (80/20 %
vol.). The solution was stirred for 12 hours, the
solvent was evaporated, and the residue was washed with
10 ml of ether. A total of 373 mg of solid was obtained
(72% yield). Product was ~80% pure by RP-HPLC. This
compound may be co-polymerized with a suitable monomer as
described previously, deprotected, and used to detect
glucose.
HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.050 mL injection, 0.75 mL/min,
360 nm detection, A = water (0.1% HFBA) and B = MeCN
(0.1% HFBA), gradient 10% B 2 min, 10-80% B over 18 min,
80-100% B over 2 min, 100% B 2 min, retention time 16.0
min.
Example 10

A. N-2-(tert-butoxycarbonyl)aminoethyl-4-
bromonaphthalene-1,8-dicarboximide:
N-t-Boc-ethylened lamine (Fluka, 1.6 g, 10 mmole) and
4-bromo-l,8-naphthalic anhydride (Aldrich, 2.77 g, 10
mmole) were combined with 60 ml of anhydrous ethanol, the

suspension was stirred at 60°C for 20 hours, cooled to
room temperature, and filtered. The obtained solid was
washed with 30 ml of cold EtOH and dried under vacuum.
Yield 3.84 g (91%). NMF (CDCl3): 1.28 (9H, s) ; 3.52 (2H,
t); 4.35 (2H, t); 4.92 (1H, s);7.84 (1H, t); 8.04 (1H,
d) ; 8.42 (1H, d); 8.58 (1H, d); 8.67 (1H, d).

B. N-2- (tert-butoxycarbonyl) aminoethyl-4- (N' -
methylaminoethylamino)naphthalene-1,8-dicarboximide:
N-Methylethylenedlamine (1.48 g, 20 mmole) was
combined with 2 ml of --methyl-2-pyrrolidinone (NMP)
followed by addition o: N-2-(tert-
butoxycarbonyl)aminoethyl-4-bromonaphthalene-l,8-
dicarboximide (0.35 g, 0.845 mmole). The resulting
solution was stirred at 45°C for 40 hours after which NMP
and N-methylethylenediamine were evaporated under vacuum.
The obtained residue was subjected to column
chromatography (20 g of silica gel, initially CH2Cl2/MeOH
(90/10), then CH2Cl2/MeCH/Et3N (75/20/5)). A yellow solid
was obtained (0.311 g, 89 % yield). Purity was checked by
RP-HPLC.

C. N-aminoethyl-4-(N -aminoethylene-N'-
[2- (borono)benzyl]methylamino)naphthalene-l, 8-
dicarboximide trifluoroacetic acid salt:
N-2- (tert-butoxycarbonyl)aminoethyl-4-(N'-
methylaminoethylamino; naphthalene-1, 8-dicarboximide (0.3
g, 0.73 mmole), 2-broromethylphenyl boronic acid, pinacol
ester (0.6 g, 2 mmole), N,N-diisopropyl-N-ethylamine (1.3
ml, 8 mmole), and 10 nl of CH2Cl2 were combined. The
solution was stirred for 20 hours, followed by addition
of 2 g of PS-Trisamine resin (Argonaut Technologies, 3.38
mmol/g). The reaction mixture and resin were agitated
for 10 hours after which the resin was removed by
filtration and washed with CH2Cl2 (2X20 ml) . Combined
CH2Cl2 solutions were evaporated and dried under vacuum.

Methylene chloride solution containing 20% vol. TFA and
5% vol. triisopropyl silane was added to the resulting
orange residue. The resulting solution was stirred at
room temperature for 10 hours, after which the solvent
was evaporated and the residue triturated with ether to
yield a yellow solid. The solid was filtered and dried
in vacuum (yield 580 mg). Purity of the material was
checked by RP-HPLC. The solid was used as is in the next
step.

D. N-(3-Borono-5-nitrobenzamido)ethyl-4-(N'-
aminoethylene-N' -
[2 - (borono)benzyl]methy lamino) naphthalene-1, 8-
dicarboximide:
N-aminoethyl-4-(N'-aminoethylene-N'-
[2-(borono)benzyl]methylamino)naphthalene-1,8-
dicarboximide trifluoroacetic acid salt (0.225 g, 0.4
mmole), 3-carboxy-5-nitrophenylboronic acid (0.085 g, 0.4
mmole), diphenylphosphoryl azide (0.13 ml, 0.6 mmole),
and 2 ml of anhydrous [MF were combined. N,N-
diisopropyl-N-ethyl amine (0.7 ml, 4 mmole) was added and
the solution was stirred for 20 hours. Ether (10 ml) was
added to the reaction nixture and the insoluble residue
was separated and sonicated with 5 ml of CH2Cl2 to yield
an orange solid which was filtered and dried under vacuum
(38 mg, 15% yield) . Purity of the solid was checked by
RP-HPLC. NMR (dmso-d6/020, 90/10): 6 2.32 (3H, s); 2.82
(2H, t); 3.58 (2H, t); 3.65 (2H, t), 3.70 (2H, s); 6.65
(1H, d) ; 7.0-7.3 (4H, m ; 7.68 (1H, t) ; 8.18 (1H, d) ;
8.42 (1H, d); 8.47 (1H, d); 8.1-8.35 (3H, m) .
E. Test of N- (3-borono-5-nitrobenzamido) ethyl-4-(N' -
aminoethylene-N' ' -
[2- (borono)benzyl]mettylamino) naphthalene-1,8-
dicarboximide for interaction with glucose as monitored
by fluorescence
This experiment was conducted in MeOH/phosphate
buffered saline, (PBS, 10 mM, pH=7.4). The concentration
of N-(3-borono-5-nitrobenzamido)ethyl-4- (N' -
aminoethylene-N'- [2-
(borono) benzyl]methylaimino) naphthalene-1, 8-dicarboximide
in MeOH/PBS, (50/50 vol. %) was 15 M. The glucose

concentration was vared from 0 mM to 50 mM, and the L-
sodium lactate concentration was varied from 0 mM to 7
mM. The experiment was conducted in a Shimadzu RF-5301
PC spectrofluorimeter excitation wavelength was set at
430 nm, emission was monitored in the 480-650 nm range,
slit width 3/1.5 nm, high sensitivity of PMT.
The results are shown in Figures 12 and 13, which
show that the fluorescence of the indicator of this
example was affected by the presence of glucose, but not
by the presence of lactate.
Example 11
6-(Cyclohexanecarboxamido)hexylamine indicator monomer

A. 9- [N- [3- (methacrylamido)propylamino]methyl] -10-N-
[(6-aminohexylamino)methyl]anthracene. To a solution of
3-aminopropylmethacrylamide (0.775 g, 5.45 mmol, 10.0
equiv.) and tert-butyl N-(6-aminohexyl)carbamate (1.18 g,

5.45 mmol, 10.0 equiv.) and several crystals of BHT in
200 mL CHCl3 was added 9,10-bis(chloromethyl)anthracene
(0.150 g, 0.545 mmol). The reaction mixture was
subsequently stirred in the dark at ambient temperature
for 4 days. At this time, the CHCl3 was evaporated and
the residue was dissolved in 100 mL ether. The organic
layer was extracted w: th 8 x 125 mL sat'd aqueous NaHCO3 •
and 5 x 200 mL phosphite buffer (0.4 M, pH 7.0). The pH
of the combined phosphate buffer washes was adjusted to
pH 11 by addition of Na2CO3 (sat'd aqueous solution),
followed by extraction with 5 x 300 mL CH2Cl2. The
combined organic layers were concentrated and the residue
dissolved in 5 mL of 1 20% solution of TFA in CH2Cl2. The
mixture was stirred at ambient temperature for 2 hours.
At this time, the reaction mixture was extracted with 4 x
10 mL sat'd aqueous NaHCO3. The pH of the combined
aqueous layers was adjusted to pH 11 by addition of Na2CO3
(sat'd aqueous solution), followed by extraction with 4 x
75 mL CH2Cl2. The combined organic extracts were dried
over anhydrous Na2SO4, filtered and concentrated in vacuo
to yield 0.068 g (27%) of product.
TLC: a) Merck Silica Gel 60 plates, Rf 0.16
with 70/30 CH2Cl3/CH3OH, see with UV (254/366), prior
to deprotection; Rf 0.27 with 85/14.5/0.5
CH2Cl2/CH3OH/iPrNH2, see with UV (254/366), final
product.
HPLC: HP 1100 HI L.C chromatograph, Waters 8 x 100 mm
NovaPak HR C18 column, 0.100 mL injection, 0.75
mL/min, 0.400 ml injection loop, 360 nm detection, A
= water (0.1% HNBA) and B = MeCN (0.1% HFBA) ,
gradient 10% B : min, 10-80% B over 18 min, 80-100%
B over 2 min, 100% B 2 min, retention time 15.5 min.

B. 9- [N- [3- (methacrylamido)propylamino]methyl] -10- [N-
[6- (cyclohexanecarboxamido) hexylamino]methyl] anthracene.
To a solution of 9-[N-[3-
(methacrylamido)propylamino]methyl]-10-N-[6-
aminohexylamino)methyl]anthracene (1.68 g, 3.63 mmol) and
a few crystals of EHT in 20 mL CH2Cl2 at ambient
temperature was adc ed dropwise a solution of
cyclohexanecarboxy.'.ic acid N-hydroxysuccinimide ester
(0.845 g, 3.76 mmo., 1.03 equiv.) over a 1 hour period.
The reaction was subsequently stirred in the dark at
ambient temperature for 16 hours. At this time, the
reaction mixture was concentrated in vacuo and the
residue dissolved in 105 mL of a solution of 90/15 ether/
CH2Cl2. The organiC layer was extracted with 4 x 225 mL
phosphate buffer ,0.4 M, pH 7.0). The pH of the combined
phosphate buffer washes was adjusted to pH 11 by addition
of Na2CO3 (sat'd aqueous solution), followed by extraction
with 6 x 500 mL CH2Cl2. The combined organic layers were
dried over anhydicus Na2SO4, filtered and concentrated in
vacuo to yield 1 2 g (60%) of product.
TLC: Merck Silica Gel 60 plates, Rf 0.30 with
85/14.5/0.5 CH2Cl2/CH3OH/iPrNH2, see with UV (254/366)
HPLC: HP 11)0 HPLC chromatograph, Waters 8 x 100 mm
NovaPak HR 318 column, 0.100 mL injection, 0.75
mL/min, 0.4 30 mL injection loop, 360 nm detection, A
- water (0.1% HFBA) and B = MeCN (0.1% HFBA),
gradient 10% B 2 min, 10-80% B over 18 min, 80-100%

C. 9-[N-(2-boronobenzy][-N-[3-
(methacrylamido) propylamine]methyl] -10- [N- (2-
boronobenzyl) -N- [6-(cyclohexanecarboxamido) hexylamino] -
methyl] anthracene. A solution of 9-[N-[3-
(methacrylamido)propylamino]methyl] -10-[N-[6-
(cyclohexanecarboxamido)hexylamino]methyl]-anthracene .
(1.0 g , 1.8 mmol), DIEA (1.81 g, 2.44 mL, 14.0 mmol, 7.8
equiv.), 2-bromomethylphenylboronic acid pinacol ester
(2.14 g, 7.20 mmol, 4.( equiv.) and a few crystals of BHT
in 30 mL CHCl3 was stirred in the dark at ambient
temperature for 60 hours. At this time, the reaction
mixture was concentrated and the residue (9-[N-[2-
(4,4,5,5,-tetramethyl-: ,3,2-dioxaborolano)benzyl]-N-[3-
(methacrylamido)propylamino] methyl] -10-[N-[2-(4,4,5,5,-
tetramethyl-1, 3, 2-dioxaborolano) benzyl] -N- [ 6-
(cyclohexanecarboxamide) hexylamino]methyl]anthracene)
suspended in 150 mL ether. The organic layer was washed
with 4 x 50 mL phosphate buffer (0.4 M, pH 7.0). The
organic layer was concentrated and the residue dissolved
in ether in 200 mL 0.1 N aqueous HCl. The aqueous layer
was washed with 3 x 50 ml. 1:1; ether: ethyl acetate and
the pH was adjusted to pK 11 by addition of Na2CO3 (sat'd
aqueous solution), followed by extraction with 3 x 150 mL
CH2Cl2. The combined organic layers were dried over

anhydrous Na2SO4, filtered and concentrated in vacuo to
yield a red oily compound. The residue was dissolved in
ether and concentrateD in vacuo to yield 1.17 g (85%) of
a yellow solid product,

D. N,N-dimethylacrylamide hydrogel with 9-[N-(2-
boronobenzyl) -N- [3- (methacrylamido) propylamino]methyl] -
10- [N- (2-boronobenzyl)- N- [6-
(cyclohexanecarboxamide)hexylamino] methyl]anthracene. A
solution of N,N-dimethylacrylamide (40% wt.) and N,N'-
methylenebisacrylamide (0.8% wt.) in phosphate buffer,
pH=7.4, 200 mM was prepared. 9-[N-(2-Boronobenzyl)-N-[3-
(methacrylamido) propylamino]methyl] -10- [N- (2-
boronobenzyl)-N-[6-(cyclohexanecarboxamido)hexylamino]
methyl] anthracene (18 mg, 2.15X10-5 mole) and 60 mg of
fructose were combined with 2 mL of MeOH. This solution

was sonicated until all of the fructose dissolved and was
subsequently evaporatec to yield a solid. To this solid,
1 mL of phosphate buffer solution containing monomers was
added. After sonicaticn for 10 min this solution was
filtered through a 0.2 uM PTFE membrane filter. Aqueous
ammonium persulfate (2C μL, 5% wt.) was combined with the
formulation. The resulting solution was placed in glove
box purged with nitrogen. An aqueous solution of
N,N,N',N'-tetramethylethylenediamine (40 μL, 5% wt.) was
added to the monomer formulation to accelerate
polymerization. The resulting formulation was poured
into a mold constructec from glass microscope slides and
a 100 uM stainless steel spacer. After being kept for 8
hours in a nitrogen atmosphere, the mold was placed in
phosphate buffered saline (pH=7.4), the microscope slides
were separated, and the hydrogel was removed. The
hydrogel was washed with 100 mL of phosphate buffered
saline (PBS) containing 1 mM lauryl sulfate sodium salt
and 1 mM EDTA tetrasodium salt for 3 days, the solution
being changed every day, followed by washing with
EtOH/PBS (20/80 by vol , 3 x 100 mL), and finally with
PBS (H=7.4, 3 x 100 mL. The resulting hydrogel film was
stored in PBS (pH=7.4) containing 0.02% wt. sodium azide
and 1 mM EDTA tetrasod: um salt.
E. Modulation of Fluorescence with Glucose.
The modulation of the fluorescence of the 6-
(cyclohexanecarboxamido)hexylamine indicator/DMA hydrogel
film prepared in this example by glucose and lactate was
determined. Figure 14 shows the relative fluorescence
emission (I @ 430 nm) of the hydrogel film in PBS (pH 7.4
containing 0.02% NaN3 and 1 mM EDTA) containing 0 to 20 mM
α-D-glucose, 0 to 10 mM I-sodium lactate, and 0-20 mM α-
D-glucose in the presence of 4 mM L-sodium lactate. The

hydrogel film (100 μM thickness, 8 mm diameter disk) was
mounted in a PMMA cuvette at a 45° angle. All
measurements were made at 37°C in a Shimadzu RF-5301
spectrofluorometer with excitation at 370 nm (slit = 3
nm) and emission at 4 30 nm (slit = 3 nm) at low PMT
sensitivity. Glucose and L-sodium lactate concentrations
were checked using the YSI Model 2300 STAT plus glucose
analyzer. Error bars are standard deviation with
triplicate values for each data point. The fluorescence
was affected by the presence of glucose, but not by the
presence of lactate. Moreover, the presence of lactate
(4 mM) had no significant effect on the 0-20 mM glucose
calibration curve.
EXAMPLE 12
2-(carboxyethyl)amine indicator monomer

Chemical Name: 9- N-(2-boronobenzyl)-N-[3-
(methacrylamido)propylamino]methyl]-10-[N-(2-
boronobenzyl)-N-[2 -
(carboxyethyl)amiro]methyl]anthracene (uncapped)
Chemical Formula: C40H45B2N3O7
MW: 701.4
Physical appearance: faint yellow powder
Solubility: PBS/methanol, methanol, ethanol,

chloroform, dichloromethane
Capped Indicator: 9-[N-[2-(4,4,5,5,-tetramethyl-
1, 3, 2-dioxaborolano)benzyl]-N-[3-
(methacrylamido)propylamino]methyl] -10-[N-[2-
(4,4,5,5,-tetramethyl-1,3,2-dioxaborolano)benzyl]-N-
[2-(carboxyethyl)amino]methyl]anthracene.
I. Synthesis

A. 9-[N-[3-(methacrylamido)propylamino]methyl]-10-[N-
[2- (tert-butoxycarbonyl)ethylamino]methyl]anthracene. To
a solution of 3-aminopropylmethacrylamide (12.9 g, 90.7
mmol, 4.99 equiv.), β-alanine tert-butyl ester (13.2 g,
90.9 mmol, 5.00 equiv.] and several crystals of BHT in
700 mL CHCl3 was added 9, 10-bis(chloromethyl)anthracene
(5.00 g, 18.2 mmol). The reaction mixture was
subsequently stirred in the dark at 30 °C for 88 hours.
At this time, the CHCl2 was evaporated and the residue was
dissolved in 500 mL ether. The solution was stirred for
1 hour at which time salts had precipitated from
solution. The ether solution was filtered and
subsequently extracted with 10 x 350 mL sat'd aqueous
NaHCO3. The ether layer was further extracted with 6 x
350 mL phosphate buffer (0.2 M, pH 6.5). The pH of the
combined phosphate buffer washes was adjusted to pH 11-12
by addition of Na2CO3 (sat'd aqueous solution), followed
by extraction with 6 x 500 mL CH2Cl2. The combined organic

layers were dried over anhydrous Na2SO4, filtered and
concentrated in vacuo to yield an oily crude product.
The crude product was purified by silica gel
chromatography (50 g flash grade silica gel, 0-5%
MeOH/CH2Cl2 step gradient) to yield 2.04 g of a sticky
yellow solid (23%).
TLC: Merck Silica Gel 60 plates, Rf 0.29 with 90/10
CH2Cl2/CH3OH, see with UV (254/366) and ninhydrin
stain.
HPLC: HP 1100 HPIC chromatography Waters 5 x 100 mm
NovaPak HR C18 column, 0.100 mL injection, 0.75
mL/min, 1.500 ml injection loop, 280 nm detection, A
- water (0.1% HEBA) and B = MeCN (0.1% HFBA),
gradient 10% B 2 min, 10-80% B over 18 min, 80-100%
B over 2 min, 100 % B 2 min, retention time 17.0
min.

B. 9-[N-[2-(4,4,5,5 -tetramethyl-1,3,2-
dioxaborolano)benzyl] • N-[3-
(methacrylamido)propy: amino] methyl] -10-[N-[2- (4,4,5,5,-
tetramethyl-1,3,2-dioxaborolano) benzyl] -N- [2- (tert-
butoxycarbonyl) ethylamino]methyl] anthracene.
A solution of 9-[N-[3-
(methacrylamido)propyl amino] methyl]--10-[N-[2-(tert-

butoxycarbonyl)ethylamino)methyl]anthracene (1.5 g , 3.1
mmol), DIEA (3.16 g, 4.26 mL, 24.4 mmol, 7.9 equiv.), 2-
bromomethylphenylboronic acid pinacol ester (3.64 g, 12.2
mmol, 3.9 equiv.) and a few crystals of BHT in 50 mL CHCl3
was stirred in the dark at ambient temperature for 16
hours. At this time, the reaction mixture was
concentrated and the residue suspended in 200 mL ether.
The ether layer was extracted with 3 x 125 mL phosphate
buffer (0.2 M, pH 7.0) dried over anhydrous Na2SO4,
filtered and concentrated in vacuo to yield a crude
product.The residue was triturated with hexanes to yield
2.14 g (76%) of a white solid.
HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.200 mL injection, 0.75
mL/min, 1.500 mL injection loop, 280 nm detection, A
= water (0.1% HFBA)- and B = MeCN (0.1% HFBA) ,
gradient 10% B 2 min, 10-80% B over 18 min, 80-100%
B over 2 min, 10C% B 2 min, retention time 19.2 min.

C. 9-[N-(2-boronobenzyl)-N-[3-
(methacrylamido) propylamino] methyl] -10- [N- (2-
boronobenzyl) -N- [2- (curboxyethyl) amino]methyl] anthracene.
A solution of 9-[N-[2 -(4,4,5,5,-tetramethyl-1,3, 2-
dioxaborolano)benzyl] -N-[3-

(methacrylamido)propylamino]methyl]-10-[N-[2- (4,4,5,5,-
tetramethyl-1,3,2-dioxaborolano)benzyl]-N-[2-(tert-
butoxycarbonyl)ethylamino]methyl]anthracene (0.294 g,
0.319 mmol) in 5 mL of 20% TFA/CH2Cl2 was stirred in the
dark at ambient temperature for 22 hours. At this time,
the reaction mixture was concentrated and the residue
triturated with ether. The residue was dissolved in 5 mL
90:10 acetone/water and stirred for 2 hours. At this
time, the reaction mixture was concentrated and the
residue triturated with water and PBS (pH 7.4 containing
0.02% NaN3 and 1 mM EDTA) resulting in the recovery of
0.062 g (28%) of a light yellow solid.
HPLC: HP 1100 HFLC chromatography Waters 5 x 100 mm
NovaPak HR C18 column, 0.100 mL injection, 0.75
mL/min, 1.500 mL injection loop, 280 nm detection, A
= water (0.1% HF3A) and B = MeCN (0.1% HFBA) ,
gradient 10% B 2 rain, 10-80% B over 18 min, 80-100%
B over 2 min, 10) % B 2 min, retention time 17.4
min.
FAB MS: Glycerol matrix; Calc'd for C46H53B2N3O7 (bis
glycerol adduct) [M] + 813; Found [M + 2]+ 815.
D. N,N-dimethylacrylamide hydrogel with 9-[N-(2-
boronobenzyl) -N- [3- (methacrylamido)propylamines] methyl] -
10- [N- (2-boronobenzyl; -N- [2-
(carboxyethyl)amino]methyl]anthracene. A solution of
N,N-dimethylacrylamide (40% wt.) and N,N'-
methylenebisacrylamide (0.8% wt.) in phosphate buffer,
pH=7.4, 200 mM was prepared. 9-[N-(2-boronobenzyl)-N-[3-
(methacrylamido)propyl amino]methyl]-10-[N-(2-
boronobenzyl)-N-[2-(carboxyethyl)amino]methyl]anthracene
(14 mg, 2.0 x 10-5 mole ) and 60 mg of fructose were
combined with 2 ml of MeOH. This solution was sonicated

until all fructose disolved and evaporated to yield a
solid. To this solid . ml of phosphate buffer solution
containing monomers was added. After sonication for 10
minutes this solution was filtered through 0.2 μM PTFE
filter. Aqueous ammonium persulfate (20 μL, 5% wt.) was
combined with the formaLation. The resulting solution
was placed in a glove box purged with nitrogen. An
aqueous solution of N,N,N',N'-tetrametylethylenediamine
(40 μL, 5% wt.) was adied to the monomer formulation to
accelerate polymerization. The resulted formulation was
poured in a mold constructed from microscope slides and
100 μM stainless steel spacer. After being kept for 8
hours in nitrogen atmosphere the mold was placed in
phosphate buffered sa]ine (10 mM, pH=7.4), the microscope
slides were separated, and the hydrogel was removed. The
hydrogel was washed with 100 ml of phosphate buffered
saline (PBS) containing 1 mM lauryl sulfate sodium salt
and 1 mM EDTA tetrasodium salt for 3 days, the solution
being changed every day, followed by washing with
EtOH/PBS (20/80 by vol ., 3 x 100 ml), and finally with
PBS (pH=7.4, 3 x 100 ml). The resulting hydrogel film was
stored in PBS (10 mM, pH=7.4) containing 0.02% wt. sodium
azide and 1 mM EDTA tetrasodium salt.
II. Modulation of Fluorescence with Glucose.
The modulation of the fluorescence of the 2-
(carboxyethyl)amine indicator/DMA hydrogel film prepared in
this example by glucose and lactate was determined. Figure
15 shows the relative fluorescence emission (I @ 430 ran) of
the hydrogel film in P3S (pH 7.4 containing 0.02% NaN3 and
1 mM EDTA) containing 0 to 20 mM α-D-glucose, 0 to 10 mM L-
sodium lactate, and 0-20 mM glucose in the presence of 3 mM
L-sodium lactate. The hydrogel film (100 μm thickness, 8
mm diameter disk) was mounted in a PMMA cuvette at a 4 5°

angle. All measurements were made at 37°C in a Shimadzu RF-
5301 spectrofluorometer with excitation at 370 nm (slit =
3 nm) and emission at 430 nm (slit = 3 nm) at low PMT
sensitivity. Glucose and L-sodium lactate concentrations
were checked using the YSI Model 2300 STAT plus glucose
analyzer. The data is plotted as the average of triplicate
values for each data point. The fluorescence was affected
by the presence of glucose, but not by the presence of
lactate. Moreover, the presence of lactate (4 mM) had no
significant effect or the 0-20 mM glucose calibration
curve.
EXAMPLE 13
Fluorescent glucose indicator containing two detectable
moieties:

Chemical Name: 9-[N-( 2-boronobenzyl)-N-[3-
(methacrylamido)propylamino]methyl]-10-[N-(2-
boronobenzyl)-N-[3-(N-6-(9-
anthracenecarboxamido hexylamino

carbonyl) ethylamino]methyl] anthracene (uncapped)
Chemical Formula: C73H17B2N507
MW: 1168
Physical appearance: Paint yellow powder
Solubility: PBS/methanol, methanol, ethanol, chloroform,
dichloromethane
Pinacol capped compound:
9-[N-[2- (4,4,5,5,-tetramethyl-1,3,2-
dioxaborolano)benzyl] - N-[3-
(methacrylamido)propyl amino]methyl]-10-[N-[2-(4,4,5,5,-
tetramethyl-l,3,2-dioxaborolano)benzyl]-N-[3-(N-6-(9-
anthracenecarboxamido)hexylamino
carbonylethylaminomethyl]anthracene.

A. 9-Anthracencyl Chloride: Anthracene-9-
carboxylic acid (1.2 g, 5.4xl0~3 mole) was combined with
15 ml of thionyl chloride. The solution was refluxed for
2 hours followed by evaporation of the volatile
components. The obtained solid was dried under high
vacuum for 24 hours yielding 1.3 g of material
(quantitative yield). This material was used as is in
the next step.

B. N- (6-Aminohexyl) -anthracene-9-carboxamide
hydrochloric acid salt: 9-Anthracenoyl chloride (1.3 g,
5.4 mmole) in 50 ml cf anhydrous CH2Cl2 was added dropwise
to 11.6 g of hexamethylenediamine (100 mmole) in 100 ml
of CH2Cl2 at 0°C. The solution was stirred at 0°C for 1
hour then allowed tc warm to room temperature and stirred
overnight. The solvent was evaporated and 200 ml of
water was added to the residue. This mixture was
sonicated and stirred for 1 hour then filtered. The
filtered solid was cried under vacuum for 24 hours. MeOH
(50 ml) and 2 ml of conc. HC1 was added to the solid,
followed by evaporation of MeOH. The resulting solid was
washed with hot CH2Cl2/MeOH (90/10 vol. %) and
recrystallized from MeOH, yielding 0.51 g of the product
(26%). The purity of the product was checked by HPLC.
HPLC: HP 1100 HPLC chromatograph, Waters 5 x 100 mm
NovaPak HR C18 colunr, 0.1 mL injection, 0.75 mL/min
flowrate, 2 mL injection loop, 280 nm detection, A =
water (0.1% HFBA) and B = MeCN (0.1% HFBA) , gradient 10%
B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100
% B 2 min, retention time 16.5 min.

C. 9-[N-[2-(4,4,5,5,-tetramethyl-1,3,2-
dioxaborolano)benzyl] -N- [3-
(methacrylamido)propylamino]methyl] -10- [N-[2- (4,4,5,5,-
tetramethyl-1,3,2-dioxaborolano) benzyl] -N-[3- (N-6- (9-
an thracenecarboxamido) hexylamino
caxbonylethylaminomethjl]anthracene :
9-[N-[2-(4,4,5,5,-tetramethyl-1,3,2-
dioxaborolano) benzyl] -N-[3-
(methacrylamido) propylamino] methyl] -10-[N-[2-(4,4,5,5,-
tetramethyl-1,3,2-dioxaborolano) benzyl] -N- [2-
carboxyethylamino]methyl]anthracene (40 mg, 4.5xl0-5 mole)
was combined with N-(6-aminohexyl)-anthracene-9-
carboxamide hydrochloric acid salt (20 mg, 5.6xl0-5 mole),
diphenylphosphoryl azide (15.4 mg, 5.6xl0-5 mole), and 2
ml of DMF. Diisopropylethylamine(39 20 μL, 2.44xl0-4
mole) was added to the mixture and the solution was
stirred at room temperature for 24 hours. The DMF was
evaporated under high vacuum, the residue was dissolved

in 50 ml of EtOAc and washed with water (3x10 ml). The
EtOAc solution was separated, dried (Na2SO4) , and
evaporated producing 6 mg of solid (87 % yield). Purity
of the material was checked by HPLC.
HPLC: HP 1100 HP] C chromatograph, Waters 5 x 100 mm
NovaPak HR C18 column, 0.1 mL injection, 0.75 mL/min
flowrate, 2 mL injection loop, 280 nm detection, A =
water (0.1% HFBA) and B = MeCN (0.1% HFBA), gradient 10%
B 2 min, 10-80% B over 18 min, 80-100% B over 2 min, 100%
B 2 min, retention time 20.42 min.
FAB mass-spectrum, glycerol matrix: calculated for
C67H75B2N509 (bis glycerol adduct) [M]+=1116, found
[M+l]+=1117.
II . Effect of glucose on fluorescence of indicator
immobilized in hydroge.. film
Preparation of HEMA/Methacrylic acid hydrogel with
glucose indicator:
A 50 % wt. solution of 2-hydroxyethylmethacrylate(4.75 g)
and methacrylic acid ((.25 g) in phosphate buffer,
pH=7.4, 200 mM was prepared. Glucose indicator (11 mg,
1.0 x 10-5 mole) and 60 rag of fructose were combined with
2 ml of MeOH. This solution was sonicated until all
fructose dissolved and evaporated to yield a solid. To
this solid 1 ml of phosphate buffer solution containing
monomers was added. After sonication for 10 minutes this
solution was filtered through 0.2 μM PTFE filter.
Aqueous ammonium persulfate (20 μL, 5% wt.) was combined
with the formulation. The resulting solution was placed
in a glove box purged with nitrogen. An aqueous solution
of N,N,N',N'-tetramethylethylenediamine (40 μL, 5% wt.)
was added to the monomer formulation to accelerate
polymerization. The resulting formulation was poured in

a mold constructed from microscope slides and a 100 μM
stainless steel spacer. After being kept for 8 hours in
a nitrogen atmosphere the mold was placed in phosphate
buffered saline (10 mM, pH=7.4), the microscope slides
were separated, and the hydrogel was removed. The
hydrogel was washed with 100 ml of phosphate buffered
saline (PBS) containirg 1 mM lauryl sulfate sodium salt
and 1 mM EDTA tetrasocium salt for 3 days, the solution
being changed every day, followed by washing with
EtOH/PBS (20/80 by vol., 3 x 100 ml), and finally with
PBS (pH=7.4, 3 x 100 ml). The resulting hydrogel film
was stored in PBS (10 mM, pH=7.4) containing 0.02% wt.
sodium azide and 1 mM EDTA tetrasodium salt.
Effect of glucose and L-sodium lactate on hydrogel
film containing glucose indicator.
The experiment was conducted in a Shimadzu RF-5301
PC spectrofluorimeter equipped with a variable
temperature attachment. Excitation wavelength was set at
370 nm,slits 3/3 nm, low PMT sensitivity, emission was
scanned from 400 to 600 nm. Glucose and L-sodium lactate
concentrations were checked using YSI Model 2300 STAT
plus glucose analyzer.
The hydrogel filn (100 μm thickness, round shape - 8
mm diameter) was mounted in a PMMA cuvette at 45° angle.
Phosphate buffered saline (PBS), pH=7.4 containing the
desired amount of glucose, L-sodium lactate, and glucose
with L-sodium lactate were heated to 37 °C in a water bath
and placed in the PMMA cell containing the mounted
hydrogel. After each addition the PMMA cell was allowed
to equilibrate for 45 min at 37°C. Fluorescence intensity
measurements for each glucose/lactate concentration were
conducted on two different samples and an average value
was used in the calibiation curve. Calibration curves

(Fluorescence Intensity at 430 nm vs. concentration) were
obtained for glucose L-sodium lactate, and glucose in
the presence of 3 mM L-sodium lactate. The results are
shown in Figure 16.
EXAMPLE 14
6-(3-carboxypropiolamido)hoxylamino indicator monomer

Pinacol capped compound:
9- [N-[2- (4,4,5,5,-tetramethyl-1,3,2-
dioxaborolano)benzyl] -N-[3-
(methacrylamido)propylamino]methyl]-10-[N-[2-(4,4,5,5,-
tetramethyl-1,3,2-dioxaborolano)benzyl]-N-[6-(3-
carboxypropionamido)hexylamino]methyl]anthracene.
Uncapped compound:
9-[N-(2-boronobenzyl)-N-[3-
(methacrylamido) propylamino]methyl] --10- [N- (2-
boronobenzyl)-N-[6-(3-
carboxypropionamido)hexylamino]methyl]anthracene.

Synthesis:
The synthesis may be carried out in an analogous
fashion to Example 11 using 9-[N-[3-
(methacrylamido)propylamino]methyl]-10-N-[6-
(hexylamino)methyl]anthracene as the starting material.
In contrast, the amine starting material is reacted with
the N-hydroxysuccinimide (NHS) ester of the mono methyl
ester of succinic acic in place of the NHS ester of
cyclohexanecarboxylic acid used in Example 11. An
additional base hydrolysis step is required to complete
the synthesis.

Chemical Name: N-(3-Methacrylamidopropyl)-4-[2-N-[[2-
(borono)benzyl]-[6-(N- [2-(borono)benzyl]-6-N-
(3-
carboxypropanamidoethyl)aminohexyl]]aminoethylamino]napht
halene-1,8-dicarboximide
Chemical Formula: C47H60B2N6O10
M. W.: 890
The compound may be synthesized as shown below:

EXAMPLE 16
Alternate glucose indicator/monomer excited with visible light

Chemical Name: N-Butyl -4-- [2-N- [ [2- (borono) benzyl] - [ 6- (N-
[2-(borono)benzyl]-6-N-
(2-
methacrylamidoethyl)aminohexyl]] aminoethylamino] naphthale
ne-1,8-dicarboximide
Chemical Formula: C44H51B2N5O7
M. W. : 789.5
The compound may be synthesized as shown below:

WE CLAIM:
1. A method for detecting the presence or concentration of
glucose in a sample which may also contain an alpha-hydroxy acid
or a beta-diketone, which comprises:
a) exposing the sample tc a compound having at least two
recognition elements for glucose, oriented such that the
interaction between the compound and glucose is more stable than
the interaction between the compound and the alpha-hydroxy acid
or beta-diketone, said con pound also containing a detectable
moiety having a detectable quality that changes in a
concentration-dependent manner when said compound is exposed to
glucose in said sample; and
b) measuring any change in said detectable quality to thereby
determine the presence or concentration of glucose in said
sample, wherein the preserce of the alpha-hydroxy acid or the
beta-diketone does not substantially interfere with said
determination, wherein the compound is selected from the group
consisting of:
9-[N-(2-boronobenzyl) -M-[3-(methacrylamido) propyl amino ]
methyl] -10-|N-(2-boronobenzyl)-N-[6-(cyclohexanecarboxamido)
hexylamino]methylanthracene;
9-[N-(2-boronobenzyl) -N-[3-(methacrylamido)propyl ami no ] -
methyl ] -10- [ N- (2-boronobenzyl ) -N- [2- (carboxyethyl ) amino ) methyl ] -
anthracene;
9-[N-(2-boronobenxyl) -N-[3-(methacrylamido)propyl amino]-
methyl ]-10-[N-(2-boronobenzyl)-N-[3-(N-6-(9-anthracenecarbox-
amido)hexylamino carbonyl) ethylamino]methyl ] anthracene;
9-[N-(2-boronobenzyl) -M-[3-(methacrylamido)propylamino]-
methyl ]-10-[N-(2-boronobenzyl)-N-[6-(3-carboxypropionamido)-
hexylamino ] methyl ] anthracene ;

N-(3-Methacrylamidoprocpyl)-4-[2-N-[[2-(borono)benzyl]-[6-
(N-|2-(borono)benzyl]-6-N- (3-carboxypropanamidoethyl)
aminohexyl ] ]-aminoethylamino ] naphthalene-1, 8-dicarboximide;
N-Butyl-4-[2-N-[[ 2- (borono) benzyl]- [-6- (N-[2- (borono)
benzyl]-6-N-(2-methacrylaridoethyl)aminohexyl]]aminoethylamino]-
naphthalene-1 , 8-dicarboximide; and salts thereof.
2. The method as claimed in claim 1,. wherein the sample is
a physiological fluid .
3. The method as claimed in claim 2, wherein the
physiological fluid is selected from the group consisting of
blood, plasma, serum, interstitial fluid, cerebrospinal fluid,
urine, saliva, intraocular fluid, lymph, tears, sweat, and
physiological buffers.
4. The method as claimed in claim 1, wherein the compound
is exposed to the sample in solution.
5. The method as claimed in claim 1, wherein the compound
is immobilized on or within a solid support.
6. The method as claimed in claim 5, wherein the solid
support is a polymeric matrix.
7. A compound selected from the group consisting of:
9- [N- (2-boronobonzyl) -N- [3 - methacrylamido) propylamine-] methyl] -
1 0- [N- (2-boronobenzyl ) -N- [ 6- (cyclohexanecarboxamido) hexylamino]
methyl ] anthracene;

9-[N-(2-boronobenzyl -N-[3-(methacrylamido)propylamino]-
methyl ]- 10-|N-(2-boronobenzyl)-N-[2-(carboxyethyl)amino]methyl]-
anthracene;
9-[N- (2-boronobenzyl)-N-[3-(methacrylamido)propylamino]-
methyl]-10-[N-(2-boronobenzyl)-N-[3-(N-6-(9-anthracenecarbox-
amido) hoxylamino carbonyl) ethyl amino] methyl] anthracene;
9- ( N- (2-boronobenzyl) -N-- [3- (methacrylamido) propylamino] -
methyl ]-10-[N- (2-boronobenzyl)-N-[ 6-(3-carboxypropionamido)-
hexylamino ] methyl] anthracene;
N-(3-Methacrylamidopropoyl)-4-[2-N-[ 2-(borono)benzyl]-[6-
(N-[2-(borono)benzyl]-6-N-(3-carboxypropanamidoethyl)
aminohexy 1 | ] -aminoethylamino] naphthalene-1, 8-dicarboximide;
N-Butyl-4-[2-N-[[2-(borono)benzyl]-|6-(N-[2-(borono)
benzy 1 ) -6-N- (2-methacrylamidioethyl) aminohexyl] ] aminoethyl amino] -
naphthalene-1,8-dicarboximide; and salts thereof.

Compositions and methods for determining the presence or concentration of glucose in a sample which may also contain an alpha-hydroxy acid or a beta-diketone.The method uses a compound having at least two recognition elements for glucose, oriented such that the interaction between the compound and glucose is more stable than the interaction between the compound and
the alpha-hydroxy acid or beta-diketone, such that the presence of the alpha-hydroxy acid or the beta-diketone does not substantially
interfere with said determination.

Documents:

1474-KOLNP-2004-CORRESPONDENCE.pdf

1474-KOLNP-2004-FORM 27.pdf

1474-KOLNP-2004-FORM-27.pdf

1474-kolnp-2004-granted-abstract.pdf

1474-kolnp-2004-granted-assignment.pdf

1474-kolnp-2004-granted-claims.pdf

1474-kolnp-2004-granted-correspondence.pdf

1474-kolnp-2004-granted-description (complete).pdf

1474-kolnp-2004-granted-drawings.pdf

1474-kolnp-2004-granted-examination report.pdf

1474-kolnp-2004-granted-form 1.pdf

1474-kolnp-2004-granted-form 18.pdf

1474-kolnp-2004-granted-form 3.pdf

1474-kolnp-2004-granted-form 5.pdf

1474-kolnp-2004-granted-gpa.pdf

1474-kolnp-2004-granted-reply to examination report.pdf

1474-kolnp-2004-granted-specification.pdf

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Patent Number

230129

Indian Patent Application Number

1474/KOLNP/2004

PG Journal Number

09/2009

Publication Date

27-Feb-2009

Grant Date

25-Feb-2009

Date of Filing

05-Oct-2004

Name of Patentee

SENSORS FOR MEDICINE AND SCIENCE, INC.

Applicant Address

12321 MIDDLEBROOK ROAD, SUITE 210, GERMANTOWN, MD

Inventors:

#	Inventor's Name	Inventor's Address
1	DANILOFF GEORGE Y	1935 POLK COURT, MOUNTAIN VIEW, CA 94040
2	KALIVRETENOS ARISTOTLE G	7106 LASTING LIGHT WAY, COLUMBIA, MD 21045
3	NIKOLAITCHIK ALEXANDRE V	7104 OBERLIN CIRCLE, FREDERICK, MD 21703

PCT International Classification Number

C07D 417/00

PCT International Application Number

PCT/US03/07938

PCT International Filing date

2003-03-14

PCT Conventions:

#	PCT Application Number	Date of Convention	Priority Country
1	60/363, 885	2002-03-14	U.S.A.
2	10/187,903	2002-07-03	U.S.A.