Title of Invention	COMPOSITIONS SUITABLE FOR PREPARING SUBCUTANEOUS IMPLANTS AND A PROCESS FOR PREPARING THE SAME
Abstract	ABSTRACT IN/PCT/2001/936/CHE "Composition suitable for the preparation of subcutaneous implants and a process for preparing the same" Compositions comprising a peptide and a polyactic-glycolic acid (PLGA) wherein the distribution of the size of the particles of the peptide in the PLGA results highly heterogeneous, suitable to the preparation of subcutaneous implants having a release time equal to 6 months.

Title of Invention

COMPOSITIONS SUITABLE FOR PREPARING SUBCUTANEOUS IMPLANTS AND A PROCESS FOR PREPARING THE SAME

Abstract

ABSTRACT IN/PCT/2001/936/CHE "Composition suitable for the preparation of subcutaneous implants and a process for preparing the same" Compositions comprising a peptide and a polyactic-glycolic acid (PLGA) wherein the distribution of the size of the particles of the peptide in the PLGA results highly heterogeneous, suitable to the preparation of subcutaneous implants having a release time equal to 6 months.

Full Text	The present invention refers to compositions comprising a peptide and polylacllc-glycollc acid suitable for the preparation of subcutaneous implants. Prior art Compositions made up of mixtures of a drug with a polymer of lactic acid or a polymer of glycolic acid or with a copolymer of lactic acid and glycolic acid, as described in the U.S. patent 3.773.919 (Du Pont) are well known . These compositions are indicated for potential administration and have the characteristics of releasing effective quantities of the drug over a set period of time. The drug and the polymeric substance can be combined in accordance with any of the known techniques or the particles of the drug can be coated in the polymer operating In accordance with known techniques. The U.S. patent 4.767.628 (ICI) describes compositions containing a peptide and a polymer of lactic acid or a copolymer of lactic acid and giycolic ackl. When preparing the compositions, the pestle and the (oo)polymer are dissolved in a solvent which can be the same or different for the two substances, for Example dioxane or water, and then the two solutions are mixed. The subsequent operations consist of removing the solvent at low temperature and in extruding the powder obtained in this way. In this way a composition in the form of cylinders is obtained in which the peptide is distributed homogeneously throughout the polymer. It is already known from the U.S. patent 5.366.734 (Zeneca) that the compositions covered by the U.S. patent 4.767.628 referred to above can be used In preparing subcutaneous implants. The polymer of lactic acid and the copolymer of lactic acid and giycolic acid are incompatible with the peptide therefore diffusion of the peptide through the polymer is impossible. When these implants are introduced into a buffer solution at 37 °C, the water peptides over a limited period of time, generally of around 3 months. Summary of the Invention The applicant has now found compositions suitable for preparing subcutaneous implants which allow the active substance to be released over a period of time of at least 6 months. These compositions consist of a polylactlc-glycollc add (PLGA) and a peptide and have the characteristic of distributing peptide particles In the PLGA whose dimensions, under microscopic examination, are extremely heterogeneous, with peptide particles of diameter of between 1 and 60 micrometers dispersed In the polymer matrix. These and other characteristics of the compositions In accordance with the invention and the process for preparing them will be illustrated in greater depth in the following detailed description. Brief description of the drawings Figure 1 represents a microscope test of a cross section of an Implant according to the invention. Figure 2 represents a microscope test of a cross section of an implant acconiing to the prior art Figure 3 represents the cumulative amount of avoreline released from implants of Example 1. Figure 4 represents the cumulative amount of avoreline released from implants of Example 2. Figure 5 represents the plasmatic concentration of LH, FSH and testosterone by clinical experimentation using Implants having an avoreline content of 10 mg. Figure 6 represents the plasmatic concentration of LH, FSH and testosterone by clinical experimentation using implants having an avoreline content of 15 mg. Figure 7 represents tiie plasmatic concentration of avoreline and testosterone by clinical experimentation using implants having an avoreline content of 10 mg. Figure 8 represents the plasmatic concentration of avoreline and testosterone by clinical experimentation using Implants having an avoreline content of 15 mg. Detailed description of the Invention This invention refers to compositions consisting of polylactic-glycolic acid (PLGA) implants. This difficulty cannot be overcome by using the known techniques of mixing by dissolving in a solvent shared by the two compounds or in one solvent for one of the two compounds, nor by means of the techniques for mixing In the melted state. This difficulty has been resolved In this invention by means of wet granulation of the PLGA with the peptide. This operation and the subsequent operations allow the initial heterogeneity of the peptide particles to be retained. The Invention also refers to the process for preparing these compositions and to the aforementioned subcutaneous implants. One such process Is a wet granulation process. This process consists of the following stages: a) the peptide in the form of particles having a diameter of between 1 and 60 micrometers is homogeneously mixed when dry with PLGA in the form of particles whose granulometry is between 10 to 150, preferably 50 and 150, micrometres; b) the mixture obtained from stage a) is granulated using wet granulation by adding a suitable liquid, for example ethanol or water, c) the granulate is then dried until the residual liquid content Is 0.1-3.0%, preferably 0.5-2.0% by weight. This liquid content is fundamental in that it gives the granule sufficient cohesion to prevent the constituents of the mixture from separating during subsequent treatments: d) the mixture obtained from stage c) is extruded. Exposure time in the extruder is from between 1 and 10, preferably between 4 and 6 minutes, with a temperature profile which ranges from 20°C, preferably 30°C. on entering the extruder to no higher than 120'C. preferably 110°C, on leaving the extruder. Under these conditions the PLGA melts forming a continuous matrix which coats the peptide particles while maintaining the heterogeneous nature of these partied dimensions. e) the cylinders produced from extension may be slightly stretched and then cut to obtain dimensions suitable for the subcutaneous implants, namely a diameter of between 1.0 and 1.7, preferably between 1.3 and 1.5 mm, and a length of between 10 and 30, preferably between 16 and 24 mm; f) finally, if needed, the cylinders obtained from stage e) are sterilised. Suitable polylactic-glycolic acid copolymers for use in the invention have molecular The peptide released during in vitro and in vivo trials takes place over a time period of at least 6 months. However the overall time for releasing the peptide can be controlled by varying the diameter and the length of the implant Clinical trials conducted using subcutaneous implants in accordance with this invention in patients with prostate tumours have shown the testosterone suppression within 4 weeks with this effect lasting from approximately 7 months to approximately 12 months. In order to illustrate the invention the following Examples are quoted. Example 1 10 grams of avoreline were mixed thoroughly with 30 grams of polylactic-giycotic acid (PLGA). The avoreline had the following characteristics: • acid-alkalimetric titer: 88.1 % by weight; • pKa: 6.15-9.70-12.02; • granulometric distribution: between 1 and 60 micrometres. The PLGA had the following characteristics: • molecular weight of 116,500 O; • molar ratio between lactic monomer and glycol monomer. 70: 30; • intrinsic viscosity {CHCI3); 0.98 dl/g measured at 25°C, • granulometric distribution: In 90% of cases between 50 and 150 micrometers. The mixture obtained was granulated wet by adding 16 ml of ethanol using a 16mm grid. The granulate obtained was desiccated for 12 hours at a temperature of 25'C in a cunent of dry air. After drying the ethanol content In the granulate was 0.66% by weight. Finally the granulate was extruded using an extruder with a die head of diameter 1.5 mm and length 17.55 mm. The speed of rotation of the screws was 5 rev/minute and the temperature was 30-0 on entering the extruder and 100X on leaving the extruder. The cylinder obtained by the extrusion was slightly stretched and then cut into segments of length 18 mm which were finally radiosteritised. In this way implants The results are shown in Figure 3 in which in the X-axis shows the time expressed in days and the Y-axis shows the cumulative quantity of avoreline released expressed in mg. Example 2 Example 1 was repeated, with the difference that implants were produced with a diameter of 1.5 mm, length 15 mm and avoreline content of 20.9% by weight. Microscopic examination produced similar results to Example 1. The results of the in vitro release test are shown In Figure 4 in which the parameters are the same as those in Figure 3. Example 3 Example 1 was repeated with the difference that PLGA having a molecular weight of 121,900 D was used and implants were prepared having a diameter of 1.5 mm, length 18 mm and avoreline content of 27.9% by weight. Microscopic examination and the release test produced similar results to Example 1. Example 4 9 grams of avoreline were mixed thoroughly with 24g of polylactic-glycolic acid (PLGA). The avoreline had the following characteristics: « acid-alkalimetric titer: 90.1 % by weight; • pKa:e.15 -9.70-12.02: • granulometiic distribution: between 1 and 60 micrometres. The PLGA had the following characteristics: • molecular weight: 121,900 D; • molar ratio between lactic monomer and glycolic monomer 70: 30; • granulometric distribution: in 90% of cases between 50 and 150 micrometres. The mixture obtained was granulated wet by adding 6 ml of water using a 1.6mm grid. The granulate obtained was desiccated for 12 hours at a temperature of 25 °C in a current of dry air. After drying the water content In the granulate was 1.8% by weight. Extrusion and the subsequent operations were conducted as in Example 1. Microscopic examination and the release test prexjuced similar results to Example 1. Clinical experimentation Clinical trials were conducted in 60 patients suffering from prostate tumours, using subcutaneous implants prepared in accordance with this invention. A group of patients was treated with implants having an avoreline content of 10 mg and a second group was treated virith Implants having an avoreline content of 15 mg. The results of the experiments are shown in Figures 5 to 8. The graphs for these Figures can be interpreted as follows: • Graph a) represents the average plasma concentration of the FSH; • Graph b) represents the average plasma concentration of testosterone; • Graph c) represents the average plasma concentration of LH; • Graph d) represents the average plasma concentration of avoreline; • line e) is the line of castration with reference to testosterone. Figure 5 and Figure 7 refer to the use of implants having an avoreline content of 10 mg while Figures 6 and 8 refer to the use of implants having an avoreline content of 15 mg. With reference to Figures 5 and 6, the left ordinate shows the plasma concentration of LH and FSIH expressed in lU/L and the right ordinate shows the plasma concentration of testosterone expressed in nmol/L. With reference to Figures 7 and 8, the left ordinate shows the piasma concentration of avoreline expressed in pg/mL and the right ordinate shows the plasma concentration of testosterone expressed in nmol/L. in alt the Figures, the time from implant Insertion, expressed in weeks, Is shown on the X-axis. As can be seen from these Figures, using the implants in accordance with this invention, testosterone is suppressed within four weeks after the Implant Is inserted with this effect lasting for a period of between approximately seven months and approximately twelve months. The plasma concentrations whirfi can be determined for avoreline were measured for approximately 6 months after Inserting the implant. penetrates and diffuses in the implant and Js distributed between ttie polymer and the peptide forming regions of hydrated peptides. The first stage in releasing the peptide described in the U.S. patent 5.366.734 is a stage of diffusion caused by the polymer swelling. When the polymer swells this allows channels of hydrated peptide to form where the peptide diffuses to the surface. If swelling stops, the peptide is no longer released. The second stage of release is caused by the polymer matrix degrading. During this stage holes and cractcs form in the matrix which allow the release of the hydrated peptides which are still isolated in ttie matrix. The total release time Is limited to the sum of the release times for each stage. However the maximum release time observed is in the order of three months. In the application for intemational patent WO 98/0g613 (Deghenghi) a process for preparing subcutaneous implants capable of releasing bioacUve peptides is descrit>ed. This process consists of the following stages: • milling a copolymer of lactic add and glycolic acid, • wetbng the copolymer with an aqueous slurry of a peptide (In the Examples an aqueous solution of avoraline acetate is used): • mixing this copolymer with the aforementioned sluny so as to obtain a homogeneous mixture; • drying this mixture at a temperature of no higher than 25°C; • extnjding the mixture at 70-1100 in order to obtain small extruded cylinders suitable for use as subcutaneous implants. This process cannot be carried out using industrial methods because it is not possible to sufficiently eliminate water from the mixture. The results declared in WO 98/109613 cannot therefore be reproduced. However the fundamental characteristic of the compositions for subcutaneous implants in the patents referred to above consists of the homogeneous distribution of the peptide in the polymeric substance, resulting from using a solution of at least one of the two components. The implants currently on the marttet have the disadvantage of releasing the and a peptide suitable for the preparation of long-release subcutaneous implants. The implants prepared from compositons in accordance with this invention consist of a PLGA matrix of a high molecular weight incorporating a peptide in the form of particles having extremely heterogeneous dimensions. This structure allows the peptide to be released in three stages, which are, respectively: pure diffusion, diffusion with swelling of the PLGA and release caused by PLGA degradation. This allows the total release time to be significantly increased. When these Implants are introduced into an aqueous environment the water diffuses through the polymer matrix, reaches the peptide particles closest to the surface and then the more intemal zones, resulting in the formation of a porous lattice of the hydrated peptide, through which the phenomenon of peptide release via pure diffusion (first stage) occurs. The implant remains unchanged for approximately 6 weeks and over this period releases approximately 30% of the peptide. The duration of this pure diffusion stage is essentially determined by the degree of heterogeneity of the dimensions of the peptide particles and the speed is essentially determined by the peptide content in the PLGA matrix. As a result of the wide diversity in the dimensions of the peptide granules, a sufficient quantity of peptide remains after the first stage of dissolution to be released over the subsequent stages. In the second stage the peptide is released by diffusion with 3V,-c!lir.g of the polymer, in the third stage, the residual peptide is released when the matrix is destroyed. The succession of the three stages for releasing the peptide without dead time depends on the appropriate choice of constituents in the composition, in particular; • the heterogeneous nature of the dimensions of the peprtide particles determines the first stage of release; • the characteristics of the PLGA (molecular weight and molar ratio) have an influence on the stages of the swelling and matrix degradation. The technical difficulty of this invention lies in retaining the heterogeneous natiJre of the dimensions of the peptide particles throughout the process for preparing the weights ranging from 50.000 to 150,000 and a molar ratio between the lactic acid and the glycolic monomer comprised t>etween 50:50 and 95:5. Preferred potylactic-glycolic acid (PLGA) to be used in the process In accordance with this Invention has a high nominal molecular weight, of between 100,000 and 150,000 D, and a motar ratio between lactic monomer and glycolic monomer of between 70/30 and 75/25. The peptides which can be used In this invention are preferably, but not exclusively, analogues of LHRIH and comprise, for example avoretine: 5-oxo-L-prolyl-L-histidiI-L-tryptophil-L-seryl-L-tyrosH-2-methyl- D-tryptophil-L-leucyl-L-arginyl-N-ethyl-prolylamide; tryptoreline: 5-oxo-L-prolyl-L-histldyl-Utryptophil-L-seryl-L-tyrosil-D-tryptophil-L- leucyl-L-arginyl-L-prolyl-glicinamide: leuproreline: 5-oxo-L-profil-L-histidyl-L-tryptophll-L-seryl-L-tyrosil-D-teucyl-L-leucyl- L-argin^-N-etll-L-prolylamide; gosereline: - 5^)xo-L.prolyl-L-hlstldyl-L-tfyptophll-L-seryl-L-tyrosH-tert-butyl-ID- seryl-L-leucyl-L-arginyl-L-prolyl-NH-NH-CaNHj. The peptide preferably used In this Invention is avorellne. The content of peptide in the composition Is between 20 and 40%, preferably between 20 and 36% by weight. The quantity of liquid added for granulation is between 10 and 60, preferably between 20 and 45 parts by weight In comparison with the mixture. The desiccation involved in stage c) takes place at- a temperaUire of between 20- 50, preferably l>etween 20-30*C in a current of dry air. The transversal section of the cylinders obtained from stage f) reveals under microscope a heterogeneous stmcture containing peptide particles having the same granulometry as the initial peptide immersed In the matrix constituted by the PLGA. The cylinders obtained from stage f) can be successfully used, for subcutaneous implants. Each implant having a diameter of between 1.0 and 1.7, preferably between 1.3 and 1.5 mm. and a length of between 10 and 30, preferably between 15 and 24 mm, has a peptide content of between 5 and 20 mg. for subcutaneous use with diameter of 1.5 mm, length 18 mm and avoreline content of 25.3% by weight were obtained. The transversal section of these implants examined under microscope under x275 enlargment reveals a heterogeneous distribution of the particles of avoreline In the mass of PLGA, as shown in Figure 1. In particular the particles of avoreline retain their initial granulometry of between 1 micrometi^ ad 60 microrrtetre. The same microscopic examination was carried out on an Implant produced using a known technique obtained in accordance with US 5.366.734 which under 1100x enlargement reveats a homogeneous drstribution of the two components as \rFigure 2. Kinetics of in vitro release The implants prepared in accordance with Example 1 were tested in vitro in order to examine the kinetics of releasing avoreline. The test was canried out under the following conditions. Five implants were Introduced into one flask and the 5 ml of phosphate buffer at pH 7.4 were added. The test was conducted at 37°C for a period of 210 days, continuousfy stirring the solution using 100 turns per minute. Each week the buffer solution containing the active constituent released over ttie same period was sampled and analysed, while 5ml of phosphate buffer were added to the flask as above. The content of avoreline in the solutions was determined by means of HPLC under the following conditions: Column; Vydac 218TP 54300A medium, 5 ^m, dimensions 250 x 4.6 mm Mobile phase: 750 ml phosphoric acid 0.1 M were added to 250 ml of acetonitrlle and the pH was con-eded to 2.5 with trietiiylamine and the mixture filtered over an FH type filter (miliipore). Output: 1.5 ml/minute. Temperature: SO'^C Determination: UV at 220 nm Injection: volume 10 nl Analysis time: 15 minutes The implants obtained had an avoreline titer of 27.6% by weight. Microscopic examination and the release test produced similar results to Example 1. Example 5 6 grams of tryptoreline were thoroughly mixed with 14 grams of PLGA. The tryptoreline had a titer of 90.5% by weight and a granulometric distribution of between 1 and 60 micrometres. The PLGA had a molecular weight of 121,900 D, a molar ratio between lactic monomer and glycolic monomer of 70 :30 and a 90% granulometric distribution of between 50 and 150 micrometres. The mixture obtained was granulated wet by adding B ml of ethanol using a 1,6mm grid. The granulate obtained was desiccated for 12 hours at a temperature of 25°C in a current of dry air. After desiccation the ethanol content In the granulate was 1.0% by weight. Extrusion and the subsequent operations were conducted as In Example 1. The implants obtained had an avoreline titer of 24.7% by weight. Microscopic examination and the release test produced similar results to Example 1. 6 grams of gosereline were thoroughly mixed with 14 grams of PLGA. The gosereilne had a titer of 89.5% by weight and a granulometric distribution of between 1 and 60 micrometres. The PLGA had a molecular weight of 121,900 D, a molar ratio between lactic monomer and glycolic monomer of 70 : 30 and a 90% granulometric distribution between 50 and 150 micrometres. The mixture obtained was granulated wet by adding 8 ml of ethanol using a 1.6mm grid. The granulate was desiccated for 12 hours at a temperature of 25 "C in a current of dry air. After desiccation the ethanol content in the granulate was 1.1% by weight. Extrusion and the subsequent operations was carried out as in Example 1. The implants obtained had a gosereline titer of 24.9% by weight. WE CLAIM; 1. Composition suitable for the preparation of subcutaneous implants having an extended release time constituted by polylactic-glycolic acid copolymer (PLGA) and a peptide, characterised in that the peptide dispersed in the PLGA matrix is in the form of particles having heterogeneous dimensions with diameters ranging from 1 to 60 micrometres. 2. The composition as claimed in claim 1, wherein when brought in contact with an aqueous solution of aphysiologic type this peptide is released in three stages, with the first stage of this release involving pure diffusion, the second stage of release involving the PLGA swelling up and'the third stage of release involving PLGA degradation. 3. The composition as claimed in claim 1, wherein the said PLGA has a molecular weight between 50,000 and 150,000 and a molar ratio between lactic monomer and glycolic monomer comprised between 50:50 and 95 -.5. 4. The composition as claimed in claim 3, wherein the said PLGA has a molecular weight of between 100,000 and 150,000 and a molar ratio between lactic monomer and glycolic monomer of between 70/30 and 75/25. 5. The composition as claimed in claim 1, wherein the said peptide is chosen from the group containing avoreline, tryptoreline, leuproreline and gosereline. 6. The composition as claimed in claim 1, wherein the said peptide is avoreline. 7. The composition as claimed in claim 1, wherein the said peptide is tryptoreline. 8. The composition as claimed In claim 1, wherein the said peptide is gosereline. 9. The composition as claimed in claim 1, wherein the peptide content is between 20 and 40%, preferably between 20 and 36% by weight. 10. Process for preparing compositions suitable for preparing subcutaneous implants in accordance with claim 1, characterised in that: a) a peptide in the form of particles having a diameter of between 1 and 60 micrometers is homogeneously mixed when dry with PLGA; b) the mixture obtained from stage a) is granulated by means of wet granulation through adding a liquid; c) the granulate is dried limit the residual liquid content is preferably 0.5 to 2.0% by weight; and d) the mixture obtained from stage c) is extruded and, if needed, cut and sterilised. 11. The process as claimed in claim 10, wherein the exposure time in the extruder of step d) is from 4 to 6 minutes at a temperature which ranges from 30°C on entering the extruder to no higher than 110°C on leaving the extruder. 12. The process as claimed in claim 10, wherein the quantity of peptide used in stage a) is between 20 and 40% and preferably between 20 and 36% by weight in comparison with the mixture constituted by the peptide and PLGA. 13. The process as claimed in claim 10, wherein when this granulation liquid is ethanol or water the quantity of liquid added is between 10 and 60, preferably between 20 and 45 parts for 100 parts of mixture by weight. 14. The process as claimed in claim 10, wherein the cylinders obtained by extrusion from stage d) have a diameter of between 1.0 and 1.7, preferably 1.3 and 1.5 mm, and a length of between 10 and 30, preferably 15 and 24 mm. 15. Subcutaneous implants obtained from the composition as claimed in claim 1. 16. Subcutaneous implants prepared using the process as claimed in claims 10 to 14. 17. Subcutaneous implants as claimed in claims 15 and 16 having a diameter of between 1.3 and 1.5 mm, length of between 15 and 24 mm and peptide content of between 5 and 20 mg. 18. Subcutaneous implants as claimed in claim 17, wherein the said peptide is chosen from the group containing avoreline; tryptoreline, leuproreline and gosereline.

Full Text

The present invention refers to compositions comprising a peptide and polylacllc-glycollc acid suitable for the preparation of subcutaneous implants. Prior art
Compositions made up of mixtures of a drug with a polymer of lactic acid or a
polymer of glycolic acid or with a copolymer of lactic acid and glycolic acid, as
described in the U.S. patent 3.773.919 (Du Pont) are well known .
These compositions are indicated for potential administration and have the
characteristics of releasing effective quantities of the drug over a set period of
time.
The drug and the polymeric substance can be combined in accordance with any of
the known techniques or the particles of the drug can be coated in the polymer
operating In accordance with known techniques.
The U.S. patent 4.767.628 (ICI) describes compositions containing a peptide and
a polymer of lactic acid or a copolymer of lactic acid and giycolic ackl.
When preparing the compositions, the pestle and the (oo)polymer are dissolved
in a solvent which can be the same or different for the two substances, for
Example dioxane or water, and then the two solutions are mixed.
The subsequent operations consist of removing the solvent at low temperature
and in extruding the powder obtained in this way.
In this way a composition in the form of cylinders is obtained in which the peptide
is distributed homogeneously throughout the polymer.
It is already known from the U.S. patent 5.366.734 (Zeneca) that the compositions
covered by the U.S. patent 4.767.628 referred to above can be used In preparing
subcutaneous implants.
The polymer of lactic acid and the copolymer of lactic acid and giycolic acid are
incompatible with the peptide therefore diffusion of the peptide through the
polymer is impossible.
When these implants are introduced into a buffer solution at 37 °C, the water

peptides over a limited period of time, generally of around 3 months.
Summary of the Invention
The applicant has now found compositions suitable for preparing subcutaneous
implants which allow the active substance to be released over a period of time of
at least 6 months.
These compositions consist of a polylactlc-glycollc add (PLGA) and a peptide and
have the characteristic of distributing peptide particles In the PLGA whose
dimensions, under microscopic examination, are extremely heterogeneous, with
peptide particles of diameter of between 1 and 60 micrometers dispersed In the
polymer matrix.
These and other characteristics of the compositions In accordance with the
invention and the process for preparing them will be illustrated in greater depth in
the following detailed description.
Brief description of the drawings
Figure 1 represents a microscope test of a cross section of an Implant according to
the invention.
Figure 2 represents a microscope test of a cross section of an implant acconiing to
the prior art
Figure 3 represents the cumulative amount of avoreline released from implants of
Example 1.
Figure 4 represents the cumulative amount of avoreline released from implants of
Example 2.
Figure 5 represents the plasmatic concentration of LH, FSH and testosterone by
clinical experimentation using Implants having an avoreline content of 10 mg.
Figure 6 represents the plasmatic concentration of LH, FSH and testosterone by
clinical experimentation using implants having an avoreline content of 15 mg.
Figure 7 represents tiie plasmatic concentration of avoreline and testosterone by
clinical experimentation using implants having an avoreline content of 10 mg.
Figure 8 represents the plasmatic concentration of avoreline and testosterone by
clinical experimentation using Implants having an avoreline content of 15 mg.
Detailed description of the Invention
This invention refers to compositions consisting of polylactic-glycolic acid (PLGA)

implants.
This difficulty cannot be overcome by using the known techniques of mixing by
dissolving in a solvent shared by the two compounds or in one solvent for one of
the two compounds, nor by means of the techniques for mixing In the melted state.
This difficulty has been resolved In this invention by means of wet granulation of
the PLGA with the peptide. This operation and the subsequent operations allow
the initial heterogeneity of the peptide particles to be retained.
The Invention also refers to the process for preparing these compositions and to
the aforementioned subcutaneous implants.
One such process Is a wet granulation process.
This process consists of the following stages:
a) the peptide in the form of particles having a diameter of between 1 and 60 micrometers is homogeneously mixed when dry with PLGA in the form of particles whose granulometry is between 10 to 150, preferably 50 and 150, micrometres;
b) the mixture obtained from stage a) is granulated using wet granulation by adding a suitable liquid, for example ethanol or water,
c) the granulate is then dried until the residual liquid content Is 0.1-3.0%, preferably 0.5-2.0% by weight. This liquid content is fundamental in that it gives the granule sufficient cohesion to prevent the constituents of the mixture from separating during subsequent treatments:
d) the mixture obtained from stage c) is extruded. Exposure time in the extruder is from between 1 and 10, preferably between 4 and 6 minutes, with a temperature profile which ranges from 20°C, preferably 30°C. on entering the extruder to no higher than 120'C. preferably 110°C, on leaving the extruder. Under these conditions the PLGA melts forming a continuous matrix which coats the peptide particles while maintaining the heterogeneous nature of these partied dimensions.
e) the cylinders produced from extension may be slightly stretched and then cut to obtain dimensions suitable for the subcutaneous implants, namely a diameter of between 1.0 and 1.7, preferably between 1.3 and 1.5 mm, and a length of between 10 and 30, preferably between 16 and 24 mm;
f) finally, if needed, the cylinders obtained from stage e) are sterilised.
Suitable polylactic-glycolic acid copolymers for use in the invention have molecular

The peptide released during in vitro and in vivo trials takes place over a time
period of at least 6 months.
However the overall time for releasing the peptide can be controlled by varying the
diameter and the length of the implant
Clinical trials conducted using subcutaneous implants in accordance with this
invention in patients with prostate tumours have shown the testosterone
suppression within 4 weeks with this effect lasting from approximately 7 months to
approximately 12 months.
In order to illustrate the invention the following Examples are quoted.
Example 1
10 grams of avoreline were mixed thoroughly with 30 grams of polylactic-giycotic
acid (PLGA).
The avoreline had the following characteristics:
• acid-alkalimetric titer: 88.1 % by weight;
• pKa: 6.15-9.70-12.02;
• granulometric distribution: between 1 and 60 micrometres. The PLGA had the following characteristics:
• molecular weight of 116,500 O;
• molar ratio between lactic monomer and glycol monomer. 70: 30;
• intrinsic viscosity {CHCI3); 0.98 dl/g measured at 25°C,
• granulometric distribution: In 90% of cases between 50 and 150 micrometers. The mixture obtained was granulated wet by adding 16 ml of ethanol using a 16mm grid.
The granulate obtained was desiccated for 12 hours at a temperature of 25'C in a
cunent of dry air.
After drying the ethanol content In the granulate was 0.66% by weight.
Finally the granulate was extruded using an extruder with a die head of diameter
1.5 mm and length 17.55 mm.
The speed of rotation of the screws was 5 rev/minute and the temperature was
30-0 on entering the extruder and 100X on leaving the extruder.
The cylinder obtained by the extrusion was slightly stretched and then cut into
segments of length 18 mm which were finally radiosteritised. In this way implants

The results are shown in Figure 3 in which in the X-axis shows the time expressed
in days and the Y-axis shows the cumulative quantity of avoreline released
expressed in mg.
Example 2
Example 1 was repeated, with the difference that implants were produced with a
diameter of 1.5 mm, length 15 mm and avoreline content of 20.9% by weight.
Microscopic examination produced similar results to Example 1. The results of the
in vitro release test are shown In Figure 4 in which the parameters are the same
as those in Figure 3.
Example 3
Example 1 was repeated with the difference that PLGA having a molecular weight
of 121,900 D was used and implants were prepared having a diameter of 1.5 mm,
length 18 mm and avoreline content of 27.9% by weight.
Microscopic examination and the release test produced similar results to Example
1.
Example 4
9 grams of avoreline were mixed thoroughly with 24g of polylactic-glycolic acid
(PLGA).
The avoreline had the following characteristics:
« acid-alkalimetric titer: 90.1 % by weight;
• pKa:e.15 -9.70-12.02:
• granulometiic distribution: between 1 and 60 micrometres. The PLGA had the following characteristics:
• molecular weight: 121,900 D;
• molar ratio between lactic monomer and glycolic monomer 70: 30;
• granulometric distribution: in 90% of cases between 50 and 150 micrometres. The mixture obtained was granulated wet by adding 6 ml of water using a 1.6mm grid.
The granulate obtained was desiccated for 12 hours at a temperature of 25 °C in a
current of dry air.
After drying the water content In the granulate was 1.8% by weight.
Extrusion and the subsequent operations were conducted as in Example 1.

Microscopic examination and the release test prexjuced similar results to Example
1.
Clinical experimentation
Clinical trials were conducted in 60 patients suffering from prostate tumours, using
subcutaneous implants prepared in accordance with this invention.
A group of patients was treated with implants having an avoreline content of 10 mg
and a second group was treated virith Implants having an avoreline content of 15
mg.
The results of the experiments are shown in Figures 5 to 8.
The graphs for these Figures can be interpreted as follows:
• Graph a) represents the average plasma concentration of the FSH;
• Graph b) represents the average plasma concentration of testosterone;
• Graph c) represents the average plasma concentration of LH;
• Graph d) represents the average plasma concentration of avoreline;
• line e) is the line of castration with reference to testosterone.
Figure 5 and Figure 7 refer to the use of implants having an avoreline content of
10 mg while Figures 6 and 8 refer to the use of implants having an avoreline
content of 15 mg.
With reference to Figures 5 and 6, the left ordinate shows the plasma
concentration of LH and FSIH expressed in lU/L and the right ordinate shows the
plasma concentration of testosterone expressed in nmol/L.
With reference to Figures 7 and 8, the left ordinate shows the piasma
concentration of avoreline expressed in pg/mL and the right ordinate shows the
plasma concentration of testosterone expressed in nmol/L.
in alt the Figures, the time from implant Insertion, expressed in weeks, Is shown on
the X-axis.
As can be seen from these Figures, using the implants in accordance with this
invention, testosterone is suppressed within four weeks after the Implant Is
inserted with this effect lasting for a period of between approximately seven
months and approximately twelve months.
The plasma concentrations whirfi can be determined for avoreline were measured
for approximately 6 months after Inserting the implant.

penetrates and diffuses in the implant and Js distributed between ttie polymer and
the peptide forming regions of hydrated peptides.
The first stage in releasing the peptide described in the U.S. patent 5.366.734 is a
stage of diffusion caused by the polymer swelling.
When the polymer swells this allows channels of hydrated peptide to form where
the peptide diffuses to the surface.
If swelling stops, the peptide is no longer released.
The second stage of release is caused by the polymer matrix degrading.
During this stage holes and cractcs form in the matrix which allow the release of
the hydrated peptides which are still isolated in ttie matrix.
The total release time Is limited to the sum of the release times for each stage.
However the maximum release time observed is in the order of three months.
In the application for intemational patent WO 98/0g613 (Deghenghi) a process for
preparing subcutaneous implants capable of releasing bioacUve peptides is
descrit>ed.
This process consists of the following stages:
• milling a copolymer of lactic add and glycolic acid,
• wetbng the copolymer with an aqueous slurry of a peptide (In the Examples an aqueous solution of avoraline acetate is used):
• mixing this copolymer with the aforementioned sluny so as to obtain a homogeneous mixture;
• drying this mixture at a temperature of no higher than 25°C;
• extnjding the mixture at 70-110*0 in order to obtain small extruded cylinders suitable for use as subcutaneous implants.
This process cannot be carried out using industrial methods because it is not
possible to sufficiently eliminate water from the mixture. The results declared in
WO 98/109613 cannot therefore be reproduced.
However the fundamental characteristic of the compositions for subcutaneous
implants in the patents referred to above consists of the homogeneous distribution
of the peptide in the polymeric substance, resulting from using a solution of at
least one of the two components.
The implants currently on the marttet have the disadvantage of releasing the

and a peptide suitable for the preparation of long-release subcutaneous implants.
The implants prepared from compositons in accordance with this invention consist
of a PLGA matrix of a high molecular weight incorporating a peptide in the form of
particles having extremely heterogeneous dimensions.
This structure allows the peptide to be released in three stages, which are,
respectively: pure diffusion, diffusion with swelling of the PLGA and release
caused by PLGA degradation.
This allows the total release time to be significantly increased.
When these Implants are introduced into an aqueous environment the water
diffuses through the polymer matrix, reaches the peptide particles closest to the
surface and then the more intemal zones, resulting in the formation of a porous
lattice of the hydrated peptide, through which the phenomenon of peptide release via pure diffusion (first stage) occurs.
The implant remains unchanged for approximately 6 weeks and over this period
releases approximately 30% of the peptide.
The duration of this pure diffusion stage is essentially determined by the degree of
heterogeneity of the dimensions of the peptide particles and the speed is
essentially determined by the peptide content in the PLGA matrix.
As a result of the wide diversity in the dimensions of the peptide granules, a
sufficient quantity of peptide remains after the first stage of dissolution to be
released over the subsequent stages.
In the second stage the peptide is released by diffusion with 3V,-c!lir.g of the
polymer,
in the third stage, the residual peptide is released when the matrix is destroyed.
The succession of the three stages for releasing the peptide without dead time
depends on the appropriate choice of constituents in the composition, in particular;
• the heterogeneous nature of the dimensions of the peprtide particles determines the first stage of release;
• the characteristics of the PLGA (molecular weight and molar ratio) have an influence on the stages of the swelling and matrix degradation.
The technical difficulty of this invention lies in retaining the heterogeneous natiJre of the dimensions of the peptide particles throughout the process for preparing the

weights ranging from 50.000 to 150,000 and a molar ratio between the lactic acid
and the glycolic monomer comprised t>etween 50:50 and 95:5.
Preferred potylactic-glycolic acid (PLGA) to be used in the process In accordance
with this Invention has a high nominal molecular weight, of between 100,000 and
150,000 D, and a motar ratio between lactic monomer and glycolic monomer of
between 70/30 and 75/25.
The peptides which can be used In this invention are preferably, but not
exclusively, analogues of LHRIH and comprise, for example
avoretine: 5-oxo-L-prolyl-L-histidiI-L-tryptophil-L-seryl-L-tyrosH-2-methyl-
D-tryptophil-L-leucyl-L-arginyl-N-ethyl-prolylamide;
tryptoreline: 5-oxo-L-prolyl-L-histldyl-Utryptophil-L-seryl-L-tyrosil-D-tryptophil-L-
leucyl-L-arginyl-L-prolyl-glicinamide:
leuproreline: 5-oxo-L-profil-L-histidyl-L-tryptophll-L-seryl-L-tyrosil-D-teucyl-L-leucyl-
L-argin^-N-etll-L-prolylamide;
gosereline: - 5^)xo-L.prolyl-L-hlstldyl-L-tfyptophll-L-seryl-L-tyrosH-tert-butyl-ID-
seryl-L-leucyl-L-arginyl-L-prolyl-NH-NH-CaNHj.
The peptide preferably used In this Invention is avorellne.
The content of peptide in the composition Is between 20 and 40%, preferably
between 20 and 36% by weight.
The quantity of liquid added for granulation is between 10 and 60, preferably
between 20 and 45 parts by weight In comparison with the mixture.
The desiccation involved in stage c) takes place at- a temperaUire of between 20-
50, preferably l>etween 20-30**C in a current of dry air.
The transversal section of the cylinders obtained from stage f) reveals under
microscope a heterogeneous stmcture containing peptide particles having the
same granulometry as the initial peptide immersed In the matrix constituted by the
PLGA.
The cylinders obtained from stage f) can be successfully used, for subcutaneous
implants.
Each implant having a diameter of between 1.0 and 1.7, preferably between 1.3
and 1.5 mm. and a length of between 10 and 30, preferably between 15 and 24
mm, has a peptide content of between 5 and 20 mg.

for subcutaneous use with diameter of 1.5 mm, length 18 mm and avoreline
content of 25.3% by weight were obtained.
The transversal section of these implants examined under microscope under x275
enlargment reveals a heterogeneous distribution of the particles of avoreline In the
mass of PLGA, as shown in Figure 1. In particular the particles of avoreline retain
their initial granulometry of between 1 micrometi^ ad 60 microrrtetre.
The same microscopic examination was carried out on an Implant produced using
a known technique obtained in accordance with US 5.366.734 which under 1100x
enlargement reveats a homogeneous drstribution of the two components as \rFigure 2.
Kinetics of in vitro release
The implants prepared in accordance with Example 1 were tested in vitro in order
to examine the kinetics of releasing avoreline.
The test was canried out under the following conditions.
Five implants were Introduced into one flask and the 5 ml of phosphate buffer at
pH 7.4 were added. The test was conducted at 37°C for a period of 210 days,
continuousfy stirring the solution using 100 turns per minute.
Each week the buffer solution containing the active constituent released over ttie
same period was sampled and analysed, while 5ml of phosphate buffer were
added to the flask as above.
The content of avoreline in the solutions was determined by means of HPLC under
the following conditions:
Column; Vydac 218TP 54300A medium, 5 ^m,
dimensions 250 x 4.6 mm
Mobile phase: 750 ml phosphoric acid 0.1 M were added to 250 ml of acetonitrlle and the pH was con-eded to 2.5 with trietiiylamine and the mixture filtered over an FH type filter (miliipore).
Output: 1.5 ml/minute.
Temperature: SO'^C
Determination: UV at 220 nm
Injection: volume 10 nl
Analysis time: 15 minutes

The implants obtained had an avoreline titer of 27.6% by weight.
Microscopic examination and the release test produced similar results to Example
1.
Example 5
6 grams of tryptoreline were thoroughly mixed with 14 grams of PLGA.
The tryptoreline had a titer of 90.5% by weight and a granulometric distribution of
between 1 and 60 micrometres.
The PLGA had a molecular weight of 121,900 D, a molar ratio between lactic
monomer and glycolic monomer of 70 :30 and a 90% granulometric distribution of
between 50 and 150 micrometres.
The mixture obtained was granulated wet by adding B ml of ethanol using a 1,6mm
grid.
The granulate obtained was desiccated for 12 hours at a temperature of 25°C in a
current of dry air.
After desiccation the ethanol content In the granulate was 1.0% by weight.
Extrusion and the subsequent operations were conducted as In Example 1.
The implants obtained had an avoreline titer of 24.7% by weight. Microscopic
examination and the release test produced similar results to Example 1.
6 grams of gosereline were thoroughly mixed with 14 grams of PLGA.
The gosereilne had a titer of 89.5% by weight and a granulometric distribution of
between 1 and 60 micrometres.
The PLGA had a molecular weight of 121,900 D, a molar ratio between lactic
monomer and glycolic monomer of 70 : 30 and a 90% granulometric distribution
between 50 and 150 micrometres.
The mixture obtained was granulated wet by adding 8 ml of ethanol using a 1.6mm
grid.
The granulate was desiccated for 12 hours at a temperature of 25 "C in a current
of dry air.
After desiccation the ethanol content in the granulate was 1.1% by weight.
Extrusion and the subsequent operations was carried out as in Example 1.
The implants obtained had a gosereline titer of 24.9% by weight.

WE CLAIM;
1. Composition suitable for the preparation of subcutaneous implants
having an extended release time constituted by polylactic-glycolic acid copolymer
(PLGA) and a peptide, characterised in that the peptide dispersed in the PLGA
matrix is in the form of particles having heterogeneous dimensions with diameters
ranging from 1 to 60 micrometres.
2. The composition as claimed in claim 1, wherein when brought in contact with an aqueous solution of aphysiologic type this peptide is released in three stages, with the first stage of this release involving pure diffusion, the second stage of release involving the PLGA swelling up and'the third stage of release involving PLGA degradation.
3. The composition as claimed in claim 1, wherein the said PLGA has a molecular weight between 50,000 and 150,000 and a molar ratio between lactic monomer and glycolic monomer comprised between 50:50 and 95 -.5.
4. The composition as claimed in claim 3, wherein the said PLGA has a molecular weight of between 100,000 and 150,000 and a molar ratio between lactic monomer and glycolic monomer of between 70/30 and 75/25.
5. The composition as claimed in claim 1, wherein the said peptide is
chosen from the group containing avoreline, tryptoreline, leuproreline and
gosereline.

6. The composition as claimed in claim 1, wherein the said peptide is avoreline.
7. The composition as claimed in claim 1, wherein the said peptide is tryptoreline.
8. The composition as claimed In claim 1, wherein the said peptide is gosereline.
9. The composition as claimed in claim 1, wherein the peptide content is between 20 and 40%, preferably between 20 and 36% by weight.
10. Process for preparing compositions suitable for preparing subcutaneous
implants in accordance with claim 1, characterised in that:
a) a peptide in the form of particles having a diameter of between 1 and 60
micrometers is homogeneously mixed when dry with PLGA;
b) the mixture obtained from stage a) is granulated by means of wet granulation
through adding a liquid;
c) the granulate is dried limit the residual liquid content is preferably 0.5 to 2.0%
by weight; and
d) the mixture obtained from stage c) is extruded and, if needed, cut and sterilised.

11. The process as claimed in claim 10, wherein the exposure time in the extruder of step d) is from 4 to 6 minutes at a temperature which ranges from 30°C on entering the extruder to no higher than 110°C on leaving the extruder.
12. The process as claimed in claim 10, wherein the quantity of peptide used in stage a) is between 20 and 40% and preferably between 20 and 36% by weight in comparison with the mixture constituted by the peptide and PLGA.
13. The process as claimed in claim 10, wherein when this granulation liquid is ethanol or water the quantity of liquid added is between 10 and 60, preferably between 20 and 45 parts for 100 parts of mixture by weight.
14. The process as claimed in claim 10, wherein the cylinders obtained by extrusion from stage d) have a diameter of between 1.0 and 1.7, preferably 1.3 and 1.5 mm, and a length of between 10 and 30, preferably 15 and 24 mm.
15. Subcutaneous implants obtained from the composition as claimed in claim 1.
16. Subcutaneous implants prepared using the process as claimed in claims 10 to 14.
17. Subcutaneous implants as claimed in claims 15 and 16 having a diameter of between 1.3 and 1.5 mm, length of between 15 and 24 mm and peptide content of between 5 and 20 mg.

18. Subcutaneous implants as claimed in claim 17, wherein the said peptide is chosen from the group containing avoreline; tryptoreline, leuproreline and gosereline.

Documents:

in-pct-2001-0936-che abstract.pdf

in-pct-2001-0936-che claims-duplicate.pdf

in-pct-2001-0936-che claims.pdf

in-pct-2001-0936-che correspondence-others.pdf

in-pct-2001-0936-che correspondence-po.pdf

in-pct-2001-0936-che description (complete)-duplicate.pdf

in-pct-2001-0936-che description (complete).pdf

in-pct-2001-0936-che drawings-duplicate.pdf

in-pct-2001-0936-che drawings.pdf

in-pct-2001-0936-che form-1.pdf

in-pct-2001-0936-che form-19.pdf

in-pct-2001-0936-che form-26.pdf

in-pct-2001-0936-che form-3.pdf

in-pct-2001-0936-che form-5.pdf

in-pct-2001-0936-che form-6.pdf

in-pct-2001-0936-che others.pdf

in-pct-2001-0936-che pct.pdf

in-pct-2001-0936-che petition.pdf

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Patent Number

226959

Indian Patent Application Number

IN/PCT/2001/936/CHE

PG Journal Number

07/2009

Publication Date

13-Feb-2009

Grant Date

31-Dec-2008

Date of Filing

05-Jul-2001

Name of Patentee

MEDIOLANUM PHARMACEUTICALS LIMITED

Applicant Address

7TH FLOOR, HUME HOUSE BALLS BRIDGE, DUBLIN 4,

Inventors:

#	Inventor's Name	Inventor's Address
1	ALAIN MAQUIN	29 ALLEE DU MONTCHAILLOU, POMPONNE, F-77400 LAGNY SUR MARNE,
2	MAURIAC PATRICE	54, RUE DE PICPUS, F-75012 PARIS,
3	PIERRE MARION	26, AVENUE DU CENTRE, PROLONGEE, F-93360 NEUILLY PLAISANCE,

PCT International Classification Number

A61K9/00

PCT International Application Number

PCT/EP99/09536

PCT International Filing date

1999-12-06

PCT Conventions:

#	PCT Application Number	Date of Convention	Priority Country
1	M198A002655	1998-12-10	Italy