Title of Invention | LOW MOLECULAR WEIGHT PEPTIDE DERIVATIVES AS INHIBITORS OF THE LAMININ/NIDOGEN INTERACTION AND A PHARMACEUTICAL COMPOSITION COMPRISING THE SAME |
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Abstract | ABSTRACT IN/PCT/2001/01142/CHE "Low molecular weight peptide derivatives as inhibitors of the laminin/nidogen interaction and a pharmaceutical composition comprising the same" Object of the present invention are low molecular weight peptide derivatives which are able to act as inhibitors of the interaction between laminin and nidogen (laminin/nidogen interaction), a process for their preparation, pharmaceutical compositions prepared therefrom and their use for preparing pharmaceuticals and for identifying inhibitors of the laminin/nidogen interaction. |
Full Text | Low molecular weight peptide derivatives as inhibitors of the laminin/nldogen Interaction Object of the present invention are low nnolecular weight peptide derivatives which are able to act as inhibitors of the interaction between laminin and nidogen (laminin/nldogen Interaction), a process for their preparation, pharmaceutical compositions- prepared therefrom and their use for preparing pharmaceuticals and for identifying inhibitors of the laminin/nldogen interaction. The association of laminin (an 800 kDa glycoprotein) and nidogen (a 160 kDa glycoprotein) is regarded as a crucial biomolecular mechanism in the synthesis and stabilization of basement membranes (Mayer, U. and TimpI, R. (1994) in: Extracellular Matrix Assembly and Structure (P.D. Yurchenco, D. Birk and R.P. Mecham, Ed.) S. 389 - 416, Academic Press, Orlando, FL). The ability of nidogen to form ternary complexes with all main constituents of the basement membrane such as, for example, y1-containing laminin isoforms (for nomenclature see: Burgeson, R.E.; Chiquet, M.; Deutzmann, R.; Ekblom, P.; Engel, J.; Kleinmann, H.; Martin, G. R.; Meneguzzi, G.; Paulsson M.; Sanes, J.; TimpI, R.; Tryggvasson, K.; Yamada, Y.; Yurchenco, P.D. (1994) Matrix Biology 14; 209 - 211), collagen IV, perlecan and fibulin, and the association structures of each of them, means that it assumes the function of a linker which connects together, spatially organizes and stabilizes the independent macrostructures (Fox, J.W.; Mayer, U.; Nischt, R.; Aumailley, M.; Reinhardt, D.; Wiedemann, H.; Mann, K.; TimpI, R.; Krieg, T.; Engel, J.; and Chu, M.-L (1991) EMBO J. 10, 3137 - 3146). Basement membranes are highly specialized extracellular structures which are attributed with important functions in the control of cell and tissue functions, tissue architecture, tissue interactions, cell growth, cell transformation, cell migration and in tissue-specific gene expression (Adams, J.C. and Watt, F.M. (1993) Development 117, 1183 -1198).Experiments with polyclonal antilaminin antibodies have provided clear evidence of the central function of the laminin/nldogen interaction in the synthesis of a functional basement membrane. The described antibodies were obtained by immunizing rabbits with laminin PI or with the recombinantly produced nidogen-binding domain of laminin (y1 III 3-5). The antibodies concentrated by affinity chromatography on laminin P1 or laminin y1 III 3-5 matrices showed complete inhibition of the laminin/nidogen association in inhibition assays. However, this is based on steric blockade of the access of nidogen to laminin by the antibodies, whose binding regions are located in the vicinity of the nidogen-binding sequences of laminin (Mayer, U.; Nischt, R.; PbschI, E.; Mann, K.; Fukuda, K.; Gerl, M.; Yamada, Y.; TimpI, R. (1993) EMBO J. 12; 1879 - 1885). In embryonic organ cultures, the described antibodies inhibited both the development of renal tubules, the formation of pulmonary alveoli and the morphogenesis of the embryonic salivary gland. These three models are representative of ontogenesis programs which depend on unimpeded synthesis of new basement membrane (Ekblom, P.; Ekblom, M.; Fecker, L.; Klein, G.; Zhang, H.-Y.; Kadoya, Y.; Chu, M.-L.; Mayer, U.; TimpI, R. (1994) Development 120; 2003 -2014). Antibodies directed against the laminin y chain sequence region which is essential for nidogen binding are likewise able to inhibit the laminin/nidogen association. The inhibition is, however, competitive, in contrast to the antilaminin antibodies described above, because they compete directly with the nidogen for the binding site on laminin (WO 98/31709). A monoclonal antibody of the IgM subclass (antilaminin PI A6/2/4 - DSM ACC2327; see WO 98/31709) inhibits the laminin/nidogen interaction in vitro with an IC50 of 30 nM. Like the polyclonal antilaminin antibody preparation described above, it prevents the morphogenesis of the embryonic salivary gland in organ culture. This underlines the specificity of the laminin/nidogen interaction, and the importance of the LE-4 module and of the identified sequence region in the laminin y1 111 4 domain in this interaction. The nidogen binding domain of laminin has been unambiguously identified and characterized in terms of its location, sequence and its spatial structure (X-ray crystal structure and NMR structure) (Gerl, M.; Mann, K.; Aumailley, M.; TimpI, R. (1991) Eur. J. Biochem. 202; 167 -174. Mayer, U.; Nischt, R.; POschl, E.; Mann, K.; Fukuda, K.; Gerl, M.; Yamada, Y.; TimpI, R. (1993) EMBO J. 12; 1879 -1885. Baumgartner, R.; Czisch, M.; Mayer, U.; PoschI, E.; Huber, P.; TimpI, R.; Holak, T.A. (1996) J. Mol. Biol. 257; 658 - 668. Stetefeld, J.; Mayer. U.; TimpI, R.; Huber, R. (1996) J. Mol. Biol. 257; 644 - 657). It is located in an "LE module" (laminin type epidermal growth factor-like) of the short arm of the y1 chain of laminin, in the domain y1 III 4. "LE modules" are structural motifs of 50-60 amino acids which have a complex folding pattern, analogous to EOF, with 4 disulfide bridges (Bairoch, A.; (1995) Nomenclature of extracellular domains. The SWISS-PROT Protein sequence data bank, release 310. Engel, J. (1989) FEES Letters 251; 1 - 7). High-affinity binding of nidogen to the complementary laminin domain has been detected for laminin PI from the EHS tumor of mice, laminin 2 and laminin 4 from human placenta and laminin from drosophila. The cause of this species-overlapping binding specificity is the extremely large identity of sequences present in the yl 1114 domain for the species investigated. It is 97% between human and mouse, 61% between mouse and drosophila and, astonishingly, 51% between mouse and Caenorhabditis elegans when the whole domain is taken into account (Pikkarinen, T.; Kallunki, T.; Tryggvasson, K. (1987) J. Biol. Chem. 263; 6751 - 6758. Chi, H.-C; Hui, C.-F. (1989) J. Biol. Chem. 264; 1543 - 1550. Wilson, R. et al.(1994) Nature 368: 32-38. POschl, E.; Mayer, U.; Stetefeld, J.; Baumgartner, R.; Holak, T.A.; Huber, R.; TimpI, R. (1996) EMBO J. 15: 5154-5159). Besides the dependency of nidogen binding on an intact three-dimensional structure, unambiguous sequence regions located in the S-S stabilized loops a and c of the domain y1 III 4 have been identified. Five essential amino acids have been identified, four located inside a section of 7 amino acids in loop a, and a tyrosine side-chain in loop c (Mann, K.; Deutzmann, R.; TimpI, R. (1988) Eur. J. Biochem. 178; 71 - 80). Synthetic peptides which can be derived from the appropriate regions of the yl 1114 domain and are able to inhibit completely the laminin/nidogen binding in specific binding assays have been disclosed by J.W. Fox and R. TimpI (US 5,493,008). The high-affinity binding to the laminin binding site of nidogen is thought to require an interaction with a tyrosine or histidine from a loop (loop c) adjacent to the actual binding sequence. This aromatic interaction was postulated as a precondition for inhibition in the IC50 range The laminin/nidogen interaction is influenced by a strong conformational component (Mayer, U.; Nischt, R.; PoschI, E.; Mann, K.; Fukuda, K.; Gerl, M.; Yamada, Y.; TimpI, R. (1993) EMBO J. 12; 1879 -1885. Mann, K.; Deutzmann, R.; TimpI, R. (1988) Eur. J. Biochem. 178; 71 - 80). The synthetic peptides which can be derived from the nidogen binding site of laminin are not able to form a disulfide linkage pattern as is present in LE modules, but they show an activity in inhibition assays which is about 400 - 10,000-fold weaker than that of intact laminin PI or laminin y1 III 3-5 (PoschI, E.; Fox, J.W.; Block, D.; Mayer, U.; TimpI, R, (1994) EMBO J. 13; 3741 - 3747. J.W. Fox and R. TimpI; US 5,493,008). This decline in activity is not unusual, since it is known that peptides may assume a myriad of different conformations in aqueous solution and that only a certain percentage of peptides is to be found in the biologically active conformation. The most active peptide described to date (1050 of 22 nM) has a molecular weight of about 2700 Da (= about 50% of an LE module). It comprises an intact S-S loop which presumably stabilizes the structure of the essential NIDPNAV sequence region (PoschI, E.; Fox, J.W.; Block, D.; Mayer, U.; TimpI, R, (1994) EMBO J. 13; 3741 - 3747. J.W. Fox and R. TimpI; US 5,493,008). The chemical formula of the sequence NIDPNAV (Asn-lle-Asp-Pro-Asn-Ala-Val) is as follows: Inhibitors of the laminin/nidogen interaction should be suitable for preparing pharmaceuticals for diseases which are related to an increased or unwanted synthesis of basement membranes. Such diseases are e.g. all types of late complications of diabetes which are accompanied by thickening of basement membranes (especially in the kidney, eye, vascular system), hepatic fibrosis, especially alcoholic hepatic fibrosis, characterized by synthesis of a continuous basement membrane in the sinusoids and a capillarization caused thereby, all fibroses (chronic or iatrogenic) in which an increased synthesis of basement membrane or components of the basement membrane can be observed (kidney, lung, skin), atherosclerosis characterized by a limitation of the regulation of lipid metabolism, which may be caused inter alia by impaired filtration of lipoproteins through the partly capillarized liver sinusoids (the pathological changes in the vascular system which can be observed with atherosclerosis may also in part be attributed to modifications of the composition and structure of the basement membranes in the vessels), diseases in which angiogenesis contributes to a deterioration in the clinical picture, for example cancers in which neovascularization is required for tumor growth, diabetic retinopathy, retrolental fibroplasia, disorders with a strong inflammatory component (for example rheumatoid arthritis, osteoarthritis, vasculitis), hemangiomas, psoriasis, and many others. The use of peptides like those described in US patent number US 5,493,008 as medicine is however limited to a considerable extent because of their conformational flexibility, their instability to proteases and their poor bioavailability and pharmacodynamics (Milner-White, E.J. (1989) Trends Pharmacol. Sci. 10; 70 - 74. Verber, D.F.; Freidinger, R.M.; (1985) Trends Neurosci. 8; 392 - 396. Hruby, V.J. (1994) in: Peptides, Proc. Thirteenth American Peptide Symposium; (Hodges, R.S.; Smith, J.A.; Ed.) S. 3 -17; ESCOM: Leiden, Netherlands). The object of this application was thus to find low molecular weight peptide derivatives which are able to interact specifically with the laminin binding site of nidogen and to inhibit competitively the association between laminin and nidogen at low concentration. R2 means -A, -E-OH, -E-COOH or -E-CONH2, wherein E means a linear or branched C1-C10-allcyl chain, which is unsubstituted or substituted by -A, -(CH2)m-OH, -(CH2)m-C00H, -(CH2)m-C(0)NA2 or by a C5-C10-cycloalkyI group, or E means C5-C10-cycloalkyl, which is unsubstituted or substituted by -A, -(CH2)rr,-0H, -(CH2)m-C00H, -(CH2)m-C(0)NA2 or by a C5-C10-cycloalkyI group. C5-C10-cycloalkyI group, or R7 means a C5-C10-cycloalkyI group, which is unsubstituted or substituted by-A, -(CH2)m-0H, -(CH2)m-COOH, -(CH2)m-C(0)NA2 or by a C5-C10-cycloalkyI group, and R means branched or unbranched C1-C6-alkyl, C2-C6-alkenyl, C2-C6-alkinyl, C5-C10-cycloalkyl, Het or Ar which are optionally substituted by one ore more halogen, C1-C6-alkyloxy, branched or unbranched C1-C6-alkyl, C2-C6-alkenyl, C2-C6-alkinyl or C5-C10-cycloalkyI groups or by -CrC6-alkyl-Het, -C1-C6-alkyl-Ar, -O-C1-C6-alkyl-Het, -O-C1-C6-alkyl-Ar, Het or by Ar, wherein Het means a monocyclic or bicyclic, 5- up to 10-membered aromatic or non-aromatic ring containing 1 or 2 equal or different hetero-atoms as members of said ring, selected from the group consisting of nitrogen, oxygen and sulfur, which is unsubstituted or substituted by one or more hydroxy or carboxy groups, and wherein Ar means a monocyclic or bicyclic 5- up to 10-membered aromatic ring which is unsubstituted or substituted by one or more hydroxy or carboxy groups, and Z means (CH2)m, O, S, NH, NR, N-C(0)-R or NSO2R, A means H or C1-C4-alkyl and I, m and r are integers from 0 to 3, n and k are integers from 1 to 2, p is an integer from 0 to 1 and q is an integer from 1 to 3, in all its stereoisomeric forms and mixtures thereof in all ratios including all its physiologically tolerable salts. Physiologically tolerable salts are for example salts of inorganic and organic acids, e.g. hydrochloric acid, sulfuric acid, acetic acid, citric acid or p-toluenesulfonic acid, or salts of inorganic and organic bases, such as NH4OH, NaOH, KOH, Ca(0H)2, Mg(0H)2, diethanolamine or ethylenediamine, or salts of amino acids, such as arginine, lysine, lysyl-lysine or glutamic acid. One preferred embodiment of the present invention is a compound of formula I wherein n is 1. A further preferred embodiment is a compound of formula I wherein R in group X means Het or Ar which are optionally substituted by -C1-C6-alkyl-Het, -CrC6-alkyl-Ar, -O-C1-C6-alkyl-Het, -O-C1-C6-alkyl-Ar, Het or by Ar. More preferably, R in group X A preferred embodiment of the present invention is also compound of formula I wherein R in group X means Ar which is optionally substituted by -C1-C6-alkyl-Ar, -O-C1-C6-alkyl-Ar or by Ar. Preferably R in group X means Ar. In the compound of formula I X Is preferably a group of the following formula: Preferably, Y means -(CH2)r, wherein r is preferably 0 or 1 and k is preferably 1 or 2. A further preferred embodiment of the present invention is a compound of formula I wherein X is a group of the following formula wherein D preferably means -(CHzV-, wherein r is 0 or 1. An also preferred embodiment of the present invention compound of formula I wherein R1 is a group of the following formula wherein Z means preferably (CH2)m and m is 0 or 1. Preferably, R5 means -(CH2)r COOA, wherein A means preferably H, or R5 means -(CH2)i-COONH2., wherein I is 0. Preferably, R4 means -NH2 or -A, wherein A preferably means H, or preferably, R4 means -NHR1, wherein -NHR1 preferably means and I is preferably 0, or R5 of -NHR1 means preferably (CH2)i-NH2 and I Is preferably 0. A further preferred embodiment of the present invention is a compound A compound of formula I wherein R1 is a group of the following formula wherein Z means preferably -(CH2)m-.and m is preferably 1 and wherein R4 preferably means -NH2, and R5 preferably means -(CH2)rCOOA, wherein I is preferably 0 and wherein A preferably means H. A further preferred embodiment of the present invention is a compound A compound of formula I wherein R1 is a group of the following formula wherein R5 preferably means -(CH2)rC00A, wherein I is preferably 0 and A preferably means H. A further preferred embodiment of the present invention is a compound of formula I wherein R2 means A and A preferably means -CH3, or wherein R2 means -E-COOH, preferably -CH2-COOH, or wherein R2 means -E-OH, preferably -CH2-OH. A further preferred embodiment of the present invention is a compound of formula I wherein R3 Is a group of the following formula A further preferred embodiment of the present invention is a compound of formula I wherein R3 is a group of the following formula A further preferred embodiment of the present invention is a compound of formula I wherein R3 Is a group of the following formula wherein R7 is preferably a branched C1-C10-alkyI group, preferably -CH(CH3)2, -C(CH3)3, -CH(CH3)CH2-CH3 or -CH2-CH(CH3)2, and wherein R6 preferably means -H, -COOH, -CONH2, -CH2OH, -CON(CH3)2 or, more preferably, wherein R6 means wherein q is preferably 2. A further preferred embodiment of the present invention is a compound of formula I wherein R3 is a group of the following formula wherein R7 preferably means -CH(CH(CH3)2)2 or -CH2C(CH3)3. The compounds according to the present invention are unnatural (i.e. naturally not occuring), low molecular weight peptide derivatives which are able to inhibit the laminin/nidogen interaction in the nM concentration range. Surprisingly, the low molecular weight structures which have been found are capable of high-affinity binding to the laminin binding site of nidogen without this requiring an interaction with a tyrosine or histidine from a loop (loop c) adjacent to the actual binding sequence. It is all the more surprising that the low molecular weight peptide derivatives, with molecular weights between 550 and 800 Da, described in the present invention show inhibition of the same order of magnitude compared to the most active peptide described to date (IC50 of 22 nM) having a molecular weight of about 2700 Da (= about 50% of an LE module) and comprising an intact S-S loop which presumably stabilizes the structure of the essential NIDPNAV sequence region (J.W. Fox and R. TimpI; US 5,493,008). The object was achieved by specifically synthesizing, on the basis of structure/function relationships and the published three-dimensional structure of the nidogen binding site, peptide derivatives on resin supports. The building blocks for the peptide syntheses were varied in accordance with suitable criteria to ensure a wide structural diversity and the integration of unnatural building blocks. A suitable, sensitive screening assay was used to test and compare the resulting peptide derivatives for inhibitory activity after they had been cleaved off the support resin. The compounds according to the present invention can be used for preparing a pharmaceutical for the treatment of a disease which is related to an increased or unwanted synthesis of basement membranes. Therefore, possible areas of therapeutic use of the present peptide derivatives and/or the physiologically tolerable salts thereof are: 1. All types of late complications of diabetes which are accompanied by thickening of basement membranes (especially in the kidney, eye, vascular system). 2. Hepatic fibrosis, especially alcoholic hepatic fibrosis, characterized by synthesis of a continuous basement membrane in the sinusoids and a capillarization caused thereby. 3. All fibroses (chronic or iatrogenic) in which an increased synthesis of basement membrane or components of the basement membrane can be observed (kidney, lung, skin). 4. Atherosclerosis characterized by a limitation of the regulation of lipid metabolism, which may be caused inter alia by impaired filtration of lipoproteins through the partly capillarized liver sinusoids. The pathological changes in the vascular system which can be obsen/ed with atherosclerosis may also in part be attributed to modifications of the composition and structure of the basement membranes in the vessels. 5. Diseases in which angiogenesis contributes to a deterioration in the clinical picture, for example cancers in which neovascularization is required for tumor growth, diabetic retinopathy, retrolental fibroplasia, disorders with a strong inflammatory component (for example rheumatoid arthritis, osteoarthritis, vasculitis), hemangiomas, psoriasis, and many others. Thus, the compounds according to the present invention and/or their respective physiologically tolerable salts are suitable for use as a pharmaceutical. Therefore, a further object of the present invention is a pharmaceutical composition containing at least one compound according to the present invention and/or its physiologically tolerable salts. The compounds of the formula I and their physiologically tolerable salts and derivatives can be administered according to the invention to animals, preferably to mammals, and in particular to humans, as pharmaceuticals for therapy or prophylaxis. They can be administered per se, in mixtures with one another or in the form of pharmaceutical preparations which permit enteral or parenteral administration and which as active constituent contain an efficacious dose of at least one compound of the formula I and/or its physiologically tolerable salts and derivatives in addition to customary pharmaceutically innocuous excipients and/or additives. The pharmaceuticals can be administered systemically or locally. They can be administered, for example, in the form of pills, tablets, film-coated tablets, sugar-coated tablets, granules, hard and soft gelatin capsules, powders, solutions, syrups, emulsions, suspensions or in other pharmaceutical forms. However, administration can also be carried out vaginally or rectally, for example in the form of suppositories, or parenterally or by implantation, for example in the form of injection solutions or infusion solutions, microcapsules or rods, or topically or percutaneously, for example in the form of ointments, solutions or tinctures, or in another way, for example in the form of nasal sprays or aerosol mixtures or as inhalable dry powder preparations. If solutions are parenterally administered they can be aministered, for example, intravenously, intramuscularly, subcutaneously, intraarticularly, intrasynovially or in another manner, e.g. by inhalation of wet aerosols or dry powder preparations. The pharmaceutical preparations according to the invention are prepared in a manner known per se, it being possible to use pharmaceutically inert inorganic and/or organic excipients in addition to the compound(s) of the formula I and/or its/their physiologically tolerable salts and derivatives. For the preparation of pills, tablets, sugar-coated tablets and hard gelatin capsules, it is possible to use, for example, lactose, cornstarch or derivatives thereof, talc, stearic acid or its salts etc. Excipients for soft gelatin capsules and suppositories are, for example, fats, waxes, semisolid and liquid polyols, polyethylene glycols, natural or hardened oils etc. Suitable excipients for the preparation of solutions, for example injection solutions, or of emulsions or syrups are, for example, water, alcohols, glycerol, diols, polyols, sucrose, invert sugar, glucose, vegetable oils etc. Suitable excipients for microcapsules, implants or rods are, for example, copolymers of glycolic acid and lactic acid. The pharmaceutical preparations normally contain approximately 0.5 to 90% by weight of the compounds of the formula I and/or their physiologically tolerable salts and derivatives. In addition to the active compounds and excipients, the pharmaceutical preparations can additionally contain auxiliaries or additives, such as, for example, fillers, disintegrants, binders, lubricants, wetting agents, stabilizers, emulsifiers, preservatives, sweeteners, colorants, flavorings or aromatizers, thickeners, diluents, buffer substances, solvents or solubilizers, means for achieving a depot effect, salts for altering the osmotic pressure, coating agents or antioxidants. They can also contain two or more compounds of the formula I and/or their physiologically tolerable salts and derivatives. Furthermore, they can also contain one or more other therapeutically or prophylactically active substances in addition to at least one compound of the formula I and/or its physiologically tolerable salts and derivatives. The pharmaceutical preparations normally contain 0.2 to 500 mg, preferably 1 to 100 mg, of active compound of the formula I and/or its physiologically tolerable salts and derivatives per dose. If the compounds of the formula I or pharmaceutical preparations containing them are administered as aerosols, for example as nasal aerosols or by wet aerosols or dry powder inhalation, this can be effected, for example, using a spray, an atomizer, a pump atomizer, an inhalation apparatus, a metered inhaler or a dry powder inhaler, respectively. Pharmaceutical forms for administration of the compounds of the formula I as an aerosol can be prepared by the process well known to the person skilled in the art. For their preparation, for example, solutions or dispersions of the compounds of the formula I in water, water-alcohol mixtures or suitable saline solutions using customary additives, for example benzyl alcohol or other suitable preservatives, absorption enhancers for increasing the bioavailability, solubilizers, dispersants and others, and, if appropriate, customary propellants, for example chlorofluorohydrocarbons and/or fluorohydrocarbons are suitable, whereas dry powder preparations of the compounds of the formula I and/or their physiologically tolerable salts may be obtained by freeze drying or preferably spray drying aqueous solutions of the compounds of the formula I and/or their physiologically tolerable salts and of suitable water soluble additives, such as sugars or sugar derivatives and amino acids. The dose when using the compounds of the formula I can vary within wide limits, and as customary it is to be tailored to the individual conditions in each individual case, as is known to the physician. It depends, for example, on the nature and severity of the disease to be treated, on the compound employed or whether an acute or chronic disease state is treated or prophylaxis is conducted or on whether further active compounds are administered in addition to the compounds of the formula I. In general, in the case of oral administration, a daily dose of approximately 0.01 to 100 mg/kg, preferably 0.1 to 10 mg/kg, in particular 0.3 to 2 mg/kg (in each case per kg of body weight) is appropriate in an adult to achieve effective results. In the case of intravenous administration, the daily dose is in general approximately 0.01 to 50 mg/kg, preferably 0.01 to 10 mg/kg of body weight. In particular when relatively large amounts are administered, the daily dose can be divided into a number, for example 2, 3 or 4, of part administrations, if appropriate, depending on individual behavior, it may be necessary to deviate upward or downward from the indicated daily dose. Furthermore, the compounds of the formula I and their salts according to the present invention can be used as intermediates for the preparation of other compounds, in particular of other pharmaceutical active compounds which are obtainable from compounds of the formula I, for example, by modification or introduction of radicals or functional groups, for example by esterification, reduction, oxidation or other conversions of functional groups. The peptide derivatives according to the present invention thus found can on the one hand be used directly as therapeutic agent, but they can also form the basis for related structures, which are also suitable for use as therapeutic agent for treating diseases relating to an increased or unwanted synthesis of basement membranes. A further object of the present invention is a method for identifying a compound that inhibits the interaction of laminin and nidogen wherein the compound according to the present invention is used as a competetive Inhibitor. This method may further comprise the formulation of the compound identified in a pharmaceutical acceptable form. It is also an object of the present invention to provide a method for producing a pharmaceutical composition comprising the identification of a compound that inhibits the interaction of laminin and nidogen wherein the compound according to the present invention is used as a competetive inhibitor and furthermore mixing the compound identified and/or its physiologically tolerable salts with a pharmaceutical acceptable carrier. It is also an object of the present invention to provide a method for preparing the compound of the formula I according to the present invention. wherein the variables R1, X, n, R2 and R3 have the above-mentioned meanings and whereby the compounds of formulae II and III may be protected at the functional groups defined above by usual protecting groups known in peptide chemistry (see for example Houben-Weyl, Methoden der Organischen Chemie, vol. 15/1 and 15/2, Georg Thieme Verlag, Stuttgart, 1974). Suitable condensation methods are well known in the art (Houben-Weyl, Methoden der Organischen Chemie, vol. 15/1 and 15/2, Georg Thieme Verlag, Stuttgart, 1974). Suitable condensation agents or coupling reagents are for example carbonyl-diimidazoles, carbodiimides, such as dl-cyclohexyl-carbodiimide or di-isopropyl-carbodiimide, or O-((cyano(ethoxycarbonyl)methylene)-amino)-N,N,N',N'-tetra-methyl-uronium-tetrafluoro-borate (TOTU) or pyro-phosphoric acid anhydride (PPA). The condensation reactions are carried out under standard conditions. As a rule, it is necessary during peptide condensation to protect amino groups which are not intended to be involved in the coupling reaction by protecting groups which are easily removed under conditions different to the conditions under which coupling occurs. The same applies for the carboxy groups not involved in the coupling reaction, which are preferably protected as C1-C6-alkyI esters, benzyl esters or tert-butyl esters during the coupling reaction. A protection of the amino groups is not necessary in case the amino groups are still present in the form of amino group precursors, e.g. in form of nitro or cyano groups. The amino groups are then formed by a hydration step subsequent to the condensation reaction. After the condensation step the protecting groups are removed by known suitable methods, e.g. benzyloxy-carbonyl and benzyl groups can be removed by hydration in benzyl esters; protecting groups of the tert-butyl type are in general cleaved under acidic conditions; the 9-fluorenylmethyloxycarbonyl residue is removed by secondary amines. The preparation of the compound of the formula I according to the present invention may also be performed by stepwise addition of the respective components, e.g. natural, unnatural amino acids and their derivatives, on a solid phase, whereby the components may be added in various different sequences. It may also be advantageous in order to produce the compound of formula I not to directly couple the compounds of formulae I and II by a fragment condensation but to couple their respective suitable precursors in order to obtain an intermediate which can be transferred into the compound of the formula I e.g. by derivatization. The above described method for introducing functional groups not directly, but by the way of their respective precursors into the molecule in order to obtain intermediates from which the final product can easily be obtained by transforming the precursor groups into the respective functional groups subsequently to a condensation reaction may also be applied for different parts of the molecule of the compound of formula I, e.g. for the side chain of the compound of formula, I R1- or R1-X-, respectively. Examples The abbreviations have the following meanings: Agents and solvents: AcOH aq BSA DCC DCM DIPEA DMAP DMF DMSO Et20 EtOAc EtOH Fmoc-OSucc HOBT KHMDS n-Buli MeOH MTBE acetic acid aqueous bovine serum albumin N,N'-dicyclohexylcarbodiimide dichloromethane N,N-diisopropylethylamine 4-dimethylaminopyridine N,N-dimethylformamide Dimethylsulfoxide Diethylether Ethylethanoate (acetic acid ethylester) ethanol Fmoc-0-succinimide 1 -hydroxybenzotriazole potassiumhexamethyldisilazide n-butyl-lithium methanol methyl tert-butyl ether TEA TFA THF TMEDA TMSCI TOTU TrisNs triethylamine trifluoroacetic acid tetrahydrofuran tetramethylethylendiamine trimethylsilyl chloride 0-((cyano(ethoxycarbonyl)methylene)amino)- N,N,N',N'-tetramethyluroniunn tetrafluoroborate trisilyl azide 1. Screening of a library of inhibitors of Laminin/Nidogen interaction The library was designed to find smaller, more potent and more metabolically stable peptides related to the previously known heptapeptide NIDPNAV (PoschI, E.; Fox, J.W.; Block, D.; Mayer, U.; TimpI, R, (1994) EMBO J. 13; 3741-3747. PoschI, E.; Mayer, U.; Stetefeld, J.; Baumgartner, R.; Holak, T.A.; Huber, R.; TimpI, R. (1996) EMBO J. 15: 5154-5159. Baumgartner, R.; Czisch, M.; Mayer, U.; PoschI, E.; Huber, R.; TimpI, R.; Holak, TA (1996) J. Mol. Biol. 257; 658-668). The library was synthesized and screened as three sublibraries; pentamer, hexamer and heptamer. Following is a description of the screening strategy for the pentamer sublibrary. The method is representative of the methods employed for the other two sublibraries, except that the hexamers were screened in the first step at about 50 beads per well and the heptamers were screened at about 100 beads per well. 1.1 Screening of the pentamer library. The pentamer library contained 2,160 different compounds. 1) About 8,800 individual beads were suspended in 0.1% HCI and distributed into seven filter bottom 96 well microtiter plates at approximately fourteen beads per well. 2) The beads were washed twice with 200 :l de-ionized water, then 50 :1 of 500 mM HEPES, pH 7.0 was added. The linker used in the library releases one aliquot of compound when the pH is increased to 7.0, and this cleavage step was allowed to proceed overnight. 3) The plates were stacked on top of U-bottom filter plates and centrifuged. The mixtures of compounds released from the beads were collected in the bottom plate, while the corresponding beads remain in the original filter plate. 4) 25 :l DMSO per well was added to the beads to wash remaining free compound from the beads, and the plates were centrifuged again to separate the compounds in solution from the beads. The resulting stock was presumably 27 :M per compound in 333 mM HEPES, 33% DMSO. 5) The compound stocks were preincubated with nidogen (10 :l compound stock to 90 :l nidogen solution) and the assay was performed as described in the attached protocol, yielding a final screening concentration of 2.7 :M per compound. 6) In the 25 assay wells where reproducible inhibition of 62% occurred, the corresponding beads from the original filter plates were suspended in 0.05% HCI, 0.1% Tween-20 and pipetted into five new filter plates at 1 bead per well. Two control beads with the parent compound on the same linker were added to each plate as controls. 7) The beads were washed twice with 200 :l de-ionized water, then 25 :l of 50 mM NaOH was added to each well. The linker used in the library releases the second equimolar aliquot of compound when the pH is increased from 7.0 to 10.0 or more. This cleavage step was allowed to proceed for 3 hours. 8) The plates were stacked on top of U-bottom filter plates and centrifuged. The compounds released from the beads were collected in the bottom plate, while the corresponding beads remained in the original filter plate. 9) The beads were washed with 20 :l of 50 mM HEPES (initial pH 7.0) with 50 mM HCI added, and the solution was centrifuged into the lower plate and combined with the first releasate. 10) The beads were washed a third time with 25 :l DMSO, which was allowed to equilibrate with the beads for 10 minutes before centrifugation. 11) The resulting releasates were assayed at 1/10th volume, as in Step #5. 12) Solutions which inhibited as well or better than the control beads (about 50% inhibition) were considered hits. 23 hit beads were recovered, with the other two potential hit wells being explainable by additive weak inhibitors In single wells. 13) Hit solutions were subjected to mass spectrometry to determine the molecular weights. 14) The corresponding individual hit beads were subjected to Edman degradation to determine peptide sequences. 15) The combined MS and Edman data was analyzed to identify the hit compound structures. The structures and frequency of their recovery are shown below. G-Hopa = glycine hydroxypropyl amide, the linlcer remnant. D = Asp (aspartyl), P = Pro (prolyl), N = Asn (asparaginyl), A = Ala (alanyl), V = Val (vallnyl), S = Sen (seryl), I = He (isoleucyl). 1.2 Procedures: Preparation of the peptide library Peptide libraries were synthesized by a split/mix synthesis approach (Lam, K. S., Salmon, S. E., Hersh, E. M., Hruby, V. J., Kazmierski, W. M., and Knapp, R. J. (1991) Nature 354, 82; Furka, A., Sebestyen, F., Asgedom, M., and Dibo, G. (1991) Int. J. Pept. Protein Res. 37, 487) using standard solid-phase peptide Fmoc chemistry (Stewart, J. M., and Young, J. D. (1984) Solid Phase Peptide Synthesis. Pierce Chemical Co., Rockford, IL.; Atherton, E., and Sheppard, R. C. (1989) Solid Phase Peptide Synthesis. IRL Press Oxford). Each resin bead was exposed to only a single activated amino acid at each coupling cycle. Therefore, at the completion of the library synthesis, each resin bead expresses only one peptide entity. Since it is not possible to test all compounds separately, we have built the same structure on each resin bead in two copies via differentially cleavable linker, fig. 1 (Kocis, P., Krchnak, V., and Lebl, M. (1993) Tetr.Lett. 34, 7251; Lebl, M., Krchnak, V., Salmon, S.E., and Lam, K. S. (1994) A Companion to Methods in Enzymolog 6, 381). Release of the peptide from the resin bead can then be carried out in sequential steps using different mechanism of cleavage. Release of the first part of peptide as a hydroxypropylamide is performed in buffer at pH 7-9. The release of the second part of the peptide is achieved by the use of higher pH (Scheme 1). In the peptide libraries, polyethylene glycol-grafted polystyrene beads or TentaGel®S NH2 were used. In fact, any resin beads that are compatible with peptide synthesis and screening under aqueous conditions are adequate. Penta-, hexa-, and heptamer library were prepared with one fixed position (L-asparagine). Glycine hydroxypropylamide on C-terminus is a part of a linker: H-X4X3-Asn-X2X1-Gly-NH (CH2)30H (2,160 peptides) H-X5X4X3-Asn-X2X1-Gly-NH (CH2)30H (25,920 peptides) H-X6X5X4X3-Asn-X2X1-Gly-NH (CH2)30H (311,040 peptides) XI: N-Fmoc-L-amino acids (9) used in the first randomization: Valine, isoleucine, threonine, phenylalanine, fS(2-naphthyl)alanine, 2-azetidinecarboxylic acid, proline, cyclohexylglycine, phenylglycine. X2: N-Fmoc-L-amino acids (4) used in the second randomization: Alanine, glycine, serine, aspartic acid. X3=X5=X6: N-Fmoc-L-amino acids (12) used in the third, fifth and sixth randomization: Pipecolicacid, (S(2-naphthyl)alanine, glutamic acid, lysine, 2-azetidinecarboxylic acid, threonine, proline, asparagine, isoleucine, 3,5-diiodotyrosine, citrulline, arginine. X4: N-Fmoc-L-amino acids (5) used in the fourth randomization: Aspartic acid, glutamic acid, 2-aminoadipic acid, O-sulfate tyrosine, (-carboxyglutamic acid. Resin (PEG-PS-HCI, Millipore®, 20 g, loading 0.58 mmol/g, 220 |jm average particle size) was swollen in N,N-dimethylformamide for 2 hours and then neutralized with 10% N,N-diisopropylethylamine in dichloromethane. Resin was washed with dichloromethane and N,N-dimethylformamide. Linker (Fig.1, 3 eq) was coupled using 1,3-diisopropylcarbodiimide and 1-hydroxybenzotriazole (3 eq each) in N,N-dimethylformamide at room temperature for 12 hours. The reaction was monitored by bromophenol blue method (Krchnak, V., Vagner, J., Safar, P., and Lebl, M. (1988) Collec.Czech.Cem, Commun.53, 2542). Completion of the coupling was then determined by a ninhydrin test (Kaiser, E., Colescott, R. L., Bossinger, C. D., and Cook, P.I. (1969) Anal. Biochem. 34, 595). After washing with N,N- dimethylformamide, Fmoc protecting group was removed with 50 % piperidine in N,N-dimethylformamide for 15 min. Resin was then washed with N,N-dimethylformamide and the amount of released fulvene-piperidine adduct was quantitated by UV spectrometry (302 nm). A stable level of resin loading (mmol/g) determined in this manner throughout the library synthesis served as one of the quality control measures. The resin was divided into 9 equal portions. Nine Fmoc-protected amino acids (XI) were then added separately into each of the resin aliquot and coupled by described procedure for 2 hours. The resin was then pooled in a cylindrical glass vessel fitted with a frit at the bottom. Dry nitrogen was bubbled through for mixing of the resin. Fmoc protecting group was removed as described above. The resin was divided into 4 equal portions. Four Fmoc-protected amino acids (X2) were then added separately into each of the resin aliquot and coupled using the same coupling protocol. Fmoc protecting group was removed and resin loading was determined. In next cycle, L-asparagine was coupled by described procedure. The resin was then divided into aliquots for another cycle of coupling. After all the randomization steps were completed, the Fmoc group was removed and the side chain protecting groups were cleaved with a mixture of trifluoroacetic acid (82.5%), anisole (5%), water (5%), thioanisole (5%), ethanedithiole (2.5%) during 2,5 hours. The resin was then washed with trifluoroacetic acid, dichloromethane, N,N-dimethylformamide and methanole. The libraries were stored dried at 4°C. To verify the quality of the library, several randomly chosen beads were submitted for sequencing by Edman degradation and mass spectrometric techniques. 2.1.1 Ethyl trans-3-(2'-naphthyl)-propenoate (A1) To a stirred solution of 2-naphthaldehyde (7.8 g, 50 mmol) in 50 mL ethanol was added (carbethoxymethylene)triphenylphosphorane (18.3 g, 52.5 mmol). A slight exotherm was noted. A precipitate formed while the mixture stirred overnight. The reaction mixture was diluted with Et20 (500 mL) and washed with 1 M H3PO4 (2 x 100 mL), saturated NaHCOa (1 x 100 mL), water (100 mL), and brine (100 mL). The organic fraction was dried (MgS04) and concentrated under reduced pressure. The residue was passed through a Si02 plug eluting with 9:1 hexane:EtOAc. After concentration in vacuo, a near quantitative yield of the product as an 85:15 mixture of geometric isomers (favoring trans, nmr) was recovered. The material was recrystallized from hexane/EtOAc (rich in hexane) to recover 4.5 g of the desired product as a 97:3 mixture of isomers (nmr). The mother liquor was concentrated and recrystallized as before to recover an additional 2.9 g (total 7.4 g, 33 mmol, 65% yield). NMR (CDCI3) * 7.93 (s, 1 H); 7.88-7.83 (c, 4 H); 7.67 (dd, 1 H, J = 1.6, 8.6 Hz); 7.53-7.50 (c, 2 H); 6.55 (d, 1 H, J = 16.0 Hz); 4.30 (q, 2 H, J = 7.1 Hz); 1.42 (t, 3 H, J = 7.1 Hz), 2.1.2 trans-3-(2'-Naphthyl)-propenoic acid (A2) To a solution of ester A1 (4.24 g, 18.8 mmol) in THF (75 mL) was added LiOHH20 (2.36 g, 56.3 mmol) in water (19 mL). The initially heterogenous mixture was stirred vigorously overnight and became homogenous. The reaction mixture was acidified with concentrated HCI (pH « 2) and a precipitate formed. The heterogenous mixture was transferred to a separatory funnel and extracted with EtOAc (3 x 150 mL). The combined extracts were dried (MgS04) and concentrated in vacuo to recover the carboxylic acid as a white solid (3.66 g, 98% yield). NMR (CDCI3) * 7.97 (d, 1 H, J = 15.7 Hz); 7.90 (d, 1 H, J = 15,3 Hz); 7.90-7.83 (c, 3 H); 7.70 (dd, 1 H, J = 1.6, 8.6 Hz); 7.57-7.50 (c, 2 H); 6.58 (d, 1 H, J = 16.0 Hz). 2.1.3 trans-(4S)-3-(3'-(2"-Naphthyl)-propenoyl)-4-phenyl-2-oxazolidinone (A3) A solution of carboxylic acid A2 (3.66 g, 18.5 mmol) and triethylamine (1.87 g, 2.56 mL, 18.5 mmol) in anhydrous THF (74 mL) was cooled to -78 ° C. PivaloyI chloride (2.35 g, 2.40 mL, 19.4 mmol) was added over two minutes accompanied by formation of a white precipitate. After 10 minutes, the flask was placed in a 0 ° C bath for a duration of 10 minutes after which the flask cooled back to -78 ° C for 1.5h. In a separate flask the oxazolidione derived from L-phenylglycinol (3.31 g, 20.3 mmol) in anhydrous THF (74 mL) was cooled to -78 ° C. A solution of n-BuLi (1.6 M in hexane, 11.6 mL, 18.5 mmol) was added and stirring continued for about 1 h accompanied by the metalated oxazolidinone precipitating from the THF/hexane solution. The mixed anhydride was added via cannula to the metallated oxazolidinone and the reaction mixture placed in a 0 ° bath. After 1 h the bath was removed and the mixture warmed to room temperature overnight. The reaction was quenched with 50 mL saturated NH4CI. THF was removed under reduced pressure and, after transfer to a separatory funnel, the mixture was extracted with CH2CI2 (3 x 75 mL). The combined organic fractions were washed with 1 M NaOH (2 x 50 mL), dried (MgS04) and concentrated. The residue was recrystallized from EtOAc/hexane to recover a white solid (3.87 g, 11.2 mmol, 61 % yield). NMR (CDCI3) * 8.05 (d, 1 H, J = 15.7 Hz); 7.94 (d, 1 H, J = 15.4 Hz); 7.87-7.81 (c, 3 H); 7.76 (dd, 1 H, J = 1.5, 8.6 Hz); 7.53-7.47 (c, 2 H); 7.41-7.34 (c, 5 H); 5.58 (dd, 1 H, J = 8.7, 3.9 Hz); 4.76 (t, 1 H, J = 8.7 Hz); 4.33 (dd, 1 H, J = 8.8, 3.9 Hz). 2.1.4 (3'R4S)-3-(3'-(2"-Naphthyl)-4'-pentenoyl)-4-phenyl-2-oxazoiidinone (A4) To a solution of Cul (3.96 g, 20.9 mmol) and TMEDA (2.66 g, 3.46 mL, 22.9 mmol) in anhydrous THF (92 mL) at -78 ° C was added vinylmagnesium bromide (1.0 M in THF, 20.9 mL, 20.9 mmol). The mixture was stirred for 15 minutes. In a separate flask trimethylsilyl chloride (5.69 g, 6.64 mL, 52.2 mmol) was added to a solution of unsaturated imide A3 (3.87 g, 11.3 mmol) in anhydrous THF (42 mL). Owing to insolubility of the imide, the septum of the flask containing the cuprate reagent was removed and the slurried imide added in one portion rinsing quickly with a small amount of THF. The bath temperature was raised to -30 ° C and stirring continued for 1 h. The reaction mixture was poured into 250 mL of a 3:2 mixture of saturated NH4CI;concentrated NH4OH. The layers were separated and the aqueous fraction extracted with EtOAc (3 x 200 mL). The combined organic fractions were washed sequentially with saturated NH4CI (1 x 100 mL) and water (1 x 100 mL). The organic fraction was dried (MgS04) and concentrated under reduced pressure. The residue was purified by passage through a plug of SiOz eluting with 4:1 hexane;EtOAc. The eluant was concentrated in vacuo to recover a white solid (3.64 g, 9.81 mmol, 87% yield). NMR (CDCI3) * 7.87-7.82 (c, 3 H); 7.72 (s, 1 H); 7.54-7.27 (c, 8 H); 6.11 (ddd, 1 H, J = 6.7, 10.4, 17.0 Hz); 5.34 (dd, 1 H, J = 8.6, 3.5 Hz); 5.10 (d, 1 H, J = 8.2 Hz); 5.08 (d, 1 H, J = 17.2 Hz); 4.56 (t, 1 H, J = 8.8 Hz); 4.26 (dd, 1 H, J = 8.8, 3.5 Hz); 4.16 (ddd, 1 H, J = 8.1, 7.0, 6.9 Hz); 3.68 (dd, 1 H, J = 8.4, 16.5 Hz); 3.50 (dd, 1 H, J = 6.5, 16.5 Hz). 2.1.5 (2'S3'R4S)-3-(2'-Azido-3'-(2"-naphthyl)-4'-pentenoyl)-4-phenyl-2-oxazolidinone (A5) Potassium hexamethyldisilazide (0.5 M in toluene, 25.5 mL, 12.8 mmol) was added in one portion to anhydrous THF (34 mL) at -78 ° C. Imide A4 (3.64 g, 9.81 mmol) was slurried in THF (34 mL) and added via cannula, rinsing with THF (2x11 mL) to complete the transfer. After 30 min, trisylazide (4.40 g, 14.2 mmol) was dissolved in THF (34 mL), cooled to -78 ° C, and added via cannula. Thirty minutes later, AcOH (1.41 g, 1.34 mL, 23.4 mmol) was added to quench the reaction. The mixture was stirred at room temperature overnight. The mixture was partitioned between CH2CI2 (300 mL) and dilute brine (150 mL). The layers were separated and the aqueous phase extracted with CH2CI2 (3 x 150 mL). The combined organic fractions were dried (MgS04) and concentrated under reduced pressure.The residue was purified by flash chromatography to recover the product (3.41 g, 8.28 mmol, 84 % yield). NMR (CDCI3) * 7.85-7.82 (c, 3 H); 7.72 (s, 1 H); 7.53-7.47 (c, 2 H); 7.42 (dd, 1 H, J = 1.7, 8.5 Hz); 7.37-7.31 (c, 3 H); 7.18-7.15 (c, 2 H); 6.28 (ddd, 1 H, J = 8.2, 10.2, 17.1 Hz); 5.63 (d, 1 H, J = 10.2 Hz); 5.37 (d, 1 H, J = 17.0 Hz); 5.34 (d, 1 H, J = 10.2 Hz); 4.83 (dd, 1 H, J = 3.0, 8.3 Hz); 4.14 (t, 1 H, J = 7.2 Hz); 4.07 (dd, 1 H, J = 9.3, 17.9 Hz); 3.94 (dd, 1 H, J = 3.0, 5.8 Hz); 3.68 (t, 1 H, J = 8.6 Hz). 2.1.6 Methyl (2S3R)-2-Azido-3-(2'-naphthyl)-4-pentenoate (A6) To a solution of imide A5 (3.41 g, 8.28 mmol) in THF (62 mL) was added water (21 mL), 35% H2O2 (2.7 mL), and LiOHHzO (695 mg, 16.6 mmol). Atter 2 hours Na2S03 (4.17 g, 33.1 mmol) was added as a solution in water (41 mL). The mixture was stirred for 15 minutes and THF removed under reduced pressure. The aqueous solution was acidified with HCI and extracted with EtOAc (2 x 150 mL). The combined extracts were dried (MgS04) and concentrated under reduced pressure. The residue was passed through a Si02 plug column eluting with 1:1 hexane:EtOAc to recover, after concentration, a white solid that was presumably a mixture of the carboxylic acid and chiral auxiliary. Recrystallization from hexane/EtOAc yielded the chiral auxiliary as needles. The mother liquor was concentrated and earned on to the esterification step. The residue containing the crude carboxylic acid was dissolved in anhydrous MeOH (46 mL) and cooled to 0 ° C. Thionyl chloride (1.18 g, 725 :L, 9.94 mmol) was added and, after 10 minutes, the mixture heated at reflux for 2 hours. Water (1.0 mL) was added to the mixture, stirred for 10 minutes, and the contents of the flask concentrated under reduced pressure. The residue was partitioned between EtOAc (150 mL) and brine (100 mL). The layers were separated and the organic fraction was dried (MgS04) and concentrated under reduced pressure. The residue was purified by flash chromatography (19:1 hexane: EtOAc) to recover the methyl ester (1.54 g, 5.48 mmol, 66% yield). NMR (CDCI3) * 7.84-7.80 (c, 3 H); 7.71 (s, 1 H); 7.50-7.46 (c, 2 H); 7.39 (dd, 1 H, J = 1.8, 8.5 Hz); 6.23 (ddd, 1 H, J = 8.3, 10.9, 17.6 Hz); 5.30 (d, 1 H, J = 9.9 Hz); 5.28 (d, 1 H, J = 17.7 Hz); 4.22 (d, 1 H, J = 7.5 Hz); 4.06 (t, 1 H, J = 7.9 Hz). 2.1.7 trans-3-(2'-naphthyl)-L-proline methyl ester (A7) Borane-methyl sulfide complex (2.0 M in THF, 6.57 mL, 13.1 mmol) was diluted with anhydrous THF (26 mL) and cooled to 0 ° C. Cyclohexene (2.16 g, 2.66 mL, 26.3 mmol) was added cautiously via syringe. After 30 minutes a white precipitate had formed. Stirring was continued for three hours. The contents of the flask were concentrated in vacuo. The reagent was slurried in CH2CI2 (36 mL) and cooled to 0 ° C. Vinyl azide A6 (1.23 g, 4.38 mmol) was dissolved in CH2CI2 (9 mL) and added via cannula. The reaction mixture became pale yellow and gas evolution was evident. The mixture was warmed to room temperature overnight. Added MeOH (26 mL) and stirred for an additional 15 minutes. The mixture was concentrated under reduced pressure. The residue was taken up in Et20 (25 mL) and extracted with 0.1 M HCI (5 X 25 mL). The aqueous extracts were basicified with saturated NaHCOs and extracted with CH2CI2 (3 x 100 mL). The organic extracts were dried (MgS04) and concentrated in vacuo to recover the cyclized product along with some dicyclohexyl borane derived contaminants (974 mg, 3.82 mmol, 87% yield of crude material). NMR (CDCI3) * 7.84-7.78 (c, 3 H); 7.71 (s, 1 H); 7.49-7.41 (c, 3 H); 3.91 (d, 1 H, J = 6.9 Hz); 3.69 (s, 3 H); 3.63 (m, 1 H), 3.48 (dd, 1 H, J = 8.2, 15.4 Hz); 3.27 (d, 1 H, J - 7.8 Hz); 3.25 (d, 1 H, J = 7.8 Hz); 2.33 (m, 1 H), 2.09 (m, 1 H). 2.1.8 N-Fmoc-trans-3-(2'-naphthyl)-L-proline(A8) 510 mg (2 mmol) of methyl ester (A7) in 12 ml of 6N HCI are heated 100°C for 10 hours. The reaction solution is concentrated under reduced pressure and the solid residue is suspended in 15 ml of acetone. The suspension is adjusted to pH 9-10 using 2N NaaCOs solution. 742 mg (2.2 mmol) of Fmoc-0-succinimide are then added slowly. The pH is subsequently adjusted to 9-10 and the mixture is stirred at room temperature for 4 hours and then allowed to stand at room temperature overnight. The pH is subsequently adjusted to 2 using cone. HCI, and the mixture is admixed with ethyl acetate. 560 mg of the precipitated product are filtered off with suction. The aqueous phase is extracted three times with ethyl acetate and subsequently admixed with methylene chloride. This gives a further 185 mg of product as a precipitate. Yield:745 mg (80.4%). NMR (d6-DMSO) * 7.95- 7.80 (c, 6 H); 7.68 (d, 1 H, J = 7.3 Hz); 7.60 (d, 1 H, J = 7.4 Hz); 7.50-7.34 (c, 6 H); 7.25 (m, 1 H), 4.39-4.15 (c, 4 H); 3.70-3.48 (c, 3 H); 2.29 (m, 1 H); 2.14 (m, 1 H). 2.2 N-Succinyl-trans-3-(2'-naphthyl)-L-prolyl-L-asparaginyl-L-alaninyl-L-valine-amide (34) 2.2.1 N-Fmoc-trans-3-(2'-naphthyl)-L-proline-L-asparagine-L-alanine-L-valine-amide (B1) 463.5 mg (1 mmol) of/\/-Fmoc-trans-3-(2'-naphthyl)-L-proline (AS), 338 mg of H-Asn-Ala-Val-NHa hydrochloride (prepared according to customary methods of peptide chemistry) and 135 mg of HOBT are dissolved in 20 ml of DMF. At 0°C, 0.13 ml of N-ethylmorpholine and 220 mg of DCC are added. The mixture is stirred at 0°C for 1 hour and then at room temperature for 3 hours and is subsequently allowed to stand at room temperature overnight. The precipitate is filtered off with suction and the solution is concentrated under high vacuum. The residue is partitioned between pentanol and NaHCOa solution. The pentanol phase is washed with KHSO4 solution and HaO/NaCI solution. The precipitate is filtered off with suction and thoroughly triturated with diethyl ether. This gives 473 mg of product. The pentanol phase is dried using Na2S04 and concentrated. The residue is triturated twice with diethyl ether. This gives another 257 mg of product. Yield; 730 mg (97.7%). 2.2.2 trans-3-(2'-Naphthyl)-L-proline-L-asparagine-L-alanine-L-valine-amide (B2). 248 mg (0.332 mmol) of A/-Fmoc-trans-3-(2'-naphthyl)-L-proline-L-asparagine-L-alanine-L-valine-amide B1 are taken up in 5 ml of DMF. 0.35 ml (3.32 mmol) of diethylamine are added and the mixture is stirred at room temperature for 15 minutes. The mixture is filtered off with suction through a clarifying layer and concentrated under high vacuum. The solid residue is triturated with diethyl ether and filtered off with suction. Yield; 141 mg (81%). 2.2.3 Methyl tert-butyl succinate (B3). Under argon, 13.2 g (100 mmol) of monomethyl succinate are suspended in 500 ml of methylene chloride. Over a period of 30 minutes, 12.9 ml (150 mmol) of oxalyl chloride are added dropwise, and the mixture is subsequently stirred at room temperature for 6 hours. After approximately 3.5 hours, a clear solution results. 300 ml of tert-butanol are subsequently added dropwise. The mixture is then allowed to stand at room temperature for 21 hours, and the clear solution is concentrated. The residue is dissolved in ethyl acetate and washed with H2O, NaHCOa solution and H2O. The solution is dried with Na2S04 and concentrated. Yield: 21.6 g (crude oil-like product). 2.2.4 Mono-tert-butyl succinate (B4) 9.4 g (50 mmol) of methyl tert-butyl succinate (83) are dissolved in 115 ml of 1,4-dioxane. 110 ml of 0.5N NaOH are subsequently added. The mixture is allowed to stand at room temperature, and product precipitates out. The mixture is allowed to stand at room temperature over the weekend and is subsequently concentrated. The aqueous solution is extracted using diethyl ether. The aqueous phase is cooled to 0°C and acidified to pH 4 using cold 2N H2SO4. The mixture is subsequently extracted five times using diethyl ether. The organic phases are combined, washed with H2O, dried with Na2S04 and concentrated. Yield: 5.62 g of an oil (64.5%). 2.2.5 N-tert-Sutyl-succinyl-trans-3-(2'-naphthyl)-L-proline-L-asparagine- L-alanine-L-valine-amide (85) 262 mg (0.5 mmol) of/rans-3-(2'-naphthyl)-L-proline-L-asparagine-L-alanine-L-valine-amide (B2), 87.1 mg (0.5 mmol) of mono-tert-butyl succinate ( B4) and 67.5 mg of HOBt are dissolved in 5 ml of DMF. At 0°C, 110 mg of DCC are added and the mixture is stirred at O'C for 1 liour and then at room temperature for 2 hours and allowed to stand at room temperature overnight. The precipitate is filtered off with suction and the filtrate is concentrated under high vacuum. The residue is triturated with NaHCOs solution, filtered off with suction, washed with H2O and dried in a desiccator. Yield: 169 mg (49.6%). 2.2.6 N-Succinyl-trans-3-(2'-naphthyl)-L-proline-L-asparagine-L-alanine-L-valine-amide (34) 316 mg of A/-tert-butyl-succinyi-?rans-3-(2'-naphthyl)-L-proline-L-asparagine-L- alanine-L-valine-amide (85) are dissolved in 2 ml of 90% strength trifiuoroacetic acid and allowed to stand at room temperature for 1 hour. The mixture is subsequently filtered through a clarifying layer and concentrated. The residue is triturated with diethyl ether and filtered off with suction. This gives 159 mg of crude product. For purification, the substance is chromatographed over Sephadex® LH20 using a butanol/glacial acetic acid/water mixture. Yield: 27.5 mg (9.5%). m/z: 625.298949 (M+H)"" (high resolution mass spectrum). 2.3.1 Benzyloxycarbonyl-glycine-(3-propanol)amide (C1) 627 g (30 mmol) of Gly-OH, 2.45 ml of 3-amino-1-propanol and 4.05 g of HOBt are dissolved in 60 ml of DMF. At 0°C, 6.6 g of DCC are added. The mixture is stirred at 0°C for 1 hour and at room temperature for 3 hours and allowed to stand at room temperature overnight. The precipitate is filtered off with suction and the filtrate is concentrated under high vacuum. The residue is partitioned between ethyl acetate and NaHCOs solution. The organic phase is then washed with NaHCOa solution and H20/NaCl, dried using Na2S04 and concentrated. The residue is triturated with diethyl ether. Yield: 7.05 g (88.2%). 2.3.2 Benzyloxycarbonyl-glycine-(3-propanol tert-butyl ester)amide (C2) 7 g (26.28 mmol) of benzyloxycarbonyl-glycine-(3-propanol)amide (C1) are dissolved in 60 ml of dioxane. At low temperature (liquid CO2), 6 ml of H2SO4 are added slowly. Subsequently, 60 ml of condensed isobutylene are added. The mixture is shaken in an autoclave at room temperature and a nitrogen pressure of approximately 20 bar for 3 days. The mixture is then admixed with diethyl ether and extracted three times with 2N NaaCOa solution. The aqueous solution is washed with diethyl ether. The organic phases are combined, washed with water, dried with Na2S04 and concentrated. Yield: 7.98 g (94.2%). 2.3.3 Glycine-(3-propanol tert-butyl ester)amide hydrochloride (C3) 7.98 g (24.75 mmol) of benzyloxycarbonyl-glycine-(3-propanol tert-butyl ester)amide (C2) are dissolved in 80 ml of MeOH, admixed with Pd/carbon and hydrogenated on an autotitrator using methanolic HCI and H2. The catalyst is subsequently filtered off with suction and the filtrate is concentrated. The residue is dried under high vacuum. Yield: 4.7 g (84.5%). 2.3.4 Benzyloxycarbonyl-L-valine-glycine-(3-propanol tert-butyl ester)amide (C4) 5.13 g (20.43 mmol) of benzyloxycarbonyl-Val-OH, 4.59 g (20.43 mmol) of glycine-(3-propanol tert-butyl ester)amide hydrochloride (C3) and 2.75 g of HOBt are dissolved in 60 ml of DMF. At 0°C, 2.65 ml of N-ethylmorpholine and 4.5 g of DCC are added. The mixture is stirred at 0°C for 1 hour and then at room temperature for 2 hours. The mixture is allowed to stand at room temperature overnight and then concentrated under high vacuum. The residue is partitioned between glacial acetic acid and NaHCOa solution. The glacial acetic acid phase is then washed with NaHCOa solution, KHSO4 solution and H20/NaCI, dried using Na2S04 and concentrated. The solid residue is triturated with diethyl ether and filtered off with suction. Yield: 7.32 g (85%). 2.3.5 L-Valine-glycine-(3-propanol tert-butyl ester)amide hydrochloride (C5) 7.29 g (17.3 mmol) of ben2yloxycarbonyl-L-valine-glycine-(3-propanol tert-butyl ester)amide (C4) are dissolved in 90 ml of MeOH, admixed with Pd/carbon and hydrogenated on an autotitrator using methanolic HCI. The catalyst is subsequently filtered off with suction and the filtrate is concentrated. The residue (amorphous) is dried under high vacuum, triturated with diethyl ether and filtered off with suction. Yield: 5.22 g (93.2%). 2.3.6 Benzyloxycarbonyl-L-serine(tert-butylester)-L-valine-glycine-(3-propanol tert-butyl ester)amide (C6) 5.46 g (18.5 mmol) of Z-Ser(But)OH, 6 g (18.5 mmol) of L-valine-glycine-(3-propanol tert-butyl ester)amide hydrochloride (C5) and 2.5 g of HOBt are dissolved in 60 ml of DMF. At 0°C, 2.4 ml of N-ethylmorpholine and 4.07 g of DCC are added. The mixture is stirred at 0°C for 1 hour and at room temperature for 3 hours. The mixture is allowed to stand at room temperature overnight and then concentrated under high vacuum. The solid residue is partitioned between glacial acetic acid and NaHCOs solution. The glacial acetic acid phase is washed with NaHCOa solution, KHSO4 solution and H20/NaCI, dried using Na2S04 and concentrated. The residue is triturated with diethyl ether and filtered off with suction. Yield: 9.74 g (93,2%). 2.3.7 L-Serine(tert-butyl ester)-L-valine-glycine-(3-propanol tert-butyl ester) amide hydrochloride (C7) 9.74 g (17.25 mmol) of benzyloxycarbonyl-L-serine(tert-butyl ester)-L-valine-glycine-(3-propanol tert-butyl ester)amicle (C6) are dissolved in approximately 100 ml of MeOH, admixed with Pd/carbon and hydrogenated on an autotitrator using methanoiic HCI. The catalyst is subsequently filtered off with suction and the filtrate is concentrated. The residue (amorphous) is dried under high vacuum and subsequently triturated with diethyl ether and filtered off with suction. Yield: 8.02 g (99.6%). 2.3.8 Benzyloxycarbonyl-L-aspara9ine-L-serine(tert-butyl ester)-L-valine- glycine-(3-propanol tert-butyl ester)amide (C8) 4.53 g (17 mmol) of Z-Asn-OH, 7.94 g of L-serine(tert-butyl ester)-L-valine-glycine-(3-propanol tert-butyl ester)amide hydrochloride (C7) and 2.3 g of HOBt are dissolved in 60 ml of DMF. At 0°C, 2.21 ml of N-ethylmorpholine and 3.74 g of DCC are added. The mixture is stirred at 0°C for 1 hour and at room temperature for 3 hours and then concentrated under high vacuum. The residue is partitioned between pentanol and NaHCOa solution. The pentanol phase is washed with NaHCOs solution, KHSO4 solution and H20/NaCI, dried over Na2S04 and filtered off with suction, and the filtrate is concentrated under high vacuum. The residue is triturated with diethyl ether, cooled and filtered off with suction. The product is dried in a desiccator over P2O5. Yield: 10.8 g (93.6%). 2.3.9 L-Asparagine-L-serine(tert-butyl ester)-L-varme-glycine-(3-propanol tert-butyl ester)amide hydrochloride (C9) 10.8 g (15.9 mmol) of benzyloxycarbonyl-L-asparagine-L-serine(tert-butyl ester)-L-valine-glycine-(3-propanol tert-butyl ester)amide (C8) are dissolved in approximately 160 ml of warm MeOH, admixed with Pd/carbon and hydrogenated on an autotitrator using methanoiic HCI. The catalyst is subsequently filtered off with suction and the filtrate is concentrated. The amorphous residue is dried under high vacuum, triturated with diethyl ether, cooled and filtered off with suction. Yield: 8.96 g (97%). 2.3.10 Benzyloxycarbonyl-L-2-naphthylalanine-L-asparagine-L-serine(tert- butyl ester)-L-valine-glycine-(3-propanol tert-butyl ester)amide (C10) 5.24 g (15 mmol) of benzyloxycarbony!-2-Nal-OH, 8.72 g (15 mmol) of L-asparagine-L-serine(tert-butyl ester)-L-valine-glycine-(3-propanol tert-butyl ester)amide hydrochloride (C9) and 2.04 g of HOBt are dissolved in 60 ml of DMF. At 0°C, 1.95 ml of N-ethylmorpholine and 3.3 g of DCC are added. The mixture is stirred at 0°C for 1 hour and at room temperature for 3 hours. The mixture is then allowed to stand at room temperature overnight, diluted with DMF and heated slightly. The precipitate is subsequently filtered off with suction and the filtrate is concentrated under high vacuum. The residue is triturated with NaHCOa solution and filtered off with suction and is then triturated with KHSO4 solution, filtered off with suction, triturated with H2O, filtered off with suction and washed with H2O and dried in a desiccator over P2O5. Yield: 13.25 g (>99%). 2.3.11 L-2-Naphthylalanine-L-asparagine-L-serine(tert-butyl ester)-L-valine- glycine-(3-propanol tert-butyl ester)amide hydrochloride (C11) 8.85 g (10.1 mmol) of ben2yloxycarbonyl-L-2-naphthylalanine-L-asparagine-L-serine(tert-butyl ester)-L-valine-glycine-(3-propanol tert-butyl ester)amide (CIO) are partly dissolved in 270 ml of MeOH, admixed with Pd/carbon and hydrogenated on an autotitrator using methanolic HCI. The suspension is diluted with DMF. After approximately 6 hours, the mixture is concentrated to half its original volume. All the material dissolves. The mixture is allowed to stand at room temperature overnight. The catalyst is subsequently filtered off with suction and the filtrate is diluted with the same amount of MeOH, admixed with new catalysts (Pd/carbon) and hydrogenated further on the autotitrator. After 7 hours, the mixture is allowed to stand at room temperature overnight. The mixture is subsequently hydrogenated for another 4 hours, the catalyst is filtered off with suction and the filtrate is concentrated. The residue (amorphous) is dried under high vacuum and subsequently triturated with diethyl ether and filtered off with suction. Yield: 7.56 g (96.2%). 2.3.12 N-tert-Butyl-succinyl-L-2-naphthylalanine-L-asparagine-L-serine- L-valine-glycine-(3-propanol)amide (CI2) 523 mg (3 mmol) of L-2-naphthylalanine-L-asparagine-L-serine(tert-butyl ester)-L-valine-glycine-(3-propanol tert-butyl ester)amide hydrochloride (C11), 2.33 g of mono-tert-butyl succinate ( B4) and 405 mg of HOBt are dissolved in 20 ml of DMF. At 0°C, 0.39 ml of N-ethylmorpholine and 660 mg of DCC are added. The mixture is stirred at 0°C for 1 hour, at room temperature for 2 hours and then allowed to stand at room temperature overnight. The mixture is concentrated under high vacuum and the solid residue is triturated with NaHCOa solution and filtered off with suction. The product is subsequently triturated with KHSO4 solution and filtered off with suction, washed with H2O and dried in a desiccator over P2O5. Yield: 3.04 g (crude product). 2.3.13 N-Succinyl-L-2-naphthylalanine-L-asparagine-L-serine-L-valine-glycine- (3-propanol)amide (24) 3 g (crude product) of /\/-tert-butyl-succinyl-L-2-naphthylalanine-L-asparagine-L- serine-L-valine-glycine-(3-propanol)amide (C12) are dissolved in 30 ml of 90% strength trifluoroacetic acid and allowed to stand at room temperature for 1 hour. The mixture is subsequently concentrated and the residue is triturated with diethyl ether and filtered off with suction. This gives 2.6 g of crude product. For purification, 250 mg of crude product are dissolved in warm glacial acetic acid and chromatographed over Sephadex LH20 using a butanol/glacial acetic acid/water mixture. Yield: 103 mg m/z: 730.341246 (M+H)' (high resolution mass spectrum). 3. Inhibition of laminin/nidogen interaction and biological activity Unless expressly stated, the chemicals used were purchased from Merck (Darmstadt), Sigma (Munich) or Riedel de Haen (Seeize). The isolation of laminin P1 from human placenta, human nidogen from transfected HEK-293 cells and mouse laminin y1 III 3-5 from HEK-293 cells is described in WO 98/31709. Example 3.1 Inhibition assays - inhibition of laminin/nidogen binding with the peptide derivatives found 3.1.1. HTS screening assay (highly sensitive assay variant): Time-Resolved Fluorescence Assay Coating of test tubes Microtiter plates (for example FluoroNunc®) were coated with 75 pi of a 0.1 pg/ml solution of laminin PI (in 0.159 g of NaaCOs, 0.293 g of NaHCOs, 0.02 g of NaNs/liter, pH 9.2) at room temperature for 1 hour. The solution was then tipped off, and free binding sites were blocked by incubation with 0.5% BSA (in 7.9 g of NaCI, 1.2 g of Na2HP04, 0.31 g of KCI, 0.23 g of NaH2P04, 0.04% Tween 20/liter, pH 7.2) at room temperature for 0.5 hour. Completion of the blocking reaction was followed by decantation of the solution and washing once with-250 pi of washing buffer (PBS/0.04% Tween). Sequential inhibition In parallel with the coating, a preincubation of 85-100 pi of a 0.25 nM nidogen solution (recombinantly produced human nidogen) with inhibitor or standard was carried out in a separate reaction vessel (1 hour at room temperature in 7.9 g of NaCI, 1.2 g of Na2HP04, 0.31 g of KCI, 0.23 g of NaH2P04, 0.04% Tween 20/liter, 0.5% BSA, pH 7.2). 75 |jl of the preincubation (nidogen + inhibitor or standard) were transferred into the coated wells of the microtiter plate and incubated at room temperature for 1 hour. This was followed by washing twice with PBS/0.04% Tween. Detection of the bound nidogen took place by incubation (at room temperature) for 1 hour with 75 pi of a specific antibody preparation obtained from yolks of eggs from a chicken immunized with human nidogen. The IgY fraction was used in a dilution of 1:500 in PBS/0.04% Tween. The complex of nidogen and specifically bound antibodies was, after washing twice with PBS/0.04% Tween, detected by adding anti-chicken IgY-biotin (75 pi of a 1:2500 dilution; Promega, Madison, Wl 53711, 608-274-4330). An incubation time of 1 hour and washing twice with PBS/0.04% Tween were followed for this purpose by incubation with streptavidin-europium (Wallac; 1 hour at room temperature) and washing twice with PBS/0.04% Tween. It was finally possible, after adding 100 |jl of enhancement solution (Wallac) and shaking for 5 minutes, to measure a fluorescence signal in a Victor multilabel counter using the europium protocol. The relation between the amount of bound nidogen in the solutions with inhibitor and that of nidogen without added inhibitor was found. 3.1.2. Three-day equilibrium assay Selected inhibitors were investigated for inhibitory activity in this assay variant. The assay is described in US patent number US 5,493,008. The following table compares IC50 values of selected substances with the results of the HTS screening assay. It is clear that the 3-day assay gives slightly lower measured values and, as expected, is more sensitive than the screening assay. However, It is also clear from the comparison that inhibitory structures can be identified reliably with the screening assay developed by us. Example 3.2 (hypothetical) Testing the biological activity of the peptide derivatives Several models which are described in detail in the literature can be used to test the biological activity of the peptide derivatives. Some representative ones are mentioned below: Formation of tubuli in cultures of embryonic kidneys. Grobstein, C; (1956) Exp. Cell Res. 10: 424-440. Ekblom, P. et al. (1994) Development 120: 2003-2014 Branching morphology in embryonic lungs. Ekblom, P. et al. (1994) Development 120: 2003-2014 Branching morphology in embryonic salivary glands. Grobstein, 0. (1953) J. Exp. Zool.124: 383-413 Kadoya, Y. et al. (1997) Development 124: 683-691 Basement membrane assembly in a organotypic skin culture. Smola, H.; Stark, H.-J.; Thiek6tter, G.; Mirancea, N.; Krieg, T.; Fusenig, N.E. (1998) Exp. Cell Res. 239: 399-410 Reconstitution of hydra from disintegrated cells. Yang, Y.G.; Mayura, K.; Spainhour, C.B.; Edwards Jr., J.F.; Phillips, T.D. (1993) Toxicology 85: 179-198 Thickening of basement mennbranes in hydra after culturing at increased glucose concentration. Zhang, X.; Huff, J.K,; Hudson, B.G.; Sarras Jr.; M.P. (1990) Diabetologia 33: 704- 707 All types of quantitative angiogenesis assays summarized in a review article by Jain, R.K. et al. in Nature Medicine (1997) Vol. 3, No. 11, for example: Induction of Haemangiomes in mice by implantation of cells from spontaneous hemangioendotheliomes. O'Reilly, M.S.; Brem, M.S.; Folkman, J. (1995) J. Pediatr. Surg. 30:2; 325-329 Growth of micro-vessels in a serum-free culture of rat aorta. Nicosia. R.F.; Ottinetti, A. (1990) Lab. Invest Vol.63, No. 1, 115-122 Formation of capillaries of endothelic cells on micro-carriers after imbedding into a fibrin gel. Nehls, v.; Drenckhahn, D. (1995) Microvascular Research 50: 311-322. WE CLAIM: 1. A compound of formula I Rl is a group of one of the following formulae R4 means -A, -NH2, -NHR, -NR2, A2, -NHRl, Y means O, S, -N(A)-CO- or -(CH2)r-, D means (CH2)r, O, S, NH, NR, (CH2)r-0, (CH2)r-S, (CH2)rNH or (CH2)rNR and R2 means -A, -E-OH, -E-COOH or -E-CONH2, wherein E means a linear or branched C1-C10-alkyI chain, which is unsubstituted or substituted by -A, -(CH2)m-0H, -(CH2)m- COOH, -(CH2)ni-C(0)NA2 or by a C5-C10-cycloalkyl group, or E means C5-C10-cycloalkyl, which is unsubstituted or substituted by -A, -(CH2)n,-OH, -(CH2)-C00H, -(CH2)m-C(0)NA2 or by a C5-C10-cycloalkyI group, and wherein R7 means a linear or branched C1-C10-alkyl group, which is unsubstituted or substituted by -A, -(CH2)n,-OH, -(CH2)n,- COOH, -(CH2)ni-C(0)NA2 or by a C5-C10-cycloalkyl group, or R7 means a C5-C10-cycloalkyl group, which is unsubstituted or substituted by -A, -(CH2)m-0H, -(CH2)ni-COOH, -(CH2)m- C(0)NA2 or by a C5-C10-cycloalkyl group, andR means C5-C10-cycloalkyl, Het or Ar which are optionally substituted by -C1-C6-alkyl-Het, -C, -C6-alkyl-Ar, -O-C,-Ce-alkyl-Het, -O-C1-Ce-alkyl-Ar, Het or by Ar, wherein Het means a monocyclic or bicyclic, 5- up to 10-membered aromatic or non-aromatic ring containing 1 or 2 equal or different hetero-atoms as members of said ring, selected from the group consisting of nitrogen, oxygen and sulfur, which is unsubstituted or substituted by one or more hydroxy or carboxy groups, and wherein Ar means a monocyclic or bicyclic 5- up to 10-membered aromatic ring which is unsubstituted or substituted by one or more hydroxy or carboxy groups, and Z means (CH2)m, O, S, NH, NR, N-C(0)-R or NSO2R, A means 11 or C1-C4-alkyl and 1, m and r are integers from 0 to 3, n and k are integers from 1 to 2, p is an integer from 0 to 1 and q is an integer from 1 to 3, in all its stereoisomeric forms and mixtures thereof in all ratios, including their physiologically tolerable salts. 2. The compound of formula I as claimed in claim 1, wherein n is 1. 3. The compound of formula I as claimed in claim 1 or 2, wherein R in group X means Het. 9. The compound of formula I as claimed in claim 1 or 2, wherein R in group X means Ar which is optionally substituted by -C1-C6-alkyl-Ar, -O-C1-C6-alkyl- Ar or by Ar. 10. The compound of formula I as claimed in claim 9, wherein R in group X means Ar. 13. The compound of formula I as claimed in claim 10, wherein Ar means 14. The compound of formula I as claimed in claim 10, wherein Ar means 15. The compound of formula I as claimed in claim 9, wherein R in group X means 16. The compound of formula I as claimed in claim 9, wherein R in group X means 17. The compound of formula I as claimed in one or more of claims 1 to 16 wherein X is a group of the following formula 18. The compound of formula I as claimed in claim 17, wherein Y means -(CH2)r-. 19. The compound of formula I as claimed in claim 18, wherein r is 1. 20. The compound of formula I as claimed in claim 18, wherein r is 0. 21. The compound of formula I as claimed in claims 17 to 20, wherein k is 2. 22. The compound of formula I as claimed in claims 17 to 20, wherein k is 1. 23. The compound of formula I as claimed in one or more of claims 1 to 16 wherein X is a group of the following formula 24. The compound of formula I as claimed in claim 23, wherein D means -(CH2)- 25. The compound of formula I as claimed in claim 23, wherein r is 0. 26. The compound of formula I as claimed in claim 23, wherein r is 1. 27. The compound of formula I as claimed in one or more of claims 1 to 26 wherein Rl is a group of the following formula 28. The compound of formula I as claimed in claim 27 wherein Z means (CH2)m. 29. The compound of formula I as claimed in claim 28, wherein m is 0. 30. The compound of formula I as claimed in claim 28, wherein m is 1. 31. The compound of formula I as claimed in one or more of claims 27 to 30 wherein R5 means -(CH2)i-C00A. 32. The compound of formula I as claimed in claim 31, wherein A means H. 33. The compound of formula I as claimed in one or more of claims 27 to 30 wherein R5 means -(CH2)|-COONH2. 34. The compound of formula I as claimed in one or more of claims 30 to 33 wherein 1 is 0. 35. The compound of formula I as claimed in one or more of claims 27 to 34 wherein R4 means -NH2. 36. The compound of formula I as claimed in one or more of claims 27 to 34 wherein R4 means -A. 37. The compound of formula I as claimed in claim 36 wherein A means H. 38. The compound of formula I as claimed in one or more of claims 27 to 34 wherein R4 means -NHRl. 39. The compound of formula I as claimed in claim 38 wherein -NHRl means 40. The compound of formula I as claimed in claim 39 wherein R5 41. The compound of formula I as claimed in claim 39 wherein R5 means 42. The compound of formula I as claimed in claim 39 wherein R5 means -NH2. 43. The compound of formula I as claimed in one or more of claims 1 to 26 wherein Rl is a group of the following formula 44. The compound of formula I as claimed in claim 43 wherein Z means -(CH2)m-. 45. The compound of formula I as claimed in claim 44, wherein m is 1. 46. The compound of formula I as claimed in one or more of claims 43 to 45 wherein R4 means -NH2. 47. The compound of formula I as claimed in one or more of claims 43 to 46 wherein R5 means -(CH2)rCOOA. 48. The compound of formula I as claimed in claim 47 wherein I is 0. 49. The compound of formula I as claimed in claims 47 or 48 wherein A means H. 50. The compound of formula I as claimed in one or more of claims 1 to 26 wherein Rl is a group of the following formula 51. The compound of formula I as claimed in claim 50 wherein R5 means -(CHa)!-COOA. 52. The compound of formula I as claimed in claim 51 wherein I is 0 and A means H. 53. The compound of formula I as claimed in one or more of claims 1 to 52 wherein R2 means A. 54. The compound of formula I as claimed in claim 53 wherein R2 means -CH3. 55. The compound of formula I as claimed in one or more of claims 1 to 52 wherein R2 means -E-COOH. 56. The compound of formula I as claimed in claim 55, wherein R2 means -CH2-COOH. 57. The compound of formula I as claimed in one or more of claims 1 to 52 wherein R2 means -E-OH. 58. The compound of formula I as claimed in claim 57 wherein R2 means -CH2-OH. 59. The compound of formula I as claimed in claim 1, wherein R7 is a branched C1-C10-alkyl group. 60. The compound of formula I as claimed in claim 1, wherein R7 means -CH(CH3)2. 61. The compound of formula I as claimed in claim 1, wherein R7 means -C(CH3)3. 62. The compound of formula I as claimed in claim 1, wherein R7 means -CH(CH3)CH2-CH3. 63. The compound of formula I as clamed in claim 1, wherein R7 means -CH2-CH(CH3)2. 64. The compound of formula I as claimed in one of the claims 59 to 63 wherein q is 2. 65. A pharmaceutical composition containing at least one compound as claimed in one or more of the preceding claims and/or its physiologically tolerable salts. 66. The compound as claimed in one or more of claims 1 to 64 and/or its physiologically tolerable salts as a pharmaceutical. |
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in-pct-2001-1142-che abstract-duplicate.pdf
in-pct-2001-1142-che abstract.pdf
in-pct-2001-1142-che claims-duplicate.pdf
in-pct-2001-1142-che claims.pdf
in-pct-2001-1142-che correspondence-others.pdf
in-pct-2001-1142-che correspondence-po.pdf
in-pct-2001-1142-che description (complete)-duplicate.pdf
in-pct-2001-1142-che description (complete).pdf
in-pct-2001-1142-che drawings.pdf
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in-pct-2001-1142-che form-13.pdf
in-pct-2001-1142-che form-19.pdf
in-pct-2001-1142-che form-26.pdf
in-pct-2001-1142-che form-3.pdf
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in-pct-2001-1142-che others.pdf
in-pct-2001-1142-che petition.pdf
Patent Number | 223545 | ||||||||||||||||||
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Indian Patent Application Number | IN/PCT/2001/1142/CHE | ||||||||||||||||||
PG Journal Number | 47/2008 | ||||||||||||||||||
Publication Date | 21-Nov-2008 | ||||||||||||||||||
Grant Date | 12-Sep-2008 | ||||||||||||||||||
Date of Filing | 13-Aug-2001 | ||||||||||||||||||
Name of Patentee | SANOFI-AVENTIS DEUTSCHLAND GMBH | ||||||||||||||||||
Applicant Address | BRUNINGSTRASSE 50, D-65929 FRANKFURT AM MAIN, | ||||||||||||||||||
Inventors:
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PCT International Classification Number | A61K38/06 | ||||||||||||||||||
PCT International Application Number | PCT/EP00/01386 | ||||||||||||||||||
PCT International Filing date | 2000-02-19 | ||||||||||||||||||
PCT Conventions:
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