Abstract:
Cyclohexapeptides of formula (I): 
     
       
                 
         
             
             
         
       
       
         
           
             as defined herein. The cyclohexapeptides are non-selective functional analogs of somatostatin.

Description:
This application is the U.S. national phase of International Application No. PCT/EP2008/066081 filed 24 Nov. 2008 which designated the U.S. and claims priority to Italian Application No. MI2007A002266 filed 3 Dec. 2007, and European Application No. 07425778.3 filed 7 Dec. 2007, the entire contents of each of which are hereby incorporated by reference. 
     The present invention relates to new non-selective functional analogue cyclopeptides of somatostatin, to their conjugates and complexes, to processes for the production, to the formulations which contain them and to their uses in the pharmaceutical field. 
     STATE OF THE ART 
     Cyclic peptide agonists of somatostatin have been known for some time [J Pept Res 58 (2), 91 (2001)]: in particular, two of these, octreotide and lanreotide, are clinically used for the care of acromegaly and for the symptomatic treatment of carcinomas. 
     Somatostatin acts through the interaction with 5 receptor subtypes (SSTR1, 2, 3, 4 and 5); but the analogues up to now employed in therapy are nevertheless essentially selective for the single receptor SSTR2. 
     The great majority of the already known agonists is characterised by the presence, in the peptide structure, of the fragment -DTrp-Lys-; this fragment therefore appears to be essential for the activity of the analogues and is in fact also present in octreotide and lanreotide. 
     Recently, the hypothesis has been advanced that less-selective analogues, i.e. capable of interacting also with the other receptor subtypes, can offer an advantage from the standpoint of therapeutic use [Nature Rev. Drug Discovery 2, 999 (2003)]. 
     In the patent application WO2002010192, a cyclopeptide is described which has a strong affinity for the receptor SSTR5, a lower affinity for SSTR2 and SSTR3 and a nearly zero affinity for SSTR4. For SSTR1, an affinity is described about 60 times less than that for SSTR5. 
     The same inventors of WO2002010192, in a subsequent publication [Nature Rev. Drug Discovery 2, 999 (2003)], sustain the importance of the receptors SSTR1, 2 and 5 for the antisecretory activity of somatostatin, but report, for the same cyclopeptide described in the aforesaid patent application, an affinity for SSTR1 of about 300 less than that for SSTR5. 
     It is clear that, in this case, a possible therapeutic activity mediated by the interaction with the receptor SSTR1 can only be achieved in the presence of a considerable overdosage with respect to the actions mediated by the interaction with SSTR5. 
     Therefore, while the possible therapeutic role of agonists for the receptor SSTR4 is not clear, there is clearly the need, and the possible use, for new somatostatin analogues with an affinity level comparable for all of the other four receptors. 
     In particular, the potential therapeutic advantages of agonists capable of interacting with SSTR1 are reported in the literature: M. C. Zatelli and colleagues have studied, in vitro, the effect of agonists for SSTR1 on human pituitary adenomas, both secreting [J Clin End&amp;Met 88, 2797 (2003)] and clinically non-functional [J Clin End&amp;Met 89, 5181 (2004)]; in both cases the stimulus of SSTR1 receptors lead to a reduction of the secretory activity and cell vitality. On the other hand, the potential therapeutic advantage that can derive from the use of pluripotent analogues of somatostatin (capable of interacting with the receptors SSTR 1, 2, 3 and 5) was also shown by J. van der Hoek and colleagues in a recent review [Curr. Pharm. Design 11, 1573 (2005)]; it was in fact shown how different tumours, both pituitary and gastroenteropancreatic (GEP), express, on the cell surface, variable but significant percentages of all four receptors, while the receptor SSTR4 is much less present. 
     The application WO2005014624 describes the preparation of cyclic analogues of somatostatin and the intermediates used in their preparation. These hexacyclic analogues have the tryptophan residue in position 3. 
     The application WO2006066868 describes pharmaceutical compositions for the parenteral administration of several salts of somatostatin analogues, which form a deposit gel after the injection in contact with the body fluids. By somatostatin analogues, it is intended the linear or cyclic peptides derived from somatostatin, which comprise a sequence of amino acids comprising tryptophan. 
     In  Regulatory Peptides,  1 (1980) 97-113, the importance of the indole NH group is sustained for the somatostatin activity: the substitution of Trp 8  with naphthylalanine in fact causes the loss of activity. 
     The binding data is not reported in the article, while the inhibition activity of the in vivo gastric secretion is evaluated. The results indicate that, for the gastric activity, the substitution of Trp 8  with halogen, methylated or methoxylated analogues (table II) has little influence on the biological potency, potency which is instead nearly cancelled in the analogues containing pentamethyl-phenylalanine (Pmp) or naphthylalanine (table III), rather than tryptophan. The deriving halogen compounds of D-Trp instead seem to considerably improve the inhibition activity of the GH secretion (table V). Merck S&amp;D researchers (see Veber D. F. in  Proceedings of the  12 th Am. Pep. Symp .; Smith, J. A. &amp; Rivier J. E. editors, ESCOM 1992, pp 3-14) report that, in cyclic hexapeptides, the substitution of the tryptophan with other aromatic amino acids leads to a considerable loss of in vitro activity in the inhibition of the GH secretion. 
     In  J Med Chem  (2005) 48, 507, selective analogues for SSTR1 are described along with their possible therapeutic role of agonists. The structures analysed here also have tryptophan. 
     The article describes two series of analogues derived from two cyclopeptides: one containing D-Trp and the other D-Nal; all the analogues, like the parents, only have affinity for SSTR1; the series with D-Nal is about 10 times less powerful than that with D-Trp. One particular detail of these peptides, which are inactive on all other receptor subtypes, is the substitution of the lysine with p-amine-phenylalanine. 
     From that set forth above, it is therefore evident that a pluripotent agonist of somatostatin, i.e. capable of stimulating SST1, SSTR2, SSTR3 and SSTR5, will increase the possibility of positive responses in patients affected by neuroendocrine tumours with respect to agonists whose activator function is restricted to a lower number of sub-receptors of the somatostatin. 
    
    
     DESCRIPTION OF THE INVENTION 
     The applicant has surprisingly found that the tryptophan residue, present in many known analogues, can be usefully substituted with other suitable aromatic residues, maintaining the affinity for most of the somatostatin receptors. 
     In particular, it was found that, by using amino acids whose aromatic group is sufficiently rich with electrons (being, for example, substituted with electron-donor groups) in substitution of the tryptophan residue, peptides are obtained which show a good affinity for the SSTR1 receptor, at concentration values similar to those necessary for the bond to the SSTR2, SSTR3 and SSTR5 receptors. 
     Forming the object of the present invention are therefore somatostatin analogue cyclohexapeptides, having formula (I), where by somatostatin analogue cyclohexapeptides it is intended peptides with six alpha-amino acid residues, in which a direct peptide bond is present between the alpha-carboxyl group of the sixth residue and the alpha-amine group of the first residue, with bond affinity at nanomolar concentrations, for at least one of the known somatostatin receptors: 
                                
where:
 
     m=0, 1 or 2 and n=1, 2 or 3; preferably m is equal to 1 and n is equal to 1 or 2; still more preferably n is equal to 1. 
     R1 represents an aromatic group, excluding indole, which is preferably phenyl, naphthyl, benzhydryl, fluorenyl, styrenyl, anthranyl or biphenyl, optionally substituted in one or more positions. The preferred substitution groups are those electron-donors such as alkyl, alkyloxyl, hydroxyl, alkylamine, acylamine, sulphide or alkylsulphide. 
     The group R1 is preferably naphthalene group, substituted with or more methyloxy groups, preferably with two methyloxy groups; in a still more preferred aspect of the invention, R1 is 3,8-dimethoxy-naphthalene-2-yl. 
     R4 represents an aromatic group, optionally substituted. The R4 group is preferably a phenyl group, possibly substituted with a hydroxyl group, C 1 -C 4  alkoxyl, C 1 -C 4  alkyl, halogen or nitro. 
     R2 and R3 are, independently, H or a C 1 -C 4  alkyl group, or, together, they represent a C 4 -C 5  alkylene chain, bonded to the nitrogen atom to form a cyclic structure. 
     Alternatively, R3 can be a cation or metal chelating group, directly joined to the amine group or joined through a spacer. 
     The possible spacer can be one of those already known in the art, for example those described in GB-A-2,225,579 or in WO9701579, incorporated here by reference; they can, for example be a group of formula —Z—R5-CO—, where R5 is C 1-11  alkylene, C 1-11  alkenylene or —CH(R6)-, where R6 is the side chain of an alpha amino acid, and Z is a function capable of forming a covalent bond with the chelating group; Z can for example be a functional group capable of forming an ether, ester or amidic bond with another functional group of the chelating group (for example hydroxyl, carboxyl or amine) Z preferably is an oxygen atom, a sulphur atom, a carbonyl radical (or CO) or an amino radical (or NH). 
     The group Z is still more preferably an amino radical and the group of formula —Z—R5-CO— will be a bivalent residue deriving from a carboxylic-amino acid, such as, for example, beta-Alanine (or —NH—(CH 2 ) 2 —CO—), 6-amino hexanoic acid (or —NH—(CH 2 ) 5 —CO—) or others. 
     The chelating group is a physiologically acceptable group, capable of complexing ions or other detectable or useful elements for anti-tumour radiotherapy and preferably has a hydrophilic character. 
     The chelating groups and the ions and other complexing elements can be usefully chosen from among those already known and described, for example, by Okarvi S. M. in Med. Res. Rev. 24 (3), 357 (2004), by Weiner R. E. and Thakur M. L. BioDrugs 19(3), 145 (2005) or in WO2002010192, incorporated here by reference. 
     The chelating group can be in free form, salified or complexed with ions or other elements, detectable by radioactivity (radionuclides) or with other means, or usable for radio-therapeutic aims. 
     Preferably, the chelating group will be derived from 1,4,7,10-tetraazacyclododecane-N,N′,N″,N′″-tetraacetic acid (DOTA) or diethylenetriaminepentaacetic acid (DTPA) and the ion will be a paramagnetic ion (Gd3+, Fe3+, or others), fluorescent (Eu3+) or a radionuclide emitting α, β or γ radiations (111In, 99mTc, 169Yb, 177Lu, 90Y, 213Bi or others). 
     X1 is an aminoacyl residue of formula (a), (b) or (c) 
     
       
                 
         
             
             
         
      
     
     X1 is preferably an aminoacyl residue of formula (c). 
     The aminoacyl residues, present in the cyclohexapeptides of formula (I), can have configuration L or D; preferably the residues 1, 2, and 4-6 are L, and the residue 3 is preferably D. 
     The cyclohexapeptides of formula (I) can exist in free base form or as salts. The salts include addition salts with organic acids (for example acetates, lactates, benzoates, aspartates, pamoates, etc.), polymer acids (for example polymethacrylic acid, polystyrenesulfonic acid, etc.) or inorganic acids (for example hydrochlorides, sulphates, nitrates, etc.). 
     The compounds of the invention are, in vivo, much more resistant to the degradation mechanisms in comparison with the analogue cyclodisulphides of somatostatin (octreotide, lanreotide, etc.) and consequently have a longer action duration. In some cases, the stability and action duration are also improved with respect to other cyclopeptides, including those already known for being stable somatostatin agonists. 
     The present invention also includes the processes for the production of compounds of formula (I), from here on called compounds of the invention. 
     The compounds of the invention can be produced by using different synthetic methods, analogous to methods already known for other peptides. 
     a) A corresponding linear hexapeptide, partially protected, can be produced by means of solid phase synthesis, so as to leave both the N-terminal alpha-amino group and the C-terminal alpha-carboxylic group free; the two free groups will the be made to react, in solution, by means of appropriate condensing agents and the protections of the side chains will finally be removed, obtaining the desired cyclohexapeptide.
 
b) Alternatively, the solid phase synthesis can be conducted by anchoring the peptide to the resin by means of the lysine side chain; in this case, after having selectively removed the protections from the N-terminal and C-terminal groups, the cyclisation can still be conducted in solid phase and the compounds of the invention can be obtained with a single treatment of deprotection and separation from the resin.
 
c) In another alternative, the protected linear peptide can be prepared by means of synthesis in solution and then, after having selectively removed the protections from the N-terminal and C-terminal groups, one can proceed as described in a). The linear peptide to be cyclised can be chosen from among six peptides hypothetically obtainable by means of the opening of any one of the six peptide bonds present in the compounds of the invention. The choice will be guided by considerations of synthetic suitability, known to peptide synthesis experts, but do not minimally influence the nature of the final product, which will in any case be identical whatever the chosen sequence of the linear peptide; preferably, peptides are chosen in which the C-terminal amino acid is lysine.
 
     Many of the amino acid derivatives, necessary for the synthesis of the peptides, are known and commercially available. 
     The hydroxyproline derivates can be prepared as described in WO9701579, incorporated here by reference, or with other similar procedures; alternatively, the partially protected linear peptides can contain a non-modified hydroxyproline residue, and the introduction of the side chain can be carried out directly on the linear peptides, before the deprotection, or after the cyclisation, before the final deprotection. 
     For the chelating derivatives of the compounds of the invention, the protector group of the chain bonded to the hydroxyproline can be appropriately chosen such that it is possible to selectively remove it, leaving the protection of the lysine side chain unaltered; in this manner, it will be possible to bind the chelating group to the free amino group, directly or by means of a spacer, before the final deprotection. 
     Some amino acids used in position 3 of the general formula (I), like their derivatives, are new and form a further aspect of the present invention. In particular, we refer to the amino acids:
     3-(3,8-dimethoxy-naphthalene-2-yl)-alanine,   3-(1,4-dimethoxy-naphthalene-2-yl)-alanine and   2,5-dimethoxy-homophenylalanine
 
and to their totally or partially protected derivatives, corresponding to the formulas (e), (f) and (g):
   

     
       
                 
         
             
             
         
      
     
     In formulas (e), (g) and (f), G can be a hydrogen atom or a protective group chosen from among those known to those skilled in the art, such as fluorene-9-yl-methyloxy-carbonyl, tert-Butyloxy-carbonyl or benzyloxy-carbonyl; W can be a hydroxyl group or a protective group chosen from among those known by those skilled in the art, for example methyloxy, tert-butyloxy or benzyloxy. By partially protected derivatives, it is intended those derivatives where only one, from among G and W, represents a protective group. 
     These can be prepared by adapting methods already known in literature (see for example [J Org Chem 55, 2913 (1990)], [Org. Lett. 2, 1089 (2000) and [Synthesis (1983), 38]); for example, starting from the aldehyde corresponding to the desired side chain, the method described in diagram 1 can be used. 
     
       
                 
         
             
             
         
      
       
                 
         
             
             
         
       
     
     The aforesaid derivatives can be prepared as racemic enantiomer mixtures (D/L) or, by means of stereoselective synthesis or chiral resolution methods, they can be obtained as single enantiomers D or L. 
     Among the chiral resolution methods, enzymatic deracemisation methods can be used (such as, for example, that described in US2001021519, incorporated here by reference), in which the stereoselectivity of the enzyme (for example L or D amino acid-oxidase) allows inducing the racemisation of only one of the two enantiomers, after which repeated treatment cycles permit attaining high enantiomer purity. 
     Also object of the present invention are the pharmaceutical formulations which contain the compounds of the invention. 
     The compounds of the invention can be administered in free form or in the form of pharmaceutically acceptable salts or as complexes. Such salts and complexes can be prepared in a conventional manner and show the same order of activity as the free compounds. The present invention also provides pharmaceutical compounds comprising the compounds of formula (I) in free base form or in pharmaceutically acceptable salt form, together with one or more pharmaceutically acceptable excipients or diluents. Such compositions can be formulated in a conventional manner. The compounds of the invention also can be administered in modified release form, for example as implants, microcapsules, microspheres or nanospheres comprising, for example, biodegradable polymers or copolymers, in liposome formulation form, or in autogel form, for example solid or semisolid compositions capable of forming a gel after interaction with the fluids of the patient body. 
     The compounds of the invention or their pharmaceutically acceptable salts or complexes can be administered by means of any conventional pathway, for example parenterally, in the form of an injectable solution or suspension (also including the above-indicated modified release forms), orally, using a conventional absorption promoter, nasally or as suppositories or topically, for example in the form of an ophthalmic liquid, gel, preparation as unguent or as suspension, for example liposome suspension, as microsphere or nanosphere formulation, for example for subconjunctival or intra or periocular instillation or injection. 
     According to a further aspect of the invention, a pharmaceutical composition is also provided comprising a conjugate or a complex of compounds of the invention together with pharmaceutically acceptable excipients or diluents. Such compositions can be produced in a conventional manner and can be presented, for example for the diagnostic imaging, as a kit comprising two separate doses, one being the radionuclide and the other the conjugate of the compounds of the invention, with instructions for their mixing. For the radiotherapy, the conjugate of the compounds of the invention in complexed form can preferably be in hot liquid formulation form. 
     The following examples intend to illustrate the objects of the present invention and must not in any manner be considered limiting of the same. 
     In the examples, the following abbreviations will be used:
     1,4MNal 3-(1,4-dimethoxy-Naphthalene-2-yl)-Alanine   2,5MhPhe 2,5-dimethoxy-homoPhenylalanine   3,8MNal 3-(3,8-dimethoxy-Naphthalene-2-yl)-Alanine   ACN Acetonitrile   Bn Benzyl   Boc tert-Butyloxy-carbonyl   DIPEA Diisopropylethylamine   DMF N,N-dimethylformamide   DPPA Diphenylphosphorylazide   DSC N,N-Disuccinimidylcarbonate   Fmoc Fluorene-9-yl-methyloxy-carbonyl   Fmoc-OSu Fluorene-9-yl-methyl, N-succinimidyl carbonate   HATU O-(7-Azabenzotriazole-1-yl)-N,N,N′,N′-tetramethyluronium hexafluorophosphate   hPhe homoPhenylalanine; 2-amino-4-phenyl-butyric acid   Hyp 4,Hydroxy-proline   Nal 3-(Naphthalene-2-yl)-Alanine; 2-amino-3-napthalene-2-yl-propionic acid   NMM N-methyl Morpholine   Pd/C Metal palladium on carbon   Phg Phenylglycine; 2-amino-2-phenyl-acetic acid   PVDF Polyvinylidenefluoride   Sty Styryl-Alanine; 2-amino-5-phenyl-pent-4-enoic acid   Tfa Trifluoroacetyl   THF Tetrahydrofurane   -Trt(Cl)-DVB Resin, (2-chloro)Trityl-Divinylbenzene   Z Benzyloxy-carbonyl   

     Except where otherwise indicated, the amino acids are in L configuration; with (D/L) the racemic amino acids are indicated, while with (D,L) the single enantiomers of undefined chirality are indicated. 
     General Purification Method 
     If not otherwise indicated, all of the final purifications were carried out by means of a Waters preparation HPLC/MS system with Waters Symmetry C18 5 mm 19×50 mm columns, equipped with Waters ZQ mass spectrometer. 
     Operating Conditions: 
     ES +  centroid ionisation, 15 min scanning time, 120-1000 m/z scanning, 15V cone voltage, 120° C. source temperature, 250° C. solvation temperature. 
     HPLC Eluents: 
     A=H 2 O, B=ACN, C=1% CF 3 COOH in H 2 O 
     An aliquot of the raw product to be purified was dissolved in MeOH and diluted with an ACN/H 2 O (1:1; v/v) mixture. The solution, filtered on 0.45 mm PVDF membrane, was injected in the previously described preparation system. For every run, the fractions corresponding to the peak associated with the expected molecular ion ([M+H] + ) were collected, combined and concentrated to dryness. If additional peaks were presented associated with the same molecular ion (isomers), these were collected separately. 
     Preparation of the Intermediates 
     Example 1 
     Fmoc-(D/L) 3-(3,8-dimethoxy-Naphthalene-2-yl)-Alanine 
     a) 3,8-dimethoxy-2-naphthaldeide (1 eq), 2,2-dimethyl-1,3-dioxane-4,6-dione (1.35 eq) and piperidine (0.12 eq) are dissolved in CHCl 3  and the solution is heated and refluxed for 2.5 hours. After aqueous washings, the product is recovered by evaporation of the solvent and redissolved in a mixture of THF and methanol, and NaBH 4  (5.4 eq) is added to the solution. After about 10 minutes, water is added and the mixture is acidified to pH=3. By partially evaporating, a solid is separated which is recovered and redissolved in ethanol, pyridine is added and the mixture is reflux heated until the initial product has completely disappeared (TLC control).
 
b) After having evaporated the ethanol, the product (mono-ethyl ester of 2-(3,8-Dimethoxy-naphthalene-2-yl-methyl)-malonic acid) is dissolved in chloroform and washed with acidic water. Thionyl chloride (1.3 eq) is added to the dried solution, and the mixture is reflux heated for about an hour. After repeated evaporations of the chloroform, the residue is dissolved in dichloromethane and the solution is cooled in an ice bath. Tetrabutylammonium bromide (catalytic) is added and NaN 3  (1.2 eq) dissolved in water, and after two hours at 0° C., the organic phase is recovered, which is washed with water and dried with anhydrous Na 2 SO 4 ; the solution is left at room temperature, in the presence of anhydrous Na 2 SO 4 , for an entire night. Trifluoroacetic acid (1.5 eq) is added to the filtered solution, and the mixture is reflux heated for about 6 hours. After having washed with 5% NaHCO 3 , the solvent is evaporated and the oil obtained is purified on a silica gel column.
 
c) The obtained product (Tfa-(D/L)3,8MNal-OEt) is dissolved in a mixture of THF, methanol and water, containing K 2 CO 3  (2 eq) and reflux heated for one night. The solution is partially evaporated and Fmoc-OSu (1 eq) dissolved in THF is added. Upon completed reaction (TLC control), the THF is evaporated and the product recovered by extracting the aqueous solution with ethyl acetate. With the addition of n-hexane, one obtains the precipitation of the product (Fmoc-(D/L)3,8MNal-OH) which is filtered and dried (HPLC purity: 98.5%; m/z=498 amu ([M+H]+)).
 
     Example 2 
     Fmoc-[4-(2-aminoethyl)carbamoyl]Proline 
     a) Z-Hyp-OBn and DSC (1 equivalent) are dissolved in acetonitrile and treated with triethylamine (1.2 eq). After a night at room temperature, N-Boc-diamineethane (1.2 eq) is added and the mixture is left to react for 3.5 hours. After evaporation of the solvent, the residue recovered with ethyl acetate is washed, in order, with 2.5% KHSO 4 , NaHCO 3  and NaCl. The organic solution, dried with anhydrous Na 2 SO 4 , is evaporated to dryness, recovering the product.
 
b) The product is dissolved in methanol and the protector groups (Z and benzyl ester) are removed by means of catalytic hydrogenation in the presence of 10% Pd/C. After filtration of the catalyst, the amino acid is recovered by evaporating the solvent, and is dissolved in a mixture of water and THF containing K 2 CO 3  (1 eq), and after having cooled to 0° C. Fmoc-OSu (2 eq) dissolved in THF is added. Upon completed reaction (TLC control), the THF is evaporated and the product recovered by extracting the aqueous solution with ethyl acetate. With the addition of n-hexane, one obtains the precipitation of the product, which is filtered and dried (HPLC purity: 99.9%; m/z=540 amu ([M+H] + ))
 
     Example 3 
     Fmoc-(D/L) 2,5-dimethoxy-homophenylalanine 
     a) To a suspension of 2,2-dimethyl-1,3-dioxane-4,6-dione (1.3 eq) in DMF (50 mL), cooled in an ice bath, NaCNBH 3  (1.8 eq) and 2.5-dimethoxyphenylacetaldeide (1.1 eq) are added. The reaction mixture is stirred at RT for 5 h. By adding H 2 O, a solid is separated which is filtered, purified by crystallisation from isopropanol and finally dissolved in EtOH and reflux treated with pyridine for six hours.
 
b) Operating as described in point b) of example 1, from the obtained product (mono-ethyl ester of 2-(2,5-Dimethoxy-phenyl-ethyl)-malonic acid), the partially protected amino acid Fmoc-(D/L)2,5 MhPhe-OH is prepared (HPLC purity: 96%; m/z=462 amu ([M+H] + )).
 
     Example 4 
     Fmoc-(D/L) 3-(1,4-dimethoxy-Naphthalene-2-yl)-Alanine 
     Starting from 1,4-dimethoxy-2-naphthaldeide and operating as described in example 1, the protected amino acid Fmoc-(D/L)1,4MNal-OH is obtained. (HPLC purity: 96.9%; m/z([M+H]+)=498 amu). 
     Preparation of the Cyclopeptides 
     The purity of the peptides described in the examples was analysed by means of HPLC reverse-phase chromatography (Agilent 1100 chromatograph), using the following method:
     Eluents: A) 0.1% TFA in acetonitrile/water (5:95; v/v)
       B) 0.1% TFA in acetonitrile   
       Eluent B gradient: from 20% to 80% in 30 min.   Flow: 1.0 ml/min.   Column: Jupiter 4μ (4×250 mm)   

     Example 5 
     cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH 2 )-Phe-(D,L)3,8MNal-Lys]isomer B 
     a) H-Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NHBoc)-Phe-(D/L)3,8MNal-Lys(Boc)-OH 
     Starting from the resin Fmoc-Lys(Boc)-Trt(Cl)-DVB, various cycles of solid phase peptide synthesis are carried out, in order to obtain the desired hexapeptide; in the first cycle, one uses Fmoc-(D/L)3,8Mnal-OH (see ex. 1) and in the third cycle one uses Fmoc-Pro(4-OCONH(CH 2 ) 2 NHBoc)-OH (see ex. 2); for every cycle, the Fmoc group is removed with 20% Piperidine in DMF and the subsequent amino acid, protected like Fmoc, is activated with HATU and made to react with the amino groups present on the resin. 
     At the end, the Fmoc group is removed with 20% Piperidine in DMF and the partially protected peptide is removed from the resin by means of a treatment with a mixture of acetic acid, trifluoroethanol and dichloromethane (in 1:2:7 proportion) for 30 minutes at room temperature. After having evaporated the solvent, the residue is divided between ethyl acetate and 5% NaHCO 3 , the organic phase is recovered and evaporated, obtaining a solid residue. 
     b) cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH)-Phe-(D,L)3,8-MNal-Lys] 
     The peptide obtained in c) is dissolved in (1.6 mM) DMF and cooled to −10° C.; DIPEA (2 eq) and DPPA (1.3 eq) are added and the mixture is left at +4° C. for 60 hours. After having removed DMF, the residue is recovered with ethyl acetate and washed with 5% NAHCO 3 . By evaporating the organic phase, one obtains a solid residue which is treated with TFA (95% in H2O) at 0° C. for 1 hour and then evaporated; different isomer species are present in the residue, which are separated by means of reverse-phase chromatography (column C18). The second isomer, in the order of elution from the HPLC column, (isomer B), is collected pure. 
     HPLC: RT 14.74 min.; 99.1% purity 
     MS: m/z=1133 amu ([M+H] + ) and 567 amu ([M+2H] 2+ ) 
     Example 6 
     cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH 2 )-Phe-(D,L)2,5 MhPhe-Lys] isomer B 
     a) H-Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NHBoc)-Phe-(D/L)2,5-MhPhe-Lys(Boc)-OH 
     One operates as described in point a) of example 5, using Fmoc-(D/L)2,5MhPhe-OH (ex. 3) in the first cycle and Fmoc-Hyp-OH in the third cycle. Before the removal of the terminal Fmoc group, the resin is treated with p-nitrophenylchloroformiate (5 eq) in the presence of NMM (5 eq); after three hours, the resin is washed with DCM and treated with N-Boc-diamineethane (5 eq) for another three hours, and then filtered and washed. One then proceeds as described in point a) of example 5. 
     b) cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH)-Phe-(D,L)2,5-MhPhe-Lys] 
     The peptide obtained in a) is treated as described in point b) of example 5. Also in this case, one obtains different isomers, which are separated by means of reverse-phase chromatography (column C18). The second isomer, in the order of elution from the HPLC column, (isomer B), is collected pure. 
     HPLC: RT 13.82 min.; purity 99.0% 
     MS: m/z=549 amu ([M+211] 2+ ) 
     Example 7 
     cyclo[Tyr(Bn)-Phe-Pro (4-OCONH(CH 2 ) 2 NHCH 3 )-Phe-(D,L)3,8MNal-Lys] isomer B 
     One operates as described in example 6, using Fmoc-(D/L)3,8MNal-OH (ex. 1) in the first cycle and Boc-N(CH 3 )—(CH 2 ) 2 —NH 2 ) to modify the side chain of hydroxyproline. Different isomers are obtained, which are separated by means of reverse-phase chromatography (colonna C18). The second isomer, in the order of elution from the HPLC column, (isomer B), is collected pure. 
     HPLC: RT 15.07 min.; purity 94.5% 
     MS: m/z=1147 amu ([M+H] + ) and 574 amu ([M+2H] 2+   
     Example 8 
     cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH 2 )-Phe-(D,L)1,4-MNal-Lys] isomer A 
     One operates as described in example 6, using Fmoc-(D/L)1,4MNal-OH (ex. 4) in the first cycle. Different isomers are obtained, which are separated by means of reverse-phase chromatography (column C18). The isomer with lower retention time (isomer A) corresponds to the product of the title. 
     HPLC: RT 13.71 min.; purity 80.6% 
     MS: m/z=1133 amu ([M+H] + ) and 567 amu ([M+2H] 2+ )) 
     Example 9 
     cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH 2 )-Phe-(D,L)1,4-MNal-Lys] isomer B 
     From the preparation described in the previous example, the isomer B is also collected pure, the second in the order of elution from the HPLC column. HPLC: RT 14.71 min.; purity 97.7% 
     MS: m/z=1133 amu ([M+H] + ) and 567 amu ([M+2H] 2+ ) 
     Example 10 
     cyclo[Tyr(Bn)-Phe-Pro (4-OCONH(CH 2 ) 2 NH 2 )-Phe-(D)Nal-Lys] 
     The compound is synthesised following the procedure described in example 6, using Fmoc-(D)Nal-OH in the cycle. 
     HPLC: RT 14.14 min.; purity 99.5% 
     MS: m/z=1073 amu ([M+H] + ) and 537 amu ([M+2H] 2+ ) 
     Example 11 
     cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH 2 )-Phe-(D)hPhe-Lys] 
     The compound is synthesised by following the procedure described in example 6, using Fmoc-(D)hPhe-OH in the first cycle. 
     HPLC: RT 13.81 min.; purity 94.5% 
     MS: m/z=1037 amu ([M+H] + ) and 519 amu ([M+2H] 2+ ) 
     Example 12 
     cyclo[Tyr(Bn)-Phe-Pro (4-OCONH(CH 2 ) 2 NHCH 3 )-Phg-(D) Sty-Lys] 
     The compound is synthesised following the procedure described in example 7, using Fmoc-(D)Sty-OH in the first cycle and Fmoc-Phg-OH in the second cycle. 
     HPLC: RT 13.62 min.; purity 97.8% 
     MS: m/z=1049 amu ([M+H] + ) and 525 amu ([M+2H] 2+ ) 
     Example 13 
     cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH 2 )-Phg-(D)hPhe-Lys] 
     The compound is synthesised following the procedure described in example 6, using Fmoc-(D)hPhe-OH in the first cycle and Fmoc-Phg-OH in the second cycle. 
     HPLC: RT 12.78 min.; purity 98.8% 
     MS: m/z=512 amu ([M+2H] 2+ ) 
     Example 14 
     cyclo[Tyr(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH 2 )-Tyr-(D,L)3,8MNal-Lys] isomer B 
     One operates as described in example 5, using Fmoc-Tyr(tBu)-OH in the second cycle. 
     HPLC: RT 13.13 min.; purity 95.4% 
     MS: m/z=1149 amu ([M+H] + ) and 575 amu ([M+2H] 2+ ) 
     Example 15 
     cyclo[Ser(Bn)-Phe-Pro(4-OCONH(CH 2 ) 2 NH 2 )-Phe-(D,L)3,8MNal-Lys] isomer B 
     One operates as described in example 5, using Fmoc-Ser(Bn)-OH in the fifth cycle. 
     HPLC: RT 12.26 min.; purity 98.2% 
     MS: m/z=1057 amu ([M+H] + ) and 529 amu ([M+2H] 2+ ) 
     Experimental Part 
     The compounds of the invention show important pharmacological properties, as indicated in several in vitro and in vivo tests. 
     In particular, the compounds of the invention bond, with good affinity, to at least one of the subtypes of the receptors of the somatostatin. 
     Binding Assays 
     The binding assays were carried out, as is explained below, by using preparations of recombinant human receptors, hSSTR1, hSSTR2, hSSTR3 and hSSTR5, obtained from cell membranes (for example CHO) transfected according to standard methods. 
     The membranes are incubated in duplicate for 60 min. at 25° C. with 3-[125I]iodotyrosyl11Somatostatin-14 (Amersham, IM161, 2000 Ci/mmol) as radioligand and with increasing concentrations of the compound under examination, in 25 mM Hepes (pH 7.4) buffer, containing 5 mM MgCl 2 , 1 mM CaCl 2 , 10 μg/ml of Saponin, 0.5% BSA. The incubation is terminated by means of filtration with a Filtermate Harvester (Perkin Elmer) through GF/B filters, which are then washed 6 times with buffer (25 mM Hepes pH 7.4, 5 mM MgCl 2 , 1 mM CaCl 2 ). The radioactivity of the filters is measured in a TopCount™ or MicroBeta™ reader for 1 min/well after having added the Microscint 20 liquid scintillation (Packard) and incubated for 15 min. in an orbital stirrer. The results are expressed as specific binding percentage of the radio-marked ligand, in the presence of increasing concentrations of the compound under examination. The IC 50  values were calculated by using the “GraphPad Prism” software (IC50=concentration of compound necessary for obtaining half of the maximum inhibition, in the competitive binding test described above). 
     The IC50 values of the compounds of the invention are situated in the nMolar concentration field, preferably comprised between 0.1 and 50 nM. 
                                                                                                 IC50 (nM)                    Compound   hSSTR1   hSSTR2   hSSTR3   hSSTR5                            Example 5   10.8   9.3   0.31   0.42           Example 6   10.0   25.8   0.52   0.64           Example 7   5.8   9.2   1.33   0.97           Example 8   19.1   26.6   2.92   9.78           Example 9   32.4   9.9   2.34   1.90           Example 10   113.8   1.7   1.22   0.52           Example 11   26.9   21.3   1.34   1.18           Example 12   39.3   3.3   4.03   4.86           Example 13   84.7   31.9   3.02   0.54           Example 14   21.7   1.8   0.35   0.36           Example 15   1.0   7.0   1.80   1.62                        
Assay for the Inhibition of the Growth Hormone Release on Rat Pituitary Cells
 
     The compounds of the invention also show an inhibition activity of the growth hormone release (GH), as shown from tests carried out in vitro on rat pituitary cells. The hypophysial glands drawn from adult male rats (CD1-SD, 175-200 g) are cut into little pieces and incubated with collagenase (1 mg/ml) in Hank&#39;s buffer containing 1% BSA, 20 mM Hepes, antibiotics, for 20 min. at 37° C. The dispersed cells, after having been washed several times with buffer, are distributed, with 20000 cells/well, into 48 well plates and are maintained in culture for 6-7 days (DMEM containing 5% foetal bovine serum, 5% horse serum, 1% non-essential amino acids). On the day of the experiment, the cells are washed with Hank&#39;s buffer and are then incubated at 37° C. for 1 h in the presence of Hank&#39;s buffer added with 0.1% BSA and 20 mM HEPES. The buffer is then substituted with fresh buffer, still in the presence of 0.1% BSA and 20 mM HEPES. The cells are then incubated for 3 h at 37° C. in a CO 2  incubator with various concentrations of the products under examination and with 3×10-9 M GHRH. The GH released in the medium is measured by using the Kit ELISA Rat Growth Hormone Biotrack Enzymeimmunoassay (Amersham RPN2561) or the Kit Mouse/Rat GH ELISA (DSL-10-72100) according to supplier indications. The compounds of the invention inhibit the release of GH at concentrations in the range of 10-11 to 10-6 M; the compound of example 5 has an IC50 value of 1.3 nM. 
     Assay for the Inhibition of the Growth Hormone Release on Human, GH-Secreting Hypophysial Adenoma Cells 
     The compounds of the invention also show an inhibition activity of the GH release from human, GH-secreting hypophysial adenoma cells, as indicated from in vitro tests on clinical tumour reports. The test is executed by using human tumour biopsies; the GH produced from the non-stimulated cells, in the presence of variable quantities of the compound under examination, is measured by using the kit ELISA hGH-EASIA (biosource KAP1081) according to the indications of the supplier. In the tumours sensitive to the action of Somatostatin and analogues, the compounds of the invention halve the GH production at concentrations in the range of 10-10 to 10-6 M; preferably at the concentration of 10 nM. 
     Assay for the In Vivo Inhibition of the GH Production, Stimulated by Barbiturates 
     The compounds of the invention inhibit, in vivo, the release of GH stimulated by the administration of Nembutal. The compounds are administrated subcutaneously, at different doses, in male rats (CD, Harlan Italy). Blood samples are collected, at different times, one hour after the animals were anesthetised by means of intraperitoneal administration of Nembutal (60 mg/kg); the hormone levels are measured by means of the ELISA test. In the animals treated with the compounds of the invention, at doses from 5 to 250 μg/kg, there is a decrease of the produced GH levels. The compound of example 1, at the dose of 5 μg/kg, reduces by 55% the release of GH measured six hours after the administration; at the dose of 125 μg/kg the reduction of GH is still measurable 24 hours after the administration. 
     Assay for the Pharmacokinetic Profile 
     The compounds of the invention also show, in rats, a very favourable pharmacokinetic profile. The pharmacokinetic profile was measured by administering the compounds to male rates, subcutaneously, at the dose of 1 mg/kg (CD, Sprague Dawley; 200-250 g). Blood samples were collected, at different times, up to 72 hours after the administration. The concentrations of the compound under examination were measured in the separated plasma samples, by means of an LC-MS/MS analysis method and the values were processed according to a non-compartmental model using the software “Kinetica”. In the following table, the main pharmacokinetic parameters obtained with the compound of example 1 are reported, compared with those obtained with PASIREOTIDE, another stable analogue of somatostatin, currently in clinical development phase (PASIREOTIDE was prepared by following the process described in WO2002010192). 
     
       
         
               
               
               
             
               
               
               
               
               
             
           
               
                   
                   
               
               
                   
                 Example 5 
                 PASIREOTIDE 
               
               
                   
                   
               
             
             
               
                   
               
             
          
           
               
                   
                 Dose 
                 (mg/kg) 
                 1 
                 1 
               
               
                   
                 Cmax 
                 (ng/mL) 
                 224.02 
                 667.88 
               
               
                   
                 tmax 
                 (h) 
                 4 
                 2 
               
               
                   
                 t½ 
                 (h) 
                 31.3 
                 24.4 
               
               
                   
                 AUC0-t 
                 (ng/mL * h) 
                 2728.50 
                 2781.40 
               
               
                   
                 AUCtot 
                 (ng/mL * h) 
                 2883.06 
                 2795.85 
               
               
                   
                 MRT 
                 (h) 
                 18.96 
                 4.87 
               
               
                   
                   
               
             
          
         
       
     
     The compound of example 5 is better than PASIREOTIDE both in terms of half-life and for the mean residence time (MRT); in the case of OCTREOTIDE, the t½ value is about 2 hours. 
     The compounds of the invention are consequently useful for the prevention or treatment of disorders with an origin that comprises or is associated with an excess of GH secretion and/or an excess of IGF-1, such as in the treatment of acromegaly, in the treatment of type I or type II diabetes mellitus, especially in their complications, such as for example angiopathy, proliferative diabetic retinopathy, diabetic macular edema, nephropathy and hyperglycemic phenomenon upon waking and other metabolic disorders connected with the release of insulin or glucagon, such as for example morbid obesity or hypothalamic obesity or hyperinsulenimic obesity. The compounds of the invention are useful also in the treatment of enterocutaneous and pancreatic cutaneous fistulas, irritable intestine syndrome, inflammatory diseases, such as for example Grave&#39;s disease, irritable intestine disease, psoriasis or rheumatoid arthritis, polycystic kidney disease, rapid gastric emptying disease, aqueous diarrhoea syndrome, diarrhoea connected with AIDS, diarrhoea induced by chemotherapy, acute or chronic pancreatitis, gastrointestinal hormone-secreting tumours (for example GEO tumours, such as vipomas, gluconomas, insulinomas, carcinoids and the like), malignant lymphocytes, such as lymphomas or leukaemias, hepatocellular carcinomas like gastrointestinal bleeding, like esophageal varicose bleeding. 
     The compounds of the invention are also useful in the treatment of tumours positive for the somatostatin receptors, such as for example the tumours which bear the receptors SSTR1, SSTR2, SSTR3 and/or SSTR5, as indicated in the proliferative tests with various cancer cell lines which express the receptors for somatostatin. 
     For all of the abovementioned indications, the required dosage will naturally vary in relation to, for example, the patient, the administration mode and the severity of the conditions which must be treated. Generally, however, one obtains satisfying results with administrations from 1 μg up to 0.7 mg/kg/day of the compounds of the invention. A recommended daily dosage for patients is on the order of about 2 μg up to 50 mg, preferably from about 0.01 to about 40 mg, for example from about 0.001 to about 3 mg s.c. of the compound conveniently administered in divided doses, up to 3 times per day, in single dosage forms containing, for example, from about 0.5 μg to about 25 mg, for example from about 2 μg to about 20 mg, for example from about 2 μg to about 1.5 mg of the invention compounds. The conjugates of the compounds of the invention or their pharmaceutically acceptable salts are useful both as agents for the diagnostic imaging, for example for the display of tissues and cells positive for the somatostatin receptors, such as the tumours and metastases positive for the somatostatin receptors, and for the inflammatory or autoimmune disorders which show somatostatin receptors, tuberculosis or the rejection of organs after transplant, when complexed with a detectable element, such as for example the γ nuclides or emitting positrons, a fluorescent metal ion or a paramagnetic ion, such as for example  111 In,  161 Tb,  177 Lu,  68 Ga, Eu 3+ , Gd 3+ , Fe 3+ , Mn 2+  or Cr 2+ , or as radio-drugs for the in vivo treatment of tumours and metastases positive for the somatostatin receptors, for rheumatoid arthritis, and severe inflammation conditions, when complexed with a α- or β-emitting nuclide with a cascade of Auger electrons, for example  90 Y,  161 Tb,  177 Lu,  211 At,  213 Bi  201 Tl. 
     The conjugates of the compounds of the invention in complexed form for use in the diagnostic imaging can be administered intravenously, for example in injectable solution or suspension form, preferably in single injection form. The radiotracers can preferably be made just before the patient administration. 
     In animals, a recommended dosage range can be from 0.01 to 1 μg/kg of conjugate of the compounds of the invention, complexed with 0.02-0.5 mCi of γ-emitting radionuclide. In the largest mammals, such as humans, a recommended dosage range can be from 1 to 100 μg/m 2  of conjugate of the compounds of the invention complexed for example with 1-100 mCi/m 2  of detectable element, such as  111 In,  86 Y or  177 Lu. 
     The dosages used in the radiotherapeutic use practice of the present invention will of course depend on the particular conditions which must be treated, for example the known radiotoxicity for healthy organs which express the somatostatin receptors, the size of the tumour mass and the desired therapy. In general, the dose is calculated based on the pharmacokinetic data and distribution data of the radioactivity obtained from healthy organs and based on the uptake observed on the target. A β-emitting complex or a conjugate of the compounds of the invention can be repeatedly administered, for example for a period of 1-3 months. 
     In animals, a recommended dosage range can be from 20 to 100 μg/kg of conjugate of the compounds of the invention complexed with 15-70 mCi of an α- or β-emitting nuclide, or a nuclide with the Auger electron cascade, such as for example  90 Y,  177 Lu or  161 Tb. In larger mammals, such as humans, a recommend dosage range can be from 1-100μ/m 2  of a complexed conjugated compound of the invention, for example from 1-100 mCi/m 2  of an α- or β-emitting nuclide or a nuclide with Auger electron cascade, for example  90 Y,  177 Lu or  161 Tb. 
     The conjugates of the compounds of the invention in complexed form for use as radiotherapy agents can be administered through any conventional path, for example intravenously, for example in injectable solution form. They can be advantageously injected by infusion, for example with a 15-60 min infusion. Depending on the tumour site, it can be administered as close as possible to the tumour site, for example through a catheter. The present invention also provides a pharmaceutical composition comprising a conjugate of the compounds of the invention in free base form or as pharmaceutically acceptable salt or as complex with a detectable or radiotherapeutic agent, together with one or more pharmaceutically acceptable excipients or diluents. 
     The compounds of the invention or their conjugates in complexed form are useful for mapping or treating the tumours which express or accumulate the receptors, like the pituitary tumours, gastro-entero-pancreatic tumours, carcinoids, tumours of the central nervous system, breast tumours, prostate tumours (including advanced hormone-refractory prostate cancer), ovarian or colon tumours, small cell lung tumour, malignant intestinal occlusion, paragangliomas, kidney cancer, skin cancer, neuroblastomas, pheochromocytomas, medullary carcinoma of the thyroid, myelomas, lymphomas, Hodgkins lymphomas and non-Hodgkins lymphomas, bone tumours and their metastases, along with autoimmune or inflammatory disorders, for example rheumatoid arthritis, Grave&#39;s disease or other inflammatory diseases of the eye. 
     The compounds of the invention or their complexed conjugates can be administered as single active ingredient or they can be administered in combination, for example as adjuvants, with other active ingredients. For example, they can be used in combination with an immunosuppressive agent, for example an inhibitor of the calcineurin, like cyclosporine A or FK506; with a macrocyclic lactone having immunosuppressive properties, like rapamycin; with a monoclonal antibody with immunosuppressive properties or with an anti-inflammatory agent. 
     The compounds of the invention or their complexed conjugates can also be used in combination with an anti-proliferative agent, for example a chemotherapeutic active ingredient, like paclitaxel, gemcitabine, cisplatin, doxorubicin, 5-fluorouracyl or taxol, with a hormonal or antagonist agent, for example an anti-androgen or mitoxantrone (especially in the case of prostate cancer) or with an anti-estrogen, like letrozole (especially in the breast cancer cases), with a antimetabolite, with an alkaloid from a plant, with a biological response modifier, preferably an interferon or a lymphokine, with a protein tyrosine kinase inhibitor and/or with the serine/threonine kinases, with an enzyme inhibitor of histone-deacetylase or with an agent with other or unknown action mechanisms, such as for example anepothilone or epothilone derivatives, or with a macrocyclic lactone such as for example rapamycin, RAD or CCI779. 
     When the compounds of the invention or their conjugates in complexed form are administered in combination with another drug, the doses of the co-administered drugs will of course vary as a function of the conditions to treat and so on. The terms “co-administration” or “combined administration” or the like are used here to signify an administration of the therapeutic agents chosen for a single patient, and intend to include treatment regimes in which the agents are not necessarily administered by the same administration pathway or at the same time. 
     The particular combination of the invention will be selected depending on whether the disease or disorder must be prevented or treated; for example, a combination with immunosuppressive agent, for example for the prevention or treatment of chronic transplant rejection, a combination with an insulin secretagogue, with a promoter of the insulin secretion, with an insulin sensitiser or with a low insulin dose in the treatment of diabetes and in its complications, a combination with an anti-inflammatory agent for the prevention and treatment of inflammatory diseases or disorders, a combination with an agent with anti-angiogenic effect for the prevention or treatment for example of macular edema or degeneration or cancer, a combination with a chemotherapeutic agent for use in cancer.