CA2284459C - Combinatorial synthesis of libraries of macrocyclic compounds useful in drug discovery - Google Patents

Abstract

A library of macrocyclic compounds of the formula (I) (see formula I) - where part (A) is a (see formula II) bivalent radical, a -(CH2)y- bivalent radical or a covalent bond; - where part(B) is a (see formula III) - bivalent radical, a -(CH2)z- bivalent radical, or a covalent bond; - where part (C) is a (see formula IV) - bivalent radical, a -(CH2)t- bivalent radical, or a covalent bond; and - where part (T) is a - Y - L - Z - radical wherein Y is CH2 or CO, Z is NH or O and L is a bivalent radical. These compounds are useful for carrying out screening assays or as intermediates for the synthesis of other compounds of pharmaceutical interest. A process for their preparation of these compounds in a combinatorial manner, is also disclosed.

Description

COMBINATORIAL SYNTHESIS OF LIBRARIES OF MACROCYCLIC COMPOUNDS
USEFUL IN DRUG DISCOVERY

FIELD OF THE INVENTION

The present invention relates to new macrocyclic compounds of biologically interesting structures.

The invention also relates to a process for preparing these new compounds by lactam or Mitsunobu cyclization.

BACKGROUND OF THE INVENTION

As everybody knows, medicinal chemistry research has been dramatically transformed by biotechnology. Previously synthetic chemistry and natural products screening dominated drug research, but now molecular biology has become a driving force behind screening and the establishment of molecular targets.

Over the last years, most of the research in biotech companies has been directed to peptide and protein therapeutics in spite of problems associated with their low bioavailability, rapid metabolism, and lack of oral activity.
Because of these limitations, research groups continue to rely upon chemical synthesis of nonpeptide substances for drug discovery, recognizing that small molecules are likely to remain the most viable avenue for the identification and optimization of potential drugs.

As is also known, combinatorial chemistry is a technique by which large chemical libraries can be generated by connecting together appropriate chemical building blocks in a systematic way. The ability to generate such large, chemically diverse libraries, either in a combinatiorial fashion or by any other high throughput parallel synthetic methods, combined with high throughput screening techniques, provides an immensely powerful tool for drug lead discovery and optimization.

Drug companies are increasingly interested in harnessing the ability of combinatorial synthesis to produce large collections (or libraries) of molecules to augment their existing sources of molecular diversity, and to fully exploit their capacity to capture millions of biological assay data points annually using high throughput robotic screening instrumentation.

This new science is still in its infancy, and to date most successful scaffold are derived from small heterocycles which are usually synthesized in very few steps. Thus several focused libraries have been built around bioactive cores such as benzodiazepines. However, this approach cannot be considered as a true method to generate innovative lead structures. Rather, it is a mean to optimize existing leads and is usually applied in drug development schemes.

Random libraries destined to search for innovative leads are very few today. As one example, a library based on diketopiperazine yielded a new submicromolar lead for a neurokinin-2 receptor after screening of this library on a variety of targets.

It is obvious that not all scaffolds may lead to potent drug candidates. Some very simple molecules requiring only one or two chemical steps may seem very attractive due to the huge size of the libraries that can be generated from them. Nonetheless, too simple molecules do not usually provide useful leads since they tend to lack target specificity, a prerequisite for a molecule to become a drug.

A class of organic structures with outstanding pharmaceutical activity has been termed as "macrocycle family". Compounds like Taxol, Epothilone, Erythromycin, Neocarzinostatin, Rifampin and Amphotericin are either under clinical study or already marketed drugs and belong to this important family. Most of these products are of natural origin, since they are not usually tackled by medicinal chemists due to lack of knowledge associated with their synthesis.

Over the last years, the present inventors have developed expertise in the field of macrocycles synthesis. With such an expertise, they have developed a method of synthesis and evaluation of libraries of partially peptidic macrocycles which mimic 0-turns, thereby making it possible to quickly explore huge quantities of conformationally restricted structures.

OBJECTS AND SUMMARY OF THE INVENTION

A first object of the present invention is to provide a process for preparing macrocyclic compounds, which process can be carried out with a large variety of functional functional groups and in the presence of a large variety of solvent systems and resins, and thus can be used for preparing a large variety of macrocyclic compounds of biologically interesting structures that could be used for carrying out screening assays or as instrumental for the synthesis of other macrocyclic compounds. Libraries of such synthetic compounds should actually be as attractive as the libraries of extracted natural products which are presently used in high throughput biological screening assays.

Another object of the invention is to provide libraries of macrocyclic compounds incorporating two to five building units: one to four amino-acids and a tether chain for controlling the overall shape of the molecule.

More specifically, the macrocyclic compounds of the invention have the general formula (I):

20 (13) (C) (I) (A) (1) C.
iH,.(CH 2) ~t l x and salts thereof;

- where part (A) is a H H
II (CH2)y-N

bivalent radical having its -NH- group linked to the carbonyl group of part H
(CH2)x-II I I
O R~ X
a -(CH2)y- bivalent radical, or a covalent bond;
where part (B) is a H H
C (CH2)z-N

bivalent radical having its -NH- group linked to part (A), a -(CH2)z- bivalent radical, or a covalent bond;

where part (C) is a H H
II (CH2)t N

bivalent radical having its -NH- group linked to part (B), a -(CH2)t- bivalent radical, or a covalent bond;

where part (T) is a - Y - L - Z - radical having its Y
group linked to the -NX- of formula (I) and its -Z- group linked to the carbonyl group of part (c); and - where X is a monovalent group selected from the group consisting of: -S02-Ar, -S02-CH3, -S02-CF3, -H, -CHO, -CO-CH3, -CO-Ar, -CO-R, -CO-NHR, -CO-NHAr, -CO-O-tBu, -CO-O-CH2-Ar, II s \

II ~ i U N
and j---r (CH2),,-NH-R5 Ro wherein:
= Ar being an aromatic group, substituted aromatic group or a heteroaromatic group, = a being an integer selected from the group consisting of 0, 1 and 2, = R being a monovalent group - (CH2) n-CH3 or - (CH2) n-Ar with n being an integer from 1 to 16, R0, R1, R2, R3 and R4 being independently selected *
from the group consisting of: -H, -CH3, N
H
NH
HN

OH OH, 0 OH, R8 , SH , SO3H

* SO2 * S * --S03CH3 and wherein the * indicates the bond location of R0, R1, R2, R3 and R4 to the rest of the structure;

R1, R2 and R3 being optionally protected by protecting groups (PG1), (PG2) and (PG3) respectively, said protecting groups being those used for orthogonal protections in peptide synthesis;

R5, being a monovalent radical selected from the group consisting of: -H, -S02-CH3, -S02-CF3, -CHO, -COCH3, -CO-Ar, -CO-R, -CO-NHR -CONHAr, -COO-tBu and -COO-CH2-Ar, wherein R
and Ar are defined as above, R8 being -OH or -NH2, where Y is a bivalent group -CH2-;
where Z is a bivalent group -NH- or -0-;

wherein x, y, z and t are integers being each independently 0, 1 or 2;

wherein L is a bivalent radical having the formula:

-(CH2)d-A-(CH2)j-B-(CH2)e-, d being an integer from 0 to 5, e being an integer from 1 to 5, j being an integer from 0 to 5, when j is 0, A
or B is present, with A and B being independently selected from the group consisting of:

-0-, -NH-, -NR- wherein R is defined as above, -S-, -CO-, -SO-, -CO-O-, -0-CO-, -CO-NH-, -NH-CO-, -S02-NH-, -NH-S02-,-CHOH-, -CH=CH-with the // \\
configuration Z or E, -C=C-, G1 and GZ

Gi with the substituent -G2- in a 1,2; 1,3 or 1,4 position, Gl being selected from the group consisting of:
-0-, -NH-, -NR- wherein R is defined as above, -S-, -CH=CH- with a z configuration, and -CH=N-; and G2 being selected from the group consisting of:

-0-, -NH-, and -NR- wherein R is defined as above.

Salts of said compounds are also within the scope of the invention.

As may be understood, the new macrocyclic compounds according to the invention incorporate two to five building units, one to four amino-acids units and a tether chain which controls the shape of the molecule.

These compounds display enhanced stability towards peptidases and exhibit facilitated cell penetration as compared to the corresponding open chain linear equivalents.

Some of the compounds according to the invention includes a (3--turn motif within their rings:

Ri+ O
Ri+2 N
HN H O
O H-N

Ri Ri+s Cl llz~

13-turn It is known that Q-turn is one of the three major motifs of peptide and protein secondary structure. t3-turn plays a key role in many biological molecular recognition events including interactions between antigens and antibodies, peptide hormones and their receptors, and regulatory enzymes and their corresponding substrates. In order to attain high affinity and selective binding to a targeted receptor, a R-turn mimetic must reproduce both the functionality and the orientation of the side chains of the 10 receptor-bound peptide ligand.

The inherent diversity in R-turn structure compounded with difficulties in identifying the key residues responsible for binding, make the design of R-turn mimetics quite challenging.

As may be appreciated, the present invention permits to circumvent the aforementioned difficulties by providing compounds which, thanks to their structure which incorporate numerous side chain combinations as well as multiple different side chain orientations, can be used as R-turn mimetics and evaluated accordingly.

Obviously, the preparation of libraries of a-turn mimetics represent a goal of the present invention. However, the latter is not exclusively restricted to such compounds.
There are numerous other compounds according to the invention which include other interesting di- or tri-peptide motif with their structure whose active conformation need be probed by our conformation restrictive approach.

As is known many adhesive proteins present in extracellular matrices and in the blood contain the tripeptide arginine-glycine-aspartic acid (RTGD) as their cell recognition site. These proteins include fibronectin, vitronectin, osteopontin, callagens, thrombospondin, fibrinogen adn von Willebrand factor. The RGD sequence of each of the adhesive proteins are recognized by at least one member of a family of structurally related receptors, integrins, which are heterodimeric proteins with two membrane-spanning sub-units. Some of these receptors bind to the RGD sequence of a single adhesion protein only, wheras others recognize groups of them. The conformation of the RGD sequence in the individual proteins may be critical to this recognition specificity. On the cytoplasmic side of the plasma membrane the receptors connect the extracellular matrix to the cytoskeleton.

More than ten proved or suspected RGD-containing adhesion-promoting proteins have already been identified, and the integrin family includes at least as many receptors recognizing these proteins. Together the adhesion proteins and their receptors constitute a versatile recognition system providing cells with anchorage, traction for migration, and signals for polarity, position, differentiation and possibly growth. Compounds according to the invention containing the sequence Arg-Gly-Asp in a controled topology could inhibit cell to cell adhesion processes. Such compounds could be important in the areas of antithrombotic and cancer research.

Also included within the scope of the invention are compounds of the above mentioned formula (I) containing a biaryl bridge.

Preferably, the macrocyclic compound of formula (I) can also be selected from the group consisting of:

E
CIS CH3cH2cH2c020 N 0 H
H Y --- Ae Pnco2e D

Q

NH
and e 0 40 H
H

As can be appreciated, the compounds according to the invention have much flexibility and can adopt structures very different from conventional 13-turns, according to the nature of their spacer parts. This means that the scope of the invention is broad and molecular modeling design allows the design of (3 and non-(3-turns.

A main advantage of the invention is that the compounds of the formula (I) are neither too tight like small rings nor too loose like aliphatic chains.

The invention is also directed to a process for preparing a compound of the formula (I), comprising the steps of:

a) preparing by coupling a first building block deriving from natural or synthetic amino-acids, said first building block being of the formula:
H
H i (CH2)X I II (A)-(B)-(C)-Sp-P
X Ri O

wherein x, X, R1, part (A), part (B), and part (C)are defined as above, Sp is -S or -S NH-and P is -CH3 or -CH2-Ph when the coupling is carried out in liquid phase, and Sp is 0-~. N P

-S 0- or -S NH-and P is polystyrene or methoxypoly(ethyl eneglycol) when the coupling is carried out in solid phase;

b) coupling the first building block prepared in step a) with a second building block hereafter called "tether", of the formula:

H-Y-L-Z-PGz wherein Y, L and Z are defined as above and PGz is a protecting group;

c) removing the protecting group PGz from the compound obtained in step b); and d) carrying out a macrocyclization of the unprotected product obtained in step c) and a cleavage if the above mentioned steps (a) and (b) were carried out in a solid phase, in order to obtain the requested compound of the formula (I).

As can be noted, this process uses lactam or Mitsunob cyclization to prepare the libraries of compounds according to the invention. It is very versatile and can be carried out in a combinatorial manner, either in solid phase or in solution phase.

14a The invention and its advantages will be better understood upon reading the following non restrictive detailed description and examples made with reference to the accompanying drawings.

BRIEF DESCRIPTION OF THE DRAWINGS

Figure 1 is a table detailing the structure that may have the compounds of the formula (I) according to the invention.
Figure 2a and 2b are schematic illustrations of the sequence of steps that must be carried out to obtain the library of compounds of formula (8), which is part of the "family 2"
libraries shown in Figure 1 for which Y is a methylene group (-CH2-) , and the amino-acids at positions 1, 2 and 3 are a-amino-acids (x, y, z = 0).

Figure 3 is a schematic illustration of the steps that must be carried out to obtain other libraries of compounds of formulae (9) to (12), which are also parts of the "family 2" libraries shown in Figure 1, for which Y is a methylene group (-CH2-), and the amino-acids at positions 1, 2 and 3 are a-amino-acids (x, y, z = 0).

Figures 4a and 4b are schematic illustrations of the sequence of steps that must be carried out to obtain libraries of compounds of the formulae (17) and (18) which are parts of the "family 2" libraries shown in Figure 1, for which Y is a carbonyl group (-CO-), and the amino-acids 10 at positions 1, 2 and 3 are (x-amino-acids (x, y, z = 0).

DETAILED DESCRIPTION OF THE INVENTION

As aforesaid, the process according to the invention is versatile enough to prepare a large number macrocyclic compounds, the main "families" of which are illustrated in Figure 1. This process comprise the following basic steps:

a) preparing by coupling a first building block deriving from natural or synthetic amino-acids, b) coupling the first building block prepared in step a) with a second building block called "tether", c) removing the protective group from the compound obtained in step b), and d) carrying out a macrocyclization of the unprotected product obtained in step c) to obtain the requested compound.

As aforesaid, the process permits to prepare a large number of compounds either in a solution phase or on a solid support using an IRORI combinatorial chemistry set up or an other set up like an Argonault apparatus.

In the synthesis shown in Figure 2a, a first suitably protected amino-acid identified as "A" is activated as a thioester (solution phase or solid phase) or as an oxime ester (Kaiser resin solid phase support) to give a compound of formula (1). The amine protection (PG(x in the case of a-amino-acids PG(3 in the case of R-amino-acids and PGy in the case of y-amino-acids) is removed to give the compound of formula (2). A second amino-acid identified as "B" is then added in the same way to give a compound of formula (3), followed again by removal of the amine protection to give a compound of formula (4). A third acid of formula (C) (figure 2b) is coupled to the amine of formula (4) to yield a sulfonamide of the formula (5), which is immediately coupled with an alcohol of the formula (D) under Mitsunobu conditions to give a compound of formula (6). This compound of formula (6) can also be obtained directly from the compound of formula (4) by peptide coupling with an acid of formula (E). The terminal alcohol (Z = 0) or amine (Z = NH) protecting group (PGz) is then cleaved to give the corresponding alcohol or amine of formula (7), which can undergo cyclization and cleavage all at once to give requisted compound according to the invention of formula (8).

As shown in Figure 3, the orthogonal protections (PG1, PG2, PG3 and PG4 when a fourth amino-acid is introduced) of the compound of formula (8) can be removed to yield the compound according to the invention of formula (9). Another compound according to the invention of formula (10) can be obtained from the compound of formula (8) by cleaving the sulfonamide portion of the molecules. The resulting free amine can be coupled with various acids (see X groups in figure 1) to yield a compound of formula (11) according to the invention. Subsequent cleavage of the orthogonal protecting groups (PGO when X is an amino-acid, PG1, PG2, PG3 and PG4 when a fourth amino-acid is introduced) yield a compound of formula (12) according to the invention.

As shown in figure 4, it is also possible from the amine of formula (4) to couple an amino-acid of formula (C') to yield a compound of formula (13) according to the invention, whose amine protecting group (PGa, PGb or PGg) can be cleaved to give the amine of formula (14). A
hydroxy-acid (Z = 0) or amino-acid (Z = NH) of formula (D') is then coupled to yield a compound according to the invention of formula (15). The terminal alcohol (Z = 0) or amine (Z = NH) protecting group (PGz) is then cleaved to give the corresponding alcohol or amine of formula (16), which can undergo cyclization and cleavage all at once to yield a compound according to the invention of formula (17). The orthogonal protections (PG1, PG2, PG3 and PG4 when a fourth amino-acid is introduced) of the compound of formula (17) see figure 4b can be removed to yield a compound of formula (18).

The above example of synthesis deals with the preparation of libraries of the "family 2" type for which positions 1, 2 and 3 are filled. Libraries of "families 1, 3 and 4" type as shown in Figure 1 can be prepared exactly in the same way. In "family 1" type libraries, an extra amino-acid is incorporated at position 4. In "family 3" type libraries, positions 3 and 4 are empty and in "family 4" type libraries positions 2, 3 and 4 are empty.

Thus, it is possible to develop chemical libraries of dozens, hundreds, and even many thousands of discrete chemical compounds, in an efficient and reliable manner.
This being the case, it is possible to use these libraries as chemical intermediates for the preparation of pharmaceutical compounds or for the identification of such pharmaceutical compounds or other useful species. Some of these compounds could also be used without further modification. Accordingly, the ability to prepare such complex libraries in a reliable and predictable fashion is highly desired.

The term "phamaceutical" as used herein means the ability of the compounds to provide some therapeutic or physiological beneficial effect. As used herein, the term includes any physiologically or pharmacologically activity that produces a localized or systemic effect or effects in animals including warm blooded mammals such as humans.
Pharmaceutically active agents may act on the peripheral nerves, adrenegic receptors, cholinergic receptors, the skeletal muscles, the cardiovascular system, smooth muscles, the blood circulatory system, synoptic sites, neuroeffector junctional sites, endocrine and hormone systems, the immunological system, the reproductive system, the skeletal system, the autocoid system, the alimentary and excretory systems, the histamine system and central nervous systems as well as other biological systems. Thus, compounds derived from compositions of the present invention may be used as sedatives, psychic energizers, tranquilizers, anticonvulsant, muscle relaxants, anti-Parkinson agents, analgesics, anti-inflammatories, local anesthetics, muscle contractants, antibiotic, antiviral, antiretroviral, antimalarials, diuretics, lipid regulating agents, antiandrogenic agents, antiparasities, neoplastics and chemotherapy agents. These compounds could further be used to treat cardiovascular diseases, central nervous system diseases, cancer metabolic disorders, infections and dermatological diseases as well as other biological disorders and infections.

Among the potential uses of the compounds according the present invention are uses in scientific research as research reagents. In accordance with the present invention, it is now possible to prepare pluralities of compounds to create libraries of compounds for research.
Such libraries are known to be useful and are important in the discovery of new drugs. In view of the chemical and conformational diversities of such compounds e.g. the large number of functionalizable sites, a very large number of different compounds can be prepared. Moreover, such compounds can be prepared differentially, that is, in such a fashion that a population of known species can be prepared reliably, ensuring that all potential members of a family of chemical species are in fact synthesized.

In view of the foregoing, persons of ordinary skilled in the art will know how to synthesize such libraries, comprising chemical compositions within the scope and spirit of this invention and to assay the libraries against etiological agents or in tests or assays, in order to identify compounds having antibacterial, antifungal, antiviral, antineoplastic or other desired pharmaceutical, biological, or chemical activity.

SPECIFIC EXAMPLES

Preparation of macrocyclic compounds according to the invention by the process outlined above will be illustrated by the following non-limiting specific examples Example 1 Library of 135 members (solution phase) (see Figure 2a) 10 This library (family 2 type) consists of a linear sequence of three natural L-a-amino- acids linked together by an aliphatic chain with 4 or 5 carbons in a head to tail manner. The first amino acids (AA1) are glycine, leucine and methionine, the second ones (AA2) are glycine, histidine(Doc), leucine, proline and valine, and the third ones (AA3) are gylcine, methionine and phenylalanine.

The three third amino acids (Boc-AA3) were converted to their thioesters by coupling with methyl 3-mercapto-propionate. The formed compounds were coupled with the 20 second five amino acids to produce 15 dipeptides which were then converted to 135 linear tripeptides by coupling with nine N-alkylated N-betsyl amino-acids. The end-to-end cyclization of the linear tripeptide thioesters was achieved by silver cation-assisted lactamization.

Amino acid, thioesters (Boc-AA3-S (CH2) 2CO2Me) :
Chlorotrimethylsilane (276 mL, 2.18 mol) was added slowly to a solution of 3-mercaptopropionic acid (70 g, 0.66 mol) in methanol (267 mL, 6.6 mol) at -10 C. The reaction mixture was then stirred for 1 h at 0 C and for 1 h at room temperature. The mixture was neutralized with saturated aqueous sodium bicarbonate to pH 8 and extracted with dichloromethane (3 X 300 mL). The combined organic phase was washed with saturated aqueous sodium bicarbonate (2 X
200 mL), brine (2 X 200 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure. The residue was then distilled (70 C/20 mmHg) to give methyl 3-mercaptopropionate as a colorless oil (61.2 g) in the yield of 77%.

1- (3-dimethylaminopropyl) -3-ethylcarbodiimide hydrochloride (42 mmol) was added to a solution of N-Boc amino-acid (33 mmol), methyl 3-mercaptopropionate (30 mmol) and 4-dimethylaminopyri dine (3 mmol) in dichloromethane (80 mL) at 0 C. The resulting mixture was stirred for 1 hour at 0 C
and 30 min at room temperature. The reaction mixture was diluted with ethyl acetate (200 mL), washed with 1N
hydrochloric acid (2 X 50 mL), saturated aqueous sodium bicarbonate (2 X 50 mL), brine (2 X 50 mL), dried over magnesium sulfate, and evaporated to give the desired thioester (Boc-AA3-S(CH2)2CO2Me) in yields ranging from 95 to 100%.

Dipeptides (Boc-AA2-AA3-S(CH2)2CO2Me):

To a solution of the N-Boc amino acid thioester (Boc-AA3-S(CH2)2CO2Me) (5 mmol) in dichloromethane (2 mL), triethylsilane (10 mmol) was added , followed by trifluoro-acetic acid (3 mL) . The reaction mixture was stirred for 1 h at room temperature, then diluted with toluene (2X10 mL) and the solvent was evaporated to' give the TFA salt of H-AA3-S(CH2)2CO2Me.

To a solution of N-Boc amino acid (Boc-AA2-OH) (5 mmol) and 1-hydroxybenzotriazole (5 mmol) in tetrahydrofuran (5 mL) and dichloromethane (5 mL) at 0 C, 1-(3-dimethylamino-propyl)-3-ethylcarbodiimide hydrochloride (7 mmol) was added. The resulting mixture was stirred for 5 min at 0 C
and for 20 min at room temperature, then cooled down to 0 C.

A solution of the TFA salt of H-AA3-S(CH2)2CO2Me (5 mmol) in dichloromethane (5 mL) was added to the above reaction mixture at 0 C, followed by diisopropylethylamine (7.5 mmol). The resulting reaction mixture was then stirred at the same temperature for 10 min. The ice-water bath was removed and the reaction was stirred for 2 to 4 h at room temperature. Finally, the reaction mixture was diluted with ethyl acetate (80 mL) and washed with 1N hydrochloric acid (2 X 15 mL), saturated aqueous sodium bicarbonate (2 X
15 mL), brine (2 X 20 mL), dried over magnesium sulfate, and evaporated to give the dipeptide (Boc-AA2-AA3-S(CH2)2CO2Me) in yields ranging from of 80 to 100%.

Alkylated tripeptides (N-Bts- (N-alkylated) AA1 AA2 AA3-S (CH2) 2CO ) To a solution of N-Boc dipeptide (0.5 mmol) in dichloro-methane (1 mL), triethylsilane (2 mmol) was added, followed by trifluoroacetic acid (1 mL) . The reaction mixture was stirred for 1 h at room temperature and then diluted with toluene (2X5 mL) and evaporated to give the dipeptide TFA
salt.

To a solution of alkylated N-Betsyl amino acid (0.5 mmol) and 1-hydroxybenzotriazole (0.5 mmol) in tetrahydrofuran (2 mL) and dichloromethane (2 mL) at 0 C, 1-(3-dimethyl-aminopropyl)-3-ethylcarbodiimide hydrochloride (0.7 mmol) was added. The resulting mixture was stirred for 5 min at 0 C then for 30 min at room temperature, and cooled down to 0 C .

A solution of the dipeptide TFA salt (0.5 mmol) in dichloromethane (2 mL) was added to the above reaction mixture at 0 C, followed by diisopropylethylamine (0.8 mmol). The reaction mixture was then stirred for 10 min at the same temperature. The ice-water bath was removed and the reaction was stirred for 2 to 4 h at room temperature. The reaction mixture was diluted with ethyl acetate (50 mL) and washed with 1N hydrochloric acid (2 X 10 mL), saturated aqueous sodium bicarbonate (2 X 10 mL), brine (2 X 10 mL), dried over magnesium sulfate, and evaporated to give the alkylated tripeptides (Bts-(N-alkylated)-AA1-AA2-AA3-S(CH2)2CO2Me) with yields ranging from 11 to 100%.

Preparation of cyclotripeptides To a solution of the alkylated tripeptide (Bts-(N-alkylated)-AA1-AA2-AA3-S(CH2)2CO2Me) (0.5 mmol) in dichloro-methane (1 mL), triethylsilane (2 mmol) was added, followed by trifluoroacetic acid (1 mL) . The reaction mixture was stirred for 1 h at room temperature and then diluted with toluene (2 X 5 mL) and the solvent was evaporated to give the TFA salt of alkylated tripeptide.

To a solution of the TFA salt of alkylated tripeptide (0.5 mmol) in ethyl acetate (250 mL), diisopropylethylamine (1.0 mmol) and silver trifluoroacetate (1.5 mmol) were added. The reaction mixture was stirred for 1 to 3 h at room temperature (Thin Layer Chromatography monitoring of the reaction). Brine (50 mL) and 1.0 M aqueous sodium thiosulfate (30 mL) was added and stirred for 60 min. The organic phase was washed with saturated EDTA aqueous solution (2 X 50 mL), 1N hydrochloric acid (50 mL), brine (2 X 50 mL), dried over magnesium sulfate and evaporated to give the crude product. The crude can be purified by flash column chromatography if necessary.

Name MW Quantity Yield Purity Name MW Quantity Yield Purity Level Level (mg) (%) (%) (mg) (%) (%) c-B-GGG-1 451 25 14 100 c B MLG-1 581 200 93 91 c-B-GGM-1 525 170 77 94 c-B-MLM-1 655 162 61 99 c-B-GGF-1 541 60 44 96 c-B-MLF-1 671 150 89 97 c-B-LGG-1 507 180 87 92 c-B-GPG-1 491 26 21 85 c-B-LGM-1 581 95 40 95 c-B-GPM-1 565 121 nd 87 c-B-LGF-1 597 93 83 93 c-B-GPF-1 581 80 62 89 c B MGG-1 525 80 35 96 c -B-LPG-1 547 73 63 97 c-B MGM-1 599 66 28 94 c-B-LPM-1 621 28 31 55 c-B-MGM-1 599 31 10 77 c-B-LPF-1 637 25 9 85 c-B MGF-1 615 82 27 97 c-B-LPF-1 637 135 64 92 c B MGF-1 615 25 6 69 c-B-MPG-1 565 102 58 91 c-B-GHG-1 673 107 53 91 c-B-MPM-1 639 10 98 99 c-B-GHM-1 747 97 59 98 c-B MPF-1 655 140 61 76 c-B-GHF-1 763 177 68 91 c-B-GVG-1 493 100 56 100 c-B-LHG-i 729 82 61 85 c-B-GVM-1 567 13 9 59 c-B-LHM-1 803 133 65 80 c-B-GVF-1 583 142 75 80 c-B LHF-1 819 162 74 97 c-B-LVG-1 549 142 77 96 c B-MHG-1 747 177 63 97 c-B-LVM-1 623 78 95 90 c-B-MHM-1 821 160 44 90 c B-LVF-1 639 290 85 89 c-B MHF-1 837 201 51 91 c-B MVG-1 567 303 95 90 c-B-GLG-1 507 229 90 97 c-B MVM-1 641 26 66 96 c-B-GLM-1 581 146 68 99 c-B-MVF-1 657 222 64 85 c-B-GLF-1 597 130 81 80 c-B-LLM-1 637 123 69 95 c-B LLG-1 563 152 88 92 c-B-LLF-1 653 221 97 96 Table 1. Results for the cyclic peptides with the E-alkene linker.

Name MW Quantit Yield Purity Name MW Quantity Yield Purity y (mg) (%) (%) (mg) (%) (%) c-B-GGG-2 437 2 1 89 c-B-MLG 2 567 308 55 56 c-B-GGM-2 511 250 77 86 c-B MLM-2 641 38 5 28 c-B-GGF-2 527 46 46 96 c-B MLF-2 657 206 32 44 c-B-LGG-2 493 142 76 99 c-B-GPG-2 477 31 29 92 c-B-LGM-2 567 112 23 55 c-B-GPM-2 551 76 nd 82 c-B-LGF-2 583 64 35 67 c-B-GPF-2 567 55 42 92 c-B-MGG-2 511 56 49 9,6 c-B LPG-2 533 0 nd c-B-MGM-2 585 28 10 87 c-B-LPM-2 607 34 54 49 c-B-MGM-2 585 40 14 77 c-B-LPF-2 623 19 8 96 c-B-MGF-2 601 75 20 94 c-B-MPG-2 551 46 22 78 c-B-MGF-2 601 32 9 88 c-B-MPM-2 625 5 1 59 c-B-GHG-2 659 80 49 93 c-B-MPF-2 641 44 11 49 c-B-GHM-2 733 52 22 63 c-B-GVG-2 479 61 23 85 c-B-GHF-2 749 159 39 66 c-B-GVM--2 553 59 80 93 c-B-LHG-2 715 72 47 94 c-B-GVF-2 569 191 86 76 c-B-LHM-2 789 111 31 51 c-B-LVG-2 535 92 36 89 c-B LHF-2 805 169 46 67 c-B-LVM-2 609 60 57 93 c-B-MHG-2 733 30 9 98 c-B-LVF-2 625 152 36 87 c-B MHM-2 807 90 6 42 c B-MVG-2 553 112 30 82 c-B-MHF-2 823 159 30 69 c-B MVM-2 627 6 7 48 c-B-GLG-2 493 166 97 100 c-B MVF-2 643 0 nd c-B-GLM-2 567 143 85 97 c-B-LLM-2 623 85 26 61 c-B-GLF-2 583 90 32 57 c-B-LLF-2 639 193 43 77 c-B-LLG-2 549 110 48 94 Table 2. Results for the cyclic peptides with the Z-alkene linker.

Name MW Quantity Yield Purity Name MW Quantit Yield Purity y (mg) (%) (%) (mg) (%) (%O
c-B-GGG-3 435 11 6 96 c-B-LLG-3 547 124 46 83 c-B-GGM-3 509 258 58 85 c-B-LLG-3 547 61 11 41 c-B-GGF-3 525 15 9 93 c-B-LLM--3 621 148 62 81 c-B-LGG-3 491 150 69 91 c-B-LLF-3 637 196 55 82 c-B-LGM-3 565 60 22 98 c-B-MLG-3 565 167 24 40 c-B-LGM-3 565 86 27 84 c-B-MLM-3 639 27 9 76 c-B-LGF-3 581 36 34 91 c-B-MLF-3 655 100 22 65 c-B-LGF-3 581 10 8 91 c-B-GPG-3 475 37 46 99 c B-LGF-3 581 22 18 83 c-B-GPM-3 549 15 16 50 c-B MGG-3 509 60 38 89 c-B-GPF-3 565 45 83 99 c B MGM-3 583 32 12 96 c-B-LPG-3 531 0 1 58 c-B-MGM-3 583 54 17 83 c-B-LPM-3 605 54 29 38 c-B-MGF-3 599 96 31 98 c-B-LPF-3 621 26 10 91 c-B-MGF-3 599 55 13 73 c-B-MPG-3 549 23 15 98 c-B-GHG-3 657 104 54 94 c-B-MPM-3 623 10 41 41 c-B-GHM-3 731 52 26 61 c-B-MPF-3 639 5 nd c-B-GHF-3 747 80 24 81 c-B-GVG-3 477 39 19 79 c-B LHG-3 713 119 70 85 c-B-GVM-3 551 33 34 66 c-B-LHM-3 787 173 66 73 c-B-GVF-3 567 36 6 28 c-B-LHF-3 803 224 64 75 c-B-LVG-3 533 158 64 82 c-B-MHG-3 731 107 29 93 c-B-LVM-3 607 75 64 83 c-B MHM-3 805 97 13 78 c-B-LVF-3 623 356 64 79 c-B-MHF-3 821 163 38 83 c-B-MVG-3 551 285 63 62 c-B-GLG-3 491 63 38 100 c-B-MVM-3 625 8 9 50 c-B-GLM-3 565 53 15 51 c-B-MVF-3 641 123 31 77 c-B-GLF-3 581 20 7 44 Table 3. Results for the cyclic peptides with the alkyne linker.

Spectral Data for betsylated c-Met-Leu-Phe-Linker compounds:
Trans-linker (c-B-MLF-1) .

1H NMR (CDC13r 300 MHz) : 8.32 (1 H, br) , 8.19 (1 H, dd, J =
8.0 and 1 . 7 Hz), 8.01 ( 1 H, dd, J= 8 . 5 and 1.7 Hz), 7.70-7. 59 (2 H, m), 7.34-7.22 (5 H, m), 6.91 (1 H, br), 6.66 (1H, br), 5.70-5.60 (1 H, m), 5.21-5.16 (1 H, m), 4.64-4.59 (2 H, m), 3.92-3.85 (3 H, m), 3.35-3.20 (2 H, m), 3.30 (1 H, dd, J = 14.0 and 4.7 Hz), 3.16 (1 H, dd, J = 13.9 and 9.3 Hz), 2.47-2.32 (3 H, m), 2.09-2.04 (3 H, m), 1.97 (3 H, s), 1.73-1.44 (3 H, m), 0.86 (3 H, d, J = 6.3 Hz), 0.81 (3 H, d, J = 6.3 Hz).
LC-MS : m/e : 671 (M+) Cis-linker (c-B-MLF-2) 1H NMR (CDC13r 300 MHz): 8.65 (1 H, J = 5.9 Hz), 8.05 (1 H, dd, J = 8. 9 and 1. 6 Hz) , 8.00 (1 H, d, J = 8. 1 Hz) , 7. 66-7.57 (2 H, m), 7.33-7.22 (3 H, m), 7.16 (2 H, d, J = 7.1 Hz), 6.71-6.68 (2 H, m), 5.72-5.56 (2 H, m), 5.01 (1 H, t, J = 7.3 Hz), 4.54 (1 H, dt, J = 8.7 and 4.9 Hz), 4.08-4.00 (2 H, m) , 3.94 ( 1 H, dd, J = 16. 4 and 7. 3 Hz), 3.67-3.56 (2 H, m) , 3.23 ( 1 H, dd, J = 14. 1 and 4. 8 Hz) , 3.00 ( 1 H, dd, J = 14.1 and 9.0 Hz) , 2.67-2.47 (2 H, m) , 2.36-2.11 (1 H, m), 2.09 (3 H, s), 2.07-1.99 (1 H, m), 1.92-1.82 (1 H, m), 1.61-1.52 (1 H, m), 1.49-1.41 (1 H, m), 0.93 (3 H, d, J
= 6. 5 Hz) , 0.87 (3 H, d, J = 6.3 Hz) LC-MS : m/e : 657 (M+).
Acetylene-linker (c-B-MLF-3) 1H NMR (CDC13r 300 MHz) : 8.32 (2 H, d, J = 8. 1 Hz) , 8.01 (1 H, d, J = 8.0 Hz), 7.72-7.60 (2 H, m), 7.49 (1 H, br), 7.31-7.20 (5 H, m), 6.80 (1 H, br), 4.80-4.76 (1 H, m), 4.42-4.36 (2 H, m), 4.13-3.95 (3 H, m), 3.45-3.40 (1 H, m), 3.29 (1 H, dd, J = 14.2 and 5.6 Hz), 3.14 (1 H, dd, J =
14. 1 and 10. 1 Hz) , 2.54-2.47 (3 H, m) , 2.12-2.08 (1 H, m) , 1.97 (3 H, s), 1.74 (2 H, t, J =7.6 Hz), 1.42-1.33 (1 H, m), 0.82 (3 H, d, J = 6.6 Hz), 0.78 (3 H, d, J = 6.6 Hz).
LC-MS : m/e : 655 (M+) Example 2 Removal of betsyl group of cyclotripeptides 1) in solution :
Potassium trimethylsilanolate (0.2 mmol) was added to a solution of 2-naphthalenethiol (0.2 mmol) in a deoxygenated mixture of THE and EtOH (1:1, 1 mL) at room temperature and the resulting mixture was stirred for 20 min. N-Bts-cyclotripeptide (0.1 mmol) was then added. The resulting mixture was stirred for 1 h and evaporated to dryness. The residue was purified by column to give the deprotected product with yields ranging from 77 to 86%.

2) on solid support :
Polystyrene-thiophenol Resin (0.2 mmol) was added to a solution of potassium trimethylsilanolate (0.2 mmol) in a deoxygenated mixture of THE and EtOH (1:1, 1 mL) at room temperature and the resulting mixture stirred for 20 min.
The solution was removed by filtration. The resin was washed with a deoxygenated mixture of THE and EtOH (1:1, 3 X 2 mL) and added to a solution of N-Bts-cyclotripeptide (0.1 mmol) in a deoxygenated mixture of THE and EtOH (1:1, 1 mL). The resulting mixture was stirred for 1 h. The resin was removed by filtration and washed with THE and EtOH (1:1 mixture, 2 X 2 mL). The filtrate was concentrated to give the crude product in quantitive yield.

Data for c-Met-Leu-Phe-Linker compounds:
Trans-linker (c-MLF-1) .

1H NMR (CDC13, 300 MHz) : 7.77 (1 H, d, J = 7.7 Hz), 7.30-7.14 (5 H, m), 6.65 (1 H, d, J = 7.4 Hz), 6.53 (1H, br), 5.56-5.64 (1 H, m), 5.32-5.22 (1 H, m), 4.03-3.95 (2 H, m), 3.79-3.68 (1 H, m), 3.57-3.35 (3 H, m), 3.12-3.02 (2 H, m), 2.96-2.86 (1 H, m), 2.61-2.50 (2 H, m), 2.24-1.98 (3 H, m), 10 2.10 (3 H, s), 1.78 (2 H, m), 1.55-1.39 (2 H, m), 0.86 (3 H, d, J = 6.6 Hz), 0.83 (3 H, d, J = 6.8 Hz).

LC-MS : We : 474 (M+) Cis-linker (c-MLF-2) 1H NMR (CDC13 & CD30D, 300 MHz) : 7.27-7.14 (5 H, m) , 5.80-5. 71 (1 H, m), 5.68-5.53 (1 H, m), 4.21-4.09 (2 H, m), 3.88 (1 H, dd, J = 14.0 and 6.0 Hz), 3.64 (1 H, dd, J = 14.0 and 7.3 Hz), 3.34-3.15 (5 H, m), 2.52 ( 2 H, t, J = 7.3 Hz), 2.07 (3 H, s), 2.00-1.86 (2 H, m), 1.53-1.15 (3 H, m), 0.80 (6H, d, J = 6.6 Hz).

20 LC-MS : m/e : 460 (M+).
Acetylene-linker (c-MLF-3) 1H NMR (CDC13, 300 MHz) : 7.92 (1 H, d, J = 8.8 Hz) , 7.34 (1 H, d, J = 9.2 Hz), 7.31-7.17 (5 H, m), 7.02 (1 H, t, J =
5.9 Hz), 4.21 (1 H, q, J = 8.0 Hz) , , 4.10-3.99 (2 H, m), 3.79 (1 H, dm, J = 15.5 Hz), 3.67 (1 H, dm, J = 16.0 Hz), 3.49-3.35 (3 H, m), 3.25 (1 H, dd, J = 8.8 and 4.3 Hz), 2.60-2.54 (2 H, m), 2.15-1.99 (1 H, m), 2.11 (3 H, s), 1.80-1.68 (2 H, m), 1.57-1.46 (2 H, m), 0.86 (6 H, d, J =

6.3 Hz) .

LC-MS : m/e : 458 (M+) Example 3 Preparation of N-Formyl-cyclotripeptides The free amine macrocycle (see example 2) was added to a mixture of formic acid (0.2 mL) and acetic anhydride (0.1 mL) and the reaction mixture was stirred for 15 min at room temperature, then for 5 min at 55 C and finally for 2h at room temperature. The reaction mixture was evaporated to dryness and purified by column chromatography to give the desired compounds in yields ranging from 81 to 100%
Data for formylated c-Met-Leu-Phe-Linker compounds:
Trans-linker (c-f-MLF-1) :

1H NMR (CDC13, 300 MHz): 8.72 (1 H, s), 7.92 (1 H, s), 7.38-7.22 (5 H, m), 6.78 (1 H, br), 5.83 (1 H, d, J =10.0 Hz), 5.68-5.58 (1 H, m), 4.96-4.89 (1 H, m), 4.02-3.68 (5 H, m), 3.34 (1 H, dd, J = 14.0 and 10.0 Hz), 2.78 (1 H, dd, J =
13.5 and 5.2 Hz), 2.67-2.51 (3 H, m), 2.42-2.31 (1 H, m), 2.18-2.04 (1 H, m), 2.06 (3 H, s), 1.99-1.53 (6 H, m), 1.03 (3 H, d, J = 6.0 Hz), 0.94 (3 H, d, J = 6.0 Hz).

LC-MS : m/e : 502 (M+) (84.2 %) Cis-linker (c-f-MLF-2) .

1H NMR (CDC13, 300 MHz) : 8.04 (1 H, s), 7.29-7.18 (5 H, m), 6.82-6.74 (1 H, m), 6.39 (1 H, d, J = 9.5 Hz), 6.16 (1 H, dd, J = .18.0 and 7.5 Hz), 6.94-6.85 (1 H, m), 4.80-4.72 (1 H, m), 4.24-3.68 (5 H, m), 3.50-3.43 (1 H, m), 2.87-2.79 (1 H, m) , 2.61-2.45 (3 H, m) , 2.14-2.01 (1 H, m) , 2.11 (3 H, s), 1.74-1.62 (1 H, m), 1.43-1.25 (3 H, m), 0.93-0.78 (6 H, m).

LC-MS : m/e : 488 (M+) .
Acetylene-linker (c-f-MLF-3) 1H NMR (CDC13, 300 MHz): 8.10 (1 H, s), 7.83 (1 H, br), 7.31-7.16 (5 H, m), 6.97 (1 H, br), 6.45 (1 H, br), 4.35-4. 01 (5 H, m) , 3.87-3.71 (2 H, m) , 3.38 (1 H, dd, J = 14. 5 and 5.0 Hz), 3.24-3.16 (1 H, m), 2.59-2.23 (3 H, m), 2.08 (3 H, s), 1.66-1.25 (4 H, m), 0.84 (6 H, t, J = 6.0 Hz).
LC-MS : m/e : 486 (M+) Example 4 Solid Phase Synthesis on the Kaiser Resin Anchoring Boc-amino acid to the resin :
To the Kaiser resin (2.0g, 0.95 mmol/g) was added a 0.2M
solution of N-Boc amino acid and 4-dimethylaminopyridine (0.25eq). After shaking for 5 min, diisopropylcarbodiimide (1.5 eq) was added and the reaction mixture was agitated for 16 h. The resin was washed with dichloromethane (3 X
30 mL), tetrahydrofuran (1 X 30 mL), methanol (1 X 30 mL), dichloromethane (1 X 30 mL), methanol (1 X 20 mL), tetrahydrofuran (1 X 30 mL), methanol (1 X 20 mL), dichloromethane (2 X 30 mL) and dried by nitrogen flow. The unreacted hydroxy group on the resin was then capped by reacting with acetic anhydride (5 mL) and diisopropyl-ethylamine (1 mL) in dichloromethane (20 mL) at room temperature for 2 h. The resin was washed and dried by the same procedure mentioned above. The substitution level was 0.2-0.3 mmol/g.

Formation of dipeptides (Performed on the Quest 21O T14):

25 % TFA in dichloromethane (20 mL) was added to the above resin (0.4 mmol, 2.0 g, 0.2 mmol/g) and agitated for 30 min. The resin was then washed with dichloromethane (3 X
30 mL) , methanol (1 X 20 mL) , dichloromethane (1 X 30 mL) , methanol (1 X 20 mL), dichloromethane (1 X 30 mL), methanol (1 X 20 mL), dichloromethane (2 X 30 mL) and dried by nitrogen flow.

A 0.2M solution of hydroxybenzotriazole and diisopropyl-carbodiimide in 60% dichloromethane/tetrahydrofuran was added to the N-Boc amino acid, followed by diisopropyl-ethylamine (1.5eq). The resulting mixture was stirred for 30 min at room temperature, and then transfered to the resin (200 mg on Quest 210TM) and agitated at room temperature for 30 min. Diisopropylethylamine (2.0 mmol) was then added and agitated until Kaiser test of an aliquot of the resin was negative(2 to 4 h). The resin was washed with dichloromethane (3 X 4 mL), tetrahydrofuran (1 X
4 mL), methanol (1 X 4 mL), dichloromethane (1 X 4 mL), methanol (1 X 4 mL), tetrahydrofuran (1 X 4 mL), methanol (1 X 4 mL), dichloromethane (2 X 4 mL) and dried by nitrogen flow.

Formation of tripeptides % TFA in dichloromethane (4 mL) was added to the Boc-protected dipeptide resin (0.04 mmol, 200mg g, 0.2 mmol/g) and agitated for 30 min. The resin was then washed with dichloromethane (3 X 4 mL), methanol (1 X 4 mL), dichloro-methane (1 X 4 mL), methanol (1 X 4 mL), dichloromethane (1 X 4 mL), methanol (1 X 4 mL), dichloromethane (2 X 4 mL) and dried by nitrogen flow.

A 0.2M solution of hydroxybenzotriazole and diisopropyl-carbodiimide in 60% dichloromethane/tetrahydrofuran was added to the N-Bts amino acid, followed by diisopropyl-ethylamine (1.5eq). The resulting mixture was stirred for 30 min at room temperature, and then transferred to the resin (200 mg on Quest 210TM) and agitated at room temperature for 30 min. The resin was washed with dichloromethane (3 X 4 mL), tetrahydrofuran (1 X 4 mL), methanol (1 X 4 mL), dichloromethane (1 X 4 mL), methanol (1 X 4 mL), tetrahydrofuran (1 X 4 mL), methanol (1 X 4 mL), dichloromethane (2 X 4 mL) and dried by nitrogen flow.
Mitsunobu reaction :

A 0.2M solution of 5-(tert-butoxycarbonylamino)-trans-2-penten-l-ol or N-tert-butoxycarbonyl-2-(2-hydroxyethoxy)-cinnamyl amine, and triphenylphosphine was added to the tripeptide resin (0.036 mmol, 180 mg, 0.2 mmol/g on the Quest 210TM) in anhydrous tetrahydrofuran, followed by diethyl azodicarboxylated (1.5eq). The mixture was agitated for 2 h and the resin was washed and dried by the same procedure mentioned above.

Cyclization of alkylated tripeptides The N-alkylated linear tripeptide (0.016 mmol, 80 mg) was treated with 25% TFA in dichloromethane (4 mL) for 30 min and washed with dichloromethane, methanol and dried by nitrogen flow.

Toluene(2 mL), acetic anhydride (1 mL) and diisopropyl-ethylamine (1 mL) were added to the above resin and agitated for 2 h. The resin was removed by filtration and washed with dichloromethane (3 X 4 mL). An aliquot of the the filtrate was analysized by LC-MS. The filtrate was concentrated and then diluted with ethyl acetate (15 mL) The solution was washed with iN hydrochloric acid (2 mL), saturated sodium bicarbonate (2 mL), brine (3 mL), dried and evaporated to give the crude product.

SAMPLE ID ISOLATED QUANTITY (MG) PURITY

c-B-MPG-1 5.9 (42%) Low c-B-MVG-1 4.4 (48%) Medium c-B-MGM-l 4.6 (32%) Low c-B-LPM-1 7.5 (50%) Low c-B-LLM-1 7.1 (46%) Good c-B-GVM-1 3.1 (22%) Low c-B-GLF-1 7.8 (81%) Good c-B-MVG-4* 2.4 (23%) Good c-B-MGM-4* 5.7 (34%) Low c-B-LPM-4* 3.3 (19%) Low c-B-LMM-4* 5.0 (29%) Medium c-B-GVM-4* 4.0 (25%) Low c-B-GLF-4* 2.9 (26%) Low *Nature of linker 4 is shown in Scheme 2.

Table 4. Library of Macrocyclic Tripeptides Synthesized on 10 the Kaiser Resin Using the Quest 21OTM:

Example 5 Synthesis of Betsylated Macrocyclic Tripeptides on Thio-ester Resin in IRORI MACROKANS':

Macrocyclic tripeptides were synthesized in MACROKANSTM
(160 mg of aminomethyl resin) following the same procedure as that given for the synthesis on solid support (Thioester Resin, see example 4) :

SAMPLE ID Quantity (mg) PURITY
c-B-GHG-1 7.6 (6%) Good c-B-GLF-1 16.3 (14%) Excellent c-B-GVM-1 20 (18%) Good c-B-LHF-1 43 (27%) Excellent c-B-LPM-1 26.7 (22%) Excellent c-B-LLM-1 20.6 (17%) Excellent c-B-MVG-1 10.5 (10%) Good c-B-MPG-1 6.4 (6%) Low c-B-GHG-4 12.4 (11%) Excellent c-B-GLF-4 12.4 (9%) Excellent c-B-GVM-4 9.3 (7%) Good c-B-LHF-4 21.8 (16%) Excellent c-B-LPM-4 29.1 (21%) Excellent c-B-LLM-4 25.8 (18%) Excellent c-B-MVG-4 37.5 (30%) Excellent c-B-MPG-4 30.3 (24%) Excellent Table S. Library of Macrocyclic Tripeptides Synthesized Example 6 Synthesis of Mesylated Macrocyclic Tripeptides on Thioester Resin in IRORI MINIKANSTM

Macrocyclic tripeptides were synthesized in MINIKANSTM (60mg of aminomethyl resin) following the same procedure as that given for the synthesison solid support (Thioester Resin, see example 4) SAMPLE ID Quantity (mg) PURITY
c-Ms-GLG-4 3 (9%) Low c-Ms-GLG-1 3 (12%) Low c-Ms-E (OMe) LG-4 1.9 (5%) Good c-Ms-E(Ome)LG-1 4 (13%) Good c-Ms-LPM-4 0.1 Good c-Ms-LPM-1 0.5 Low c-Ms-YLG-4 2 (5%) Good c-Ms-YLG-1 6 (18%) Good c-Ms-GLF-4 6 (16%) Good c-Ms-GLF-1 5 (15%) Good c-Ms-LLG-4 1 (3%) Low c-Ms-LLG-1 -- Low c-Ms-LLM-4 -- Low c-Ms-SLG-4 -- Good c-Ms-E(COOH)LG-4 13.3 * Good c-Ms-E(COOH)LG-1 21* Good *Unpurified Table 6. Library of Macrocyclic Tripeptides Synthesized SPECIFIC EXAMPLES OF BUILDING UNITS
Tether building blocks (type D, see figure 2b) The tether building blocks have the following formula: HO-Y-L-Z-PGz.

The three following tether building blocks 4-(tert-butoxycarbonylamino)-cis-2-buten-l-ol (Y=CH2, L=[Z]alkene, Z=CH2) and 4-(tert-butoxycarbonylamino)-2-butyn-l-ol (Y=CH2, L=alkyne, Z=CH2) and 5-(tert-butoxycarbonylamino)-trans-2-penten-l-ol (Y=CH2, L=CH2-[E]alkene, Z=CH2) were synthesized from commercial available cis-2-butene-l,4-diol, 2-butyne-l,4-diol and 3-amino-l-propanol respectively.

Preparation of 4-(tert-butoxycarbonylamino)-2-butyn-l-ol Dowex 50WX8-100 ion-exchange resin (53 g) was added to a suspension of 2-butyne-l,4-diol (153.9 g, 1.77 mol) and dihydropyran (250 mL, 2.66 mol) in dichloromethane (800 mL) at room temperature. The resulting mixture was stirred for 60 min and quenched with triethylamine (10 mL). The resin was removed by filtration. The filtrate was washed with a saturated aqueous solution of sodium bicarbonate (100 mL), brine (3 X 300 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure to give the desired monoprotected 2-butyne-l,4-diol with a yield of 50%.

To a solution of monoprotected 2-butyne-l,4-diol (20.4 g, 0.12 mol) and triphenylphosphine (40.9 g, 0.16 mol) in tetrahydrofuran (50 mL), hydrazoic acid (113 mL, 1.6 M in toluene, 0.18mol) was added at 0 C. Diisopropyl azodi-carboxylate (29.5 mL, 0.15 mol) was added dropwise to the solution whose temperature was around 0 C. The reaction was stirred for 30 min at 0 C and for 30 min at room temperature. Triphenylphosphine (40.9 g, 0.16 mol) was added at 0 C and the reaction was stirred overnight at room temperature. After addition of water (50 mL), the mixture was heated at 60 C for 4 h, 1N hydrochloric acid (140 mL) was added. After stirring for 1 h, brine (140 mL) and dichloromethane (500 mL) were added. The aqueous phase was washed with dichloromethane (3 X 100 mL). Potassium carbonate (16.5 g, 0.12 mol) was added, followed by a solution of di-tert-butyl dicarbonate (26.2, 0.12 mol) in tetrahydrofuran (100 mL). The reaction mixture was stirred for 18 h, then extracted with dichloromethane (1 X 300 mL, 2 X 50 mL). The combined organic extract was washed with brine (50 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure. The residue was purified by a dry-pack silica gel column to give the titled compound in 50% yield.

Preparation of 4-(tert-butoxycarbonylamino)-cis-2-buten-l-ol The title compound was synthesized from cis-2-butene-1,4-diol in an overall yield of 30% according to the procedure used for 4-tert-butoxycarbonylamino-2-butyn-l-o1 .

Preparation of 5-(tert-butoxycarbonylamino)-trans-2-penten-A solution of di-tert-butyl dicarbonate (382.8 g, 1.75 mol) in dichloromethane (1.6 L) was added to 3-amino-1-propanol (263.6 g, 3.51 mol) during 2 h. The reaction mixture was stirred for an additional 40 min and water (1 L) was added.

The organic phase was washed with water (3 X 500 mL),), dried over magnesium sulfate, filtered and evaporated under reduced pressure to give 3-(tert-butoxycarbonylamino)-1-propanol in 96% yield.

Dimethyl sulfoxide (321 mL, 4.5 mol) and triethylamine (941 mL, 6.75 mol) were added to a solution of 3-tert-butoxycarbonylamino-l-propanol (262.6 g, 1.5 mol) in dichloromethane (1.2 L) at 0 C. Sulfur trioxide pyridine complex (286.4 g, 1.8 mol) was added in 6 portions. The 10 reaction mixture was then stirred for 30 min at 0 C and for 30 min at room temperature. The reaction was cooled down to 0 C, quenched with 1N hydrochloric acid, washed with brine (2 X 500 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure to give 3-(tert-butoxycarbonylamino) propionaldehyde.

To a solution of the above crude aldehyde (1.5 mol) in acetonitrile (1.3 L), trimethyl phosphonoacetate (409.7 g, 2.25 mol) and lithium hydroxide (53.9 g, 2.25 mol) were added and stirred overnight at room temperature. The 20 reaction was quenched with water (50 mL). The acetonitrile solvent was removed by evaporation under reduced pressure.
The residue was then diluted with diethyl ether (800 mL), washed with 1N sodium hydroxide (3 X 300 mL), brine (2 X
500 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure to give the desired trans-unsaturated methyl ester.

Diisobutylaluminium hydride (1.12 L, 1.0 M in dichloro-methane, 1.12 mol) was added dropwise to a solution of this methyl ester (102.75 g, 0.445 mol) in dichloromethane (250 mL) at 00 C. The resulting mixture was stirred for an additional 1 h and then poured slowly into a 1M tartaric acid aqueous solution (1.4 L), extracted with dichloro-methane (3 X 500 mL) . The combined organic phase was dried over magnesium sulfate, filtered and evaporated under reduced pressure. The residue was purified by dry-pack silica gel column to give the titled compound with a yield of 40% for the three steps.

Amino-acid building block (type A and B, see figure 2a) a The N-Boc amino acids are commercial available except N -Boc-Nim-Doc-histidine which was preparated by the method described below.

Preparation of Noc-Boc-Nlm-Doc-histidine A solution of 2,4-dimethyl-3-pentanol (83.2 g, 0.72 mol) and triethylamine (125 mL, 0.90 mol) in toluene (300 mL) was added slowly (30 min) to a solution of phosgene (531 mL, 20% in toluene, 1.07 mol) in toluene (531 mL) at 0 C. The mixture was stirred for an additional 30 min at the same temperature. Ice-cold water (500 mL) was added and the organic phase was washed with ice-cold water (2 X
100 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure. The residue was then distilled under reduced pressure (6 cm of Hg, 33-35 C) to give Doc-Cl as a colorless oil (92 g, 72%).

A solution of Doc-Cl (57.9 g, 0.32 mol) in tetrahydrofuran (250 mL) was added slowly to a solution of Na-Boc-histidine (69 g, 0.27 mol) and potassium carbonate (41.1 g, 0.28 mol) in water (350 mL) at 0 C. The resulting mixture (pH=10) was stirred for 2 h at the same temperature and for 1 h at room temperature. Water (150 mL) and hexane (200 mL) were added to the reaction mixture. The separated aqueous phase was washed with a mixture of diethyl ether and hexane (1:1; 3 X
200 mL), acidified with 20% citric acid aqueous solution to pH 2-3, and then extracted with dichloromethane (3 X
200 mL) . The combined dichloromethane solution was washed with brine (200 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure to give the crude N~-Boc-Nim-Doc-histidine in quantitive yield.

Building blocks of type C (see figure 2b) N-Betsyl protected amino acids (Bts-AA1) were synthesized by the reaction of amino acids with Betsyl chloride (benzothiazole-2-sulfonylchloride) which was obtained from mercaptobenzothiazole and chlorine.

Preparation of N-Betsyl amino acid (Bts-AA1OH) Chloride gas was bubbled into a solution of acetic acid (250mL) in water (500 mL) at 5 C until an orange precipitate was formed in good quantity. A solution of mercaptobenzothiazole (0.7 mol) in aqueous acetic acid (750 mL, 33% in water) was added in portions to the above reaction mixture in a period of 3 hours. The reaction mixture was stirred for 1 h, filtered at 0 C then washed with cold water. The solid was dissolved in cold dichloromethane (500 mL) and washed with cold brine (2 X
100 mL), cold saturated sodium bicarbonate (100 mL), brine (100 mL), dried over magnesium sulfate, filtered and evaporated at 10 C under reduced pressure. The solid was then washed with cold diethyl ether (100 mL), cold acetonitrile (100 mL), filtered and pumped to give betsyl chloride (benzothiazole-2-sulfonylchloride).

To a solution of amino acid (0.11 mol) in 0.25 N aqueous sodium hydroxide (0.08 mol) at room temperature (initial pH
around 9.5), betsyl chloride (0.1 mol) was added. The resulting mixture was stirred vigorously for 18 h. The pH
of the reaction was adjusted between 9.5 to 10.0 with 1.0 N
aqueous sodium hydroxide during the reaction progress. The reaction mixture was washed with diethyl ether (3 X 50 mL).
The aqueous phase was then cooled to 0 C, acidified to pH
1.5-2.0 with 6 N HC1, and extracted with ethyl acetate (3 X
100 mL). The combined ethyl acetate solution was dried over magnesium sulfate, filtered and evaporated under reduced pressure to give the desired compound in 74-85% yield.

Building blocks of type E (see figure 2b) These building blocks correspond to building blocks of type C which have been alkylated using Mitsunobu reaction conditions with the building blocks of type D. To be able to carry out this alkylation, the acid functional group of C must be protected. The protecting group used is finally removed to get the desired compounds Preparation of N-alkylated N-Betsyl amino acid Dihydrofuran (90 mmol) and pyridinium p-toluenesulfonate (1.5 mmol) were added to a suspension of N-Betsyl amino acid (30 mmol) in dichloromethane (50 mL) at 0 C. The resulting mixture was stirred for 15 min at 0 C and for 60 min at room temperature. The reaction mixture was diluted with diethyl ether (150 mL), washed with saturated aqueous sodium bicarbonate (20 mL), brine (20 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure to give the tetrahydrofuranyl ester of amino acid.
A mixture of this ester (30 mmol), an alcohol (type D
building block) (i.e. 4-(tert-butoxycarbonylamino)-cis-2-buten-l-ol, or 4-(tent-butoxycarbonylamino)-2-butyn-l-ol, or 5-(tert-butoxycarbonylamino)-trans-2-penten-l-ol)) (43.5 mmol) and triphenylphosphine (49 mmol) were suspended in toluene (20 mL) and azeotropically distilled three times in vacuum.
The residue was dissolved in tetrahydrofuran (40 mL).
Diisopropyl azodicarboxylate (43.5 mmol) was added at 0 C.
After stirring for 15 min at 0 C and for 30 min at room temperature, 1N hydrochloric acid (30 mL) and methanol (30 mL) was added and stirred for an additional 60 min.
After removal of the organic solvents by evaporation, the aqueous phase was diluted with water (30 mL), the pH of the medium was adjusted to 12 with potassium carbonate, washed with diethyl ether (3 X 60 mL), and then acidified to pH 2-3 with 1N hydrochloric acid, extracted with dichloromethane (3 X 200 mL). The combined dichloromethane solution was washed with brine (100 mL), dried over magnesium sulfate, filtered and evaporated under reduced pressure to give the desired alkylated N-Betsyl amino acid in the overall yield of 68-89%.

Claims (15)

1. A macrocyclic compound of the formula (I):
and salts thereof;

where part (A) is a bivalent radical having its -NH- group linked to the carbonyl group of part a -(CH2)y- bivalent radical, or a covalent bond;
- where part (B) is a bivalent radical having its -NH- group linked to part (A), a -CH2)z- bivalent radical, or a covalent bond;

- where part (C) is a bivalent radical having its -NH- group linked to part (B), a -(CH2)t- bivalent radical, or a covalent bond;

- where part (T) is a - Y - L - Z - radical having its Y
group linked to the -NX- of formula (I) and its -Z- group linked to the carbonyl group of part (c); and - where X is a monovalent group selected from the group consisting of: -SO2-Ar, -SO2-CH3, -SO2-CF3, -H, -CHO, -CO-CH3, -CO-Ar, -CO-R, -CO-NHR, -CO-NHAr, -CO-O-tBu, -CO-O-CH2-Ar, wherein:
.cndot. Ar being an aromatic group, substituted aromatic group or a heteroaromatic group, .cndot. a being an integer selected from the group consisting of 0, 1 and 2, .cndot. R being a monovalent group -(CH2)n-CH3 or -(CH2)n-Ar with n being an integer from 1 to 16, R0, R1, R2, R3 and R4 being independently selected from the group consisting of: -H, -CH3, wherein the * indicates the bond location of R0, R1, R2, R3 and R4 to the rest of the structure;

R1, R2 and R3 being optionally protected by protecting groups (PG1), (PG2) and (PG3) respectively, said protecting groups being those used for orthogonal protections in peptide synthesis;

R5, being a monovalent radical selected from the group consisting of: -H, -SO2-CH3, -SO2-CF3, -CHO, -COCH3, -CO-Ar, -CO-R, -CO-NHR -CONHAr, -COO-tBu and -COO-CH2-Ar, wherein R
and Ar are defined as above, R8 being -OH or -NH2, where Y is a bivalent group -CH2-;
where Z is a bivalent group -NH- or -O-;

wherein x, y, z and t are integers being each independently 0, 1 or 2;

wherein L is a bivalent radical having the formula:
-(CH2)d-A-(CH2)j-B-(CH2)e-, d being an integer from 0 to 5, e being an integer from 1 to 5, j being an integer from 0 to 5, when j is 0, A
or B is present, with A and B being independently selected from the group consisting of:

-O-, -NH-, -NR- wherein R is defined as above, -S-, -CO-, -SO-, -CO-O-, -O-CO-, -CO-NH-, -NH-CO-, -SO2-NH-, -NH-SO2-,-CHOH-, -CH=CH- with the configuration Z or E, -C.ident.C-, and with the substituent -G2- in a 1,2; 1,3 or 1,4 position, G1 being selected from the group consisting of:

-O-, -NH-, -NR- wherein R is defined as above, -S-, -CH=CH- with a z configuration, and -CH=N-; and G2 being selected from the group consisting of:

-O-, -NH-, and -NR- wherein R is defined as above.

2. A macrocyclic compound according to claim 1, wherein said compound is of formula (8):

where L, Z, R, R1, R2, R3, (PG1), (PG2) and (PG3) have the same meanings as given in claim 1.

3. A macrocyclic compound according to claim 1, wherein said compound is of the formula (9):

where L, Z, R, R1, R2 and R3 have the same meanings as given in claim 1.

4. A macrocyclic compound according to claim 1, wherein said compound is of the formula (10):

where L, Z, R1, R2, R3, (PG1), (PG2) and (PG3) have the same meanings as given in claim 1.

5. A macrocyclic compound according to claim 1, wherein said compound is of the formula (11):

where L, X, Z, R1, R2, R3, (PG1), (PG2) and (PG3) have the same meanings as given in claim 1.

6. A macrocyclic compound according to claim 1, wherein said compound is of the formula (12):

where L, Z, X, R1, R2 and R3 have the same meanings as given in claim 1.

7. A macrocyclic compound according to claim 1, selected from the group consisting of:

8. A macrocyclic compound according to claim 1, wherein part (T) is selected from the group consisting of:

wherein NH- indicates the site of a covalent bond to part (C), while the arrow indicates a covalent bond to N(X) in formula (I).

9. A process for preparing a compound of the formula (I) as claimed in claim 1, comprising the steps of:

a) preparing by coupling a first building block deriving from natural or synthetic amino-acids, said first building block being of the formula:

wherein x, X, R1, part (A), part (B), and part (C) are defined as in claim 1, Sp is and P is -CH3 or -CH2-Phenyl when the coupling is carried out in liquid phase, and Sp is and P is polystyrene or methoxypoly(ethyleneglycol) when the coupling is carried out in solid phase;

b) coupling the first building block prepared in step a) with a second building block hereafter called "tether", of the formula:

H-Y-L-Z-PG z wherein Y, L and Z are defined as in claim 1 and PG z is a protecting group;

c) removing the protecting group PGz from the compound obtained in step b); and (1) carrying out a macrocyclization of the unprotected product obtained in step c) and a cleavage if the above mentioned steps (a) and (b) were carried out in a solid phase, in order to obtain the requested compound of the formula (I).

10. A process according to claim 9, wherein when A, B or C is Arg, the process further comprises the steps of a)utilizing a suitably protected ornithine (Orn) residue as a surrogate for Arg, b)carrying out a selective deprotection of the protecting group on the Orn side chain, and c)reacting with an appropriately protected guanylating reagent to provide a protected Arg element.

11. A process for preparing a compound of formula (8) as defined in claim 2, comprising the steps of:

a) coupling an amino-acid of the formula (A):
wherein (PG.alpha.) is an amine protecting group and R3 and PG3 are defined as in claim 1, either in a solid or a liquid phase, with a compound of the formula:

H-Sp-P
wherein Sp and P are as defined in claim 9, in order to obtain a compound of the formula (1):

b) removing the amine protecting group PG.alpha. from the compound of the formula (1) to obtain the corresponding compound of the formula (2):

c) coupling the compound of the formula (2) with another amino-acid of the formula (B):
wherein PG.alpha. is defined as above and R2 and PG2 are defined as in claim 1, in order to obtain a compound of the formula (3):

d) removing the amine protecting group PG.alpha. from the compound of the formula (3) to obtain the corresponding compound of the formula (4):

e) either coupling the compound of the formula (4) with a further amino-acid of the formula (C):

wherein R is -(CH2)n-CH3 or -(CH2)n-Ar with n ranging from 1 to 16, in order to obtain a compound of the formula (5):

and coupling said compound of the formula (5) under Mitsunobu conditions with an alcohol of the formula (D):

HO-CH2-L-ZPG z (D) wherein L and Z are defined as in claim 1 and PG z is a protecting group, in order to obtain the compound of the formula (6):

or coupling the compound of the formula (4) with a compound of the formula (E):

wherein Z, R, L, R1, PG1 and PG z are defined as above, in order to obtain directly the compound of the formula (6);

f) removing the protecting group PG z from the compound of the formula (6) to obtain the corresponding compound of the formula (7):

and g) carrying out a macrocyclisation of the compound of the formula (7) and a cleavage if the coupling steps were carried out in the solid phase, in order to obtain the requested compound of the formula (8).

12. A process for preparing a compound of the formula (9) as defined in claim 3, which comprises the steps defined in claim 11 and a further step which consists in the removal of the protecting group PG1, PG2, PG3 of the compound of formula (8) as defined in claim 2 to yield the requested compound of formula (9).

13. A process for preparing a compound of formula (10) as defined in claim 4, which comprises the steps defined in claim 11 and a further step which consists in the cleaving of the sulfonamide portion of the compound of formula (8) to yield the requested compound of formula (10) with a free amine group.

14. A process for preparing a compound of formula (11) as defined in claim 5, which comprises the steps defined in claim 13 and a further step which consists in coupling the free amine of the compound of formula (10) with an acid of formula HX, wherein X has the meaning given in claim 1, to yield the requested compound of formula (11).

15. A process for preparing a compound of formula (12) as defined in claim 6 which comprises the steps defined in claim 14 and a further step which consists in cleaving the orthogonal protecting groups PG1, PG2 and PG3 of the compound of formula (II) to yield the requested compound of formula (12).