AMINO ACID DERIVATIVES TECHNOLOGY OF THE INVENTION The present invention relates to the new side chain protected amino acid derivtives having the general formula (I) and the use thereof for the preparation of peptide by the classical liquid phase method. wherein R1 may represents -CH2CH2CH2CH2NH-, -CH2CO- or -CH2CH2CO-, and R2 may represents phenylthioethyloxycarbonyl(Ptc), phenylsulfonylethyloxycarbonyl (Psc), phenyith ioethyloxy(OPte) or phenylsulfonylethyloxy(OPse), and R3 may represents hydrogen or a-amino protecting group.

According to the present invention, these amino acid derivatives can be used for the synthesis of various pepLides, since they have high stability but also good reactivity under the process.

BACKGROUND OF THE INVENTION Peptides can be obtained by i) extracting from natural products, ii) DNA recombination technique, iii) chemical synthesis, but, among them i) and ii) have the limits, for example the low yield of active extract, the uncertainty of the identification of purity and the difficulty of the removal of impurities from microorgaism. Thus, the chemical synthesis has been widely used for larger scale commercial production of peptides, and in parallel with the advances in the new methodology of it.

In general the chemical synthesis is categorized to classical liquid phase method doing on solution and solid phase method using insoluble polymer.

The latter method is not adjustable for mass production of peptides, since it

has a few drawbacks particularly; i) side chains of the amino acids which target peptide is composed of have to be fully protected, ii) the process is carried out by using excess of amino acids under limited coupling condition, iii) it is difficult to remove the impurities builded up in big peptides, iv) a coupling can not be unexpectedly completed, probably due to the folding of the growing peptide, v) after completion of the polypeptide chain, cleavage of the resin reduce the quantity of the product deeply, vi) the resins can not be loaded too heavily with the first residue, vii) the resin, amino acid derivatives, reagent, and solvents for solid-phase technique are all quite expensive.

The former method is more likely to be used for the preparation of larger quantities and higher qualities of peptides, since i) side chains of the amino acids can be minimally protected, ii) various coupling methods can be freely choosed, iii) growing peptide can be purified at any step, iv) quantity of the reactant can be controlled unrestrictly.

However, in the case of long chain peptide, for example residues 25 to 50, the liquid phase method has the limits on preparing the high quality of peptide largely because of i) time-consuming process, ii) possibility of the side reaction, iii) low-efficiency of the reaction due to solubility, iv) difficulty of the purification of final peptide.

In this point, it is valuable and requisite today to develope the new amino acid derivatives and the process useful for larger scale preparation of peptide with high purity and in good yield based on liquid phase method.

SUMMARY OF THE INVENTION The invention provides new procedure to prepare high quality of peptides such as calcitonin efficiently by liquid phase synthesis, combined with conventional segment condensation of the fragments obtained by stepwise coupling with Boc-protected amino acids using coupling agents(DCC, HOBT) or active esters Also, the invention provides new methodology for the preparation of peptide

using newly developed side chain and C-terminal protecting groups, based on liquid phase synthesis.

The object of the invention is to provide new method for obtaining calcitonin by the use of newly side chain protected amino acid derivatives or the salts having the general formula (I). wherein R1 may represents -CH2CH2CH2CH2NH-, -CH2CO- or -CH2CH2CO-, and R2 may represents phenylthioethyloxycarbonyl(Ptc), phenylsu Ifonylethyloxycarbonyl (Psc), phenylth ioethyloxy(OPte) or phenylsulfonylethyloxy(OPse), and Rs may represents hydrogen or a-amino protecting group.

Another object of the invention is to provide new methodology to prepare peptide using above mentioned amino acid derivatives.

DESCRIPTION OF THE INVENTION According to the invention the utility of newly developed amino acid derivatives is demonstrated by the synthesis of peptides. The synthesis is based on the strategy of segment condensation which has obvious advantages in the synthesis of longer peptide chain. This methodology, however, has the likely racemization of the activated C-terminal residue of the carboxyl component. To reduce the degree of racemization, following methods are recommended; i) good selection of the activated carboxyl residue: glycine and proline are favorable, ii) controle of the reaction condition: low polarity solvent, neutral pH, low temperature, iii) appropriate selection of the mothod for activating the carboxylic acid component, iv) use of a-alkoxycarbonyl protected amino acids in the coupling reactions.

The invention is intended to give the efficient production of calcitonin by

the process, considering the points mentioned above. In accordance with the invention, there is provided the methodology useful for larger scale synthesis of calcitonin.

To clarify the superiority of the invention, the process for preparing salmon calcitonin described below and newly developed amino acid derivatives will now be explained. i s-Lys-Leu-Gln-Thr-Tyr-Pro-Arg-Thr-Asn-Thr-Gly-Ser-Cly-Thr-Pr o-NH2(1, 7-disulfide) (salmon calcitonin) H-Ser-Gly-Thr-Pro-NH2(29-32) Fragment 1 Boc-Arg-Thr-Asn -Thr-Gly-OH(24-28) Fragment 2 Boc-Leu -GI n-Thr-Tyr-Pro-OH(1 9-23) Fragment 3 Boc-Leu-His-Lys(Psc)-OH(1 6-18) Fragment 4 Boc-Lys(Psc)-Leu-Ser-Gln-Glu(OPse)-OH91 1-15) Fragment 5 H-Ser-Thr-Cys(Acm)-Val-Leu-Cly-ON se TFA(5-1 0) Fragment 6 Boc-Cys(Acm)-Ser-Asn-Leu-OH(1-4) Fragment 7 According to the invention, fragments 1 to 7 used in the synthesis of salmon calcitonin by the segment condensation are prepared by the use of only Boc group which is common, inexpensive, and simple to blocking and deblocking, differing from the other methodologies (example: JP 6-16694A) using various groups for the temporary masking of a-amino groups. Size and number of the fragments are optimized to reduce the susceptiblity of racemization; firstly, glycine or proline are selected as C-terminal residue of segments. In particular, new side chain protected amino acids are introducecl to synthesize the fragments for the preparation of larger quantities and higher qualities of salmon calcitonin. The procedure for preparing salmon calcitonin by segment condensation based on the invention is represented in the followig diagram 1.

Diagram 1

In the cases of lysine, glutamic acid, arginine, histidine, asparagine, etc., active side chains have to be protected to prevent blanching the chain in the peptide synthesis, generally. And the blocking group applied for this purpose should be unaffected during the coupling step and the removal of a-amino protecting group, and deblocked usually only at the end of the chain building process.

Selection of the side chain protecting group plays important role in the design for the synthethic route of salmon calcitonin, since it contains glutamic acid with siden carboxyl group and lysine with side amino group which have to be protected semipermanently till the completion of peptide chain. A classical approach, the use of t-butyl or benzyl group for the protection of side carboxyl function of glutamic acid and of benzyloxycarbonyl(Z) or t-butyloxycarbonyl(Boc) or trityl(Trt)group for the protection of side amino function, is still practiced mainly. Yet, there are certain limitations inherent in the groups; the methods for deblocking, catalytic hydrogenation and acidolysis, have susceptibility of side reaction and are time consuming.

To solve the problems, the invention is intended to develope new base-labile side chain protecting group which is easy to introduce, stable during coupling, and readily removed under mild and selective conditions in combination with Boc used for the transient protection of the a-amino function. As a result, Pse and Pscl groups are exploited to the protection of the side chain of glutamic acid and lysine, respectively. These groups without negative inductive effect from para substituent of phenyl group are stable not only under acidolysis and catalytic hydrogenation, but also under weak basic coupling condition, nevertheless these are readily removed by addition of piperidine within shorter time. These group protected amino acid derivatives, namely, Boc-Lys(Psc)-OH DCHA½5), Boc-Asp(OPse) -OH DCHA(8), Boc-Glu(OPse)-OI DCHA(9) are newly introduced to the synthesis of calcitonin. These compounds are prepared by the procedure as shown in diagram 2; E-amino function of lysine is protected by the addition of

phenylthioethylchloroformate(3) whilst the groups are chelated to copper(ll), followed by the oxidation. - and carboxyl function of aspartic and glutamic acid are blocked by the addition of phenylthioethanol, followed by oxidation.

Diagram 2.

According to the invention, p-nitrophenylsulphonylethyl(Nse) group is newly employed as the masking group of C-terminal of fragment 6 and 7. In selecting blocking group of C-terminal, It should be considered that the group is stable under coupling and removal of the a-amino protecting the side chain protecting group, too. So, it is intended to utilize the Nse group known in the art(Samukov, V. V. Tetrahedron Lett 35 1994, 7821 : US pat. 5,527,881) for protecting C-terminal, which is selectively removal by base, and stable under the acidolysis and the catalytic hydrogenation.

The invention will now be illustrated by means of the following non limiting examples.

EXAMPLE All the amino acids in the following description have L-configuration unless otherwise indicated. Melting points were taken on a Buch apparatus. Optical rotations were measured on a Jasco DIP 1000. HPLC: Hewlett pakard 1100.

FT-IR: Jasco 300F. Atomic Absorption Spectroscopy(AAS): Shimadzu AA-6601F. UV: Shimadzu UV-265. TLC was done on silicagel 60 F-254 precoated plates (Merck); eluents: 1 )ethyl acetate(EtOAc)/pyridine/acetic acid(AcOH)/water=42/14/6.6/1 2)n-BuOH/water/AcOH=4/1/4 3)acetonitrile(AcCN)/AcOH/water=8/0.2/2 4)AcCN/water/TFA/AcOH=20/5/0,1 5)CHCl3/MeOH/AcOH=95/5/3 6)CHCl3/MeOH/AcOH=90/10/3.

The abbreviations used in the description have the following meanings; Acm: acetamidomethyl Boc: t-buthyloxycarbonyl Bz: benzyl DCC: dicyclohexylcarbodi imide DCHA: dicyclohexylamine DMAP: dimethylaminopyridine DMF: N,N'-dimethylformamide EDTA: ethylenediaminetetraacetic acid Et: ethyl HOBT: hydroxybenzotriazole NMM: N-methyl morpholine Nse: p-nitrophenylsulphonylethyl OPse: phenylsulphonylethyloxy OPte: phenylthioethyloxy pfp: pentafl u orophen yl Psc: phenylsulphonylethyloxycarbonyl Pse: phenylsulphonylethyl Ptc: phenylthioethyloxycarbonyl

Pte: phenylthioethyl Su: succinimide Tce: trichloroethyl Tcp: trichlorophenyl TEA: triethyl amine TFA: trifluoroacetic acid C: cysteine E: glutamic acid C: glysine H: histidine K: lysine L: leucine N: asparagine P: proline Q: glutamine R: arginine S: serine T: threonine V: valine Y: tyrosine Example 1. preparation of amino acid derivatives a) H-Lys(Ptc)-OH(4) A suspension of 20.1 g of lysine hydrochloric acid salt and 1 2g of copper basic carbonate in 250mL of water was boiled for 30min, filtered, and washed with 30mL of water. To the filtrate 1 25mL of dioxane and 55mL of 2N sodium hydroxide were added, and cooled in ice bath. Then the solution of 21.7g of 2-phenylthioethyl chloroformate in 50mL of dioxane and 50mL of 2N sodium hydroxide were added to the mixture dropwise within 1.5 hr with stirring. After additional stirring for 2 hr, the mixture was filtered, and washed with 1 SOmE of water, 1 50mL of acetone, and 50mL of ether, successively. Collected precipitat was dissolved in 500mL of 2N hydrochloric acid. To the mixture a suspention of 30g of EDTA in 1L of water was added with stirring. Then the mixture was acidified to pH 4, washed with water, and dried on air to give 26g(77%) of the desired compound 4 as white powder. m.p.: 255-2590C TLC: Rf=0.65 (eluent 3) [a3g) +12.9 (20"C, 0.5N HCI) HPLC: purity 100%, Rt=19.5min IR(KBr, cm 1): 3343, 2947, 1683, 1578, 1533, 1418, 1325, 1236, 734 b) Boc-Lys(Psc)-OH(5)

To the mixture of 19.6g of 4, 12.5g of potassium carbonate, and 350mL of water-i-propanol-DMF mixture(4:2:1, v/v), 16mL of Boc2O was added with stirring at 45-500, and stirred for additional 3 hr. The mixture was concentrated to 1/2 of volume, diluted with 500mL of water, and washed with 1 50mL of ether. 200mL of EtOAc was added to aqueous layer, followed by acidification to pH=1.5. More 1 50ml of EtOAc was added, and organic layer was seperated from the mixture, and washed with 150mL of water and 100mL of brine, and dried under anhydrous Na2SO4. Evaporation of the filtrate gave 26g of oil. The oil was dissolved in 300mL of acetone. And 1 5ml of 0.3M sodium molibdate and 14mL of hydrogen peroxide were added to the solution.

After 1 hr, the mixture was stirred for 5 hr at 500C, and evaporated. The residue was diluted with 300mL of water and 300mL of EtOAc, and organic layer was separated, and washed with 1 50mL of water, 1 50mL of 0.5N hydrochloric acid, and 100mL of brine, successively. Then the solution was dried unser anhydrous sodium sulfate, evaporated, and solidified by addition of DCHA. The precipitate formed was filtered, and dried in vacuo to give 36.5g(95%) of 5 as white powder. m.,.: 109-112"C TLC: Rf=0.40 (eluent 5) (a)D: +7.2 (20"C, 10% AcOH) HPLC: purity 100%, Rt=21.4min IR(KBr, cm1): 3393, 2933, 2858, 1698, 1636, 1560, 1398, 1318, 1254,1149, 1051, 728, c) H-Asp(OPte)-OH(6) 1 3.3g of aspartic acid was dissolved in 90mL of dimethoxyethane, then 1 OmL of concentrated sulfuric acid and 40mL of 2-phenylthioethanol were added to the mixture. The mixture was stirred until clearness, then left for 2 day at room temperature. After evaporation a solution of 30g of sodium acetate in 300mL of water was added to the residue with vigorously stirring.

White precipitate formed was filtered, washed, and dried on air to afford

14.6g(54%) of 6 m.p.: 21 5-21 70C TLC: Rf=0.80 (eluent 2) [α]D: +21.2 (220C, 1N HCI) HPLC: purity 100%, Rt=17.6min IR(KBr, cm-1): 3123, 2379, 2306, 1739, 1636,1416, 1343, 1135, 730, 688 d) Boc-Asp(OPse)-OH DCHA(8) To the mixture of 1 4.0g of 6, 8.4mL of TEA, and 50mL of DMF, 1 5mL of Boc2O was added with stirring at 45-50°, and stirred for additional 3 hr. The mixture was diluted with 500mL of water, and extracted with 500mL of 5% potassium hydrogen sulfate. The organic layer was washed with 2 X 250mL of 5% potassium hydrogen sulfate and 200mL of brine, and dried under anhydrous sodium sulfate. After filtration, the filtrate was evaporated to oil.

The oil was dissolved in 250mL of acetone. And 13mL of 0.3M sodium molibdate and 12mL of hydrogen peroxide were added to the solution. After 1 hr, the mixture was stirred for 5 hr at 500C, and evaporated. The residue was diluted with 250mL of water and 250mL of EtOAc, and organic layer was separated, and washed with 150mL of water, 150mL of 0.5N hydrochloric acid, and finally 100mL of brine. Then the solution was dried under anhydrous sodium sulfate, evaporated, and solidified by adding DCHA. The precipitate formed was filtered, and dried in vacuo to give 28.8g(95%) of 8 as white powder. m.p.: 142-1440C TLC: Rf=0.20 (eluent 5) [α]D: -5.4 (23°C, 10% AcOH) HPLC: purity 100%, Rt=26.5min IR (KBr, cm-1): 3397, 2937, 2866, 1740, 1708, 1584, 1489, 1397, 1318, 1149 e) H-Glu(OPte)-OH(7) The compound 7 as white powder was obtained by the same procedure as

described in c) with an yield of 55%. m.p.: 182-1830C TLC: Rf=0.55 (eluent 2) [α]D : +17.65 (20°C, 0.5N HCl) HPLC: purity 100%, Rt=18.7min IR(KRr, cm-1): 2955, 1726, 1586, 1508, 1421, 1202, 733 f) Boc-Glu(OPse)-OH DCHA(9) The compound 9 as white powder was prepared by the same procedure as described in d) with an yield of 92%. m.p.: 155-157°C TLC: Rf=0.36 (eluent 5) [α]D: -5.8 (20°C, 10% AcOH) HPLC: purity 100%, Rt=21.5min IR(KBr, cm-1): 2938, 2857, 1733, 1701, 1637, 1560, 1449, 1399, 1297,1141, 1085, 727, 686 Example 2 Synthesis of salmon calcitonin a)H-Ser-Gly-Thr-Pro-NH2(fragment 1, 10) Fragment 1 (purity>99%, Rt=6.54min: HPLC) as white powder was obtained by the conventional stepwise coupling using active esters with an overall yield of 75% coupling/ reactant 1 reactant 2 product yield Rf deblokinn Boc-Thr-OPfh H-Pro-NH2 HCl H-T-P-NH2 TFA 95# active ester/TFA 1)0.13 17.0g 6.2g 17 (12.4g) Boc-Gly-OPfp H-G-T-P-NH2 TFA 95% 17 12.0g active ester/TFA 1)0.09 13.6g 18 (14.0g) Boc-Ser-OPfp H-S-G-T-P-NH2 TFA 85% 18 14.0g active ester/TFA 2)0.17 14.8g 10 (13.0g) b) Boc-Arg-Thr-Asn-Thr-Gly-OH(fragment 2, 11) Fragment 2(purity>99%, Rt=1 2.6min : HPLC) as white powder was obtained by the stepwise synthesis using acive esters or condensing agents (DCC, HOBT) well known, followed by catalytic(Pd-C) reduction for deblocking of Benzyl group with an overall yield of 59%. coupling/ reactant1 reactant 2 product yield Rf debloking Boc-Thr-OH H-Gly-OBz DCC, HOBT/ H-T-G-OBz TFA 90% 1)0.32 9.6g Ts()H 3.6g TFA 19 (14.0R) Boc-Asn-OH r)CC, HOBT/ H-N-T-G-OBz TFA 86% 19 13.8g 1)0.17 9.4g TFA 20 (15.6g) Boc-Thr-OPfp H-T-N-T-G-OBz TFA 90% 20 14.6g active ester/TFA 1)0.20 12.4g 21 (15.6g) Boc-Arg-OH Boc-R-T-N-T-G-OBz TFA 100% 21 15.6g active ester 1)0.40 8.2g 22 (22.6g) Boc-R-T-N-T-G-OH TFA 84% 22 22.6g Pd-C, H2 1)0.17 11 (14.4g) c) Boc-Leu-Gln-Thr-Tyr-Pro-PH(fragment 3, 12) Fragment 3(purity>99%, Rt=1 8.9min: HPLC) as white powder was obtained by the conventional stepwise coupling using condensing agents (DCC, HOBT), followed by base catalized hydrolysis and catalytic(Pd-C) reduction with an overall yield of 49%.

coupling/ reactant1 reactant2 product yield Rf debloking quantita Boc-Tyr(Bz)-OH DCC,HOBT/ H-Y(Bz)-P-OEt TFA H-Pro-OEt 9.0g tive 1)0.10 15.0g TFA 23 (26.0g) quantita Boc-Thr-OH DCC,HOBT/ H-T-Y(Bz)-P-OEt TFA 23 26.0g tive 1)0.10 9.5g TFA 24 (30.0g) Boc-Gln-OH DCC,HOBT/ H-Q-T-Y(Bz)-P-OEt TFA 70% 24 30.0g 1)0.37 9.8g TFA 25 (21.0g) Boc-Leu-OH DCC,HOBT/ Boc-L-Q-T-Y(Bz)-P-OEt 85% 25 21.0g 1)0.37 10.0g TFA 26 (20.4g) NaOH, water, Boc-L-Q-T-Y(Bz)-P-OH 90% 26 20.4g 5)0.27 MeOH 27 (17.6g) Boc-L-()-T-Y-P-OH 92% 27 17.6g Pd-C, H2 3)0.58 12 (14.6g) d) Boc-Leu-His-Lys(Psc)-OH(fragment 4, 13) Fragment 4 was obtained by the following steps with an overall yield of 81 %; firstly, α-carboxyl function of Boc-Lys(Psc)-OH was blocked by trichloroethyl group, and coupled stepwisely after deblocking of Boc, finally deprotected by catalytic(Zn) hydrogenation to give 13 (purity>99%, Rt=23.6min: HPLC) as white powder. reactant 1 reactant 2 coupling/ product yield Rf debloking Boc-His(Boc)- H-Lys(Psc)- Boc-H-K(Psc)-OTce 94% active ester 4)0.63 OTcp 10.2g OTce 10.5g 28 (15.5g) Boc-Leu-OSu active ester Boc-L-H-K(Psc)-OTce 93% 28 15.5g 5)0.33 8.7g /HCl,AcOH 29 (14.6g) Boc-L-H-K(Psc)-OH 93% 29 14.6g Zn, AcOH 1)0.30 13 (11.5g) e) Boc-Lys(Psc)-Leu-Ser-Gln-Clu (OPse)-OH(fragment 5, 14 ) Fragment 5(purity>99%, Rt=23.5min: HPLC) was obtained by the conventional stepwise coupling as follows with an overall yield of 58%; firstly, α-carboxyl function of Boc-Glu(OPse)-OH was blocked by

trichloroethyl group, and coupled stepwisely by the methods as shown below after deblocking of Boc, finally deprotected by catalytic hydrogenation to give 13 as white powder. coupling/ reactant 1 reactant 2 product yield Rf deblokinR H-Glu(OPse) Boc-Gln-OH Boc-Q-E(OPse)-OTce 93% -OTce TFA DCC,HOBT 5)0.42 7.4g 30 (16.3g) 14.5R Boc-Ser-OPfp TFV/ Boc-S-Q-E(OPse)-OTce 90% 30 16.3g 5)0.32 10.0g DCC,HOBT 31 (16.5g) Boc-Leu-OTcp TFA/ Boc-L-Q-E(OPse)-OTce 88% 31 16.5g 5)0.42 10.3g active ester 32 (16.7g) Boc-Lys(Psc)- TFA/ Boc-K(Pac)-L-S-Q-E(OPse)-OTce 93% 32 16.7g 5)0.33 OTcp 13.8g active ester 33 (21.5g) Boc-K(Psc)-L-S-Q-E(OPse)-OH 85% 33 21.5g Zn, AcOH 5)0.22 14 (16.0g) f) H-Ser-Thr-Cys(Acm)-Val-Leu-Gly-ONse TFA(fragment 6, 15) Fragment 6(purity>99%, Rt=1 9.6min HPLC) as white powder was obtained by the procedure as shown below with an overall yield of 67%; a -carboxyl function of Boc-Gly-OH was blocked by Nse group, and then after deblocking of Boc coupled stepwisely by the conventional methods using active esters or condensing agents(DCC, HOBT) to give 15 as white powder. coupling/ reactant 1 reactant 2 product yield Rf debloking Boc-Leu-OH H-Gly-ONse DCC,HOBT/ H-L-G-Onse 94% 1)0.47 5.9R 8.3R TFA 34 (10.1g) Boc-Val-OH DCC,HOBT/ H-V-L-G-ONse 89% 34 10.1g 1)0.48 5.2g TFA 35 (10.6g) Boc-Cys(Acm)- H-C(Acm)-V-L-G-ONse 94% 35 10.6g active ester/TFA 1)0.47 OPfp 5.9g 36 (12.8g) Boc-Thr-OPfp H-T-C(Acm)-V-L-G-ONse 98% 36 12.8g active ester/TFA 1)0.27 7.1g 37 (14.2g) H-S-T-C(Acm)-V-L-G-ONs 87% Boc-Ser-OPfp 37 14.2g active ester/TFA e (13.7g) 1)0.38 5.9g 15

g) H-Cys(Acm)-Ser-Asn-Leu-OH(fragment 7, 16) Fragment 7 was obtained by the procedure as described below; at first, a-carboxyl function of Boc-leu-OH was protected by the additon of Nse-OI # in the presence of DMAP, then the Boc group was deprotected to afford H-Leu-ONse quantitatively. Then the product was stepwisely coupled by the conventional methods using active esters or condensing agents(DCC, HOBT), finally deprotected by piperidine to give 16(purity>99%, Rt=16.4min: HPLC) as white powder. coupling/ reactant 1 reactant 2 product yield Rf debloking Boc-Asn-OH H-Leu-ONse r)CC,HOBT/ H-N-L-ONse TFA 85% 1)0.36 8.2R TFA 1 4.5R TFA 38 (1 5.4g) Boc-Ser-OPfp active ester H-S-N-L-ONse TFA 94% 38 15.4g 1)0.23 11.1g /TFA 39 (16.6g) Boc-Cys(Acm)- Boc-C(Acm)-S-N-L-ONse 93% 39 16.6g active ester 5)0.43 OPfp 9.1g 40 (19.1g) Boc-C(Acm)-S-N -L-OH 87% 40 19.1g piperidine 2)0.57 16 (12.3n) -Leu-Il is-Lys-Leu-Gln-Thr-Tyr-Pro-Arg-Thr r-Asn-Th r-GIy-Ser-Cly-Thr -Pro-NH2 (salmon calcitonin) Biological active salmon calcitonin as white powder was prepared by the segment condensation as shown in diagram 1. The synthesis was started from i) the condensation of fragment 1, the tetrapeptide corresponding to the carboxamide end of the salmon calcitonin sequence, with Boc-protected fragment 2 by the conventional method using DCC and HOBT. And stepwise condensations with Boc-protected fragment 3, 4, 5 and Boc group removals were mediated by the DCC/HOBT and TFA, respectively, to give newly side chain protected docosapeptide 45 in moderate yield. For the preparation of cyclic decapeptide 46 Acm-protected fragment 6 was condensed with Acm-protected fragment 7 by the conventional method, the Nse group for C-terminal blocking was deprotected with piperidine, and two Acm groups for masking of thiol function were simultaneously deprotected/oxidated with iodine in AcOll. After the final condensation of docosapeptide 45 with decapeptide 46, the resulting peptide was treated with TFA and piperidine in DMSO for shorter time to afford salmon calcitonin which showed a purity of 66% to 70So in analytical HPLC. The crude one was purified by preparative HPLC to give salmon calcitonin with high purity of above 98%. m.p.: 2200C [α]D: -55.0 (20°C, 50% AcOH) #max: 275nm LC/Mass: (1mm, C-18 column, 4Oul/min, water/Acetonitrile/TFA buffer) m/z 3431.8(M+) 1717.2([M+2H]2+) 1144.8([M+3H]3+) 859.0([M=4H]4+ Rt=22.90min AAA: Arg(0.93) Asp(0.97) Cys/2(1.0) Glu(0.90) Gly(1.0) His(0.92) Leu(1.05) Lys(1.0) Pro(0.92) Ser(0.91) Thr(0.98) Tyr(1.1)

coupling/ rcactant 1 reactant 2 debloking DCC,HOBT/ H-R-T-N-G-S-G-T-P-NH2 2TFA 83% 11 8.6g 10 10.5g 1)0.13 TFA 42 (15.0g) H-L-Q-T-Y-P-R-T-N-G-S-G-T-P DCC,HOBT/ 79% 12 10.4g 42 14.3g -NH2 2TFA 1)0.13 TFA (17.4g) 43 H-L-H-K(Psc)-L-Q-T-Y-P-R-T-N-G DCC,HOBT/ 90% 4)3) 13 7.7g 43 17.0g -S-G-T-P-NH2 3TFA TFA (21.5g) 0.24 44 H-K(Psc)-L-S-Q-G(OPse)-L-H-K [)CC,HOBT/ (F'sc)-L-(1-T-Y-F'-R-T-N-G-S-G-T 75% 14 12.0g 44 20.1g 6)0.38 TFA -P-NH2 3TFA (21.2g) 45 DCC,HOBT/ Boc-C-S-N-L-S-T-C-V-L-G-OH 77% 4)3) 15 13.6g 16 10.6g i)piperidin (1,7-disulfide bond) (12.0g) 0.32 ii)l2,AcOH 46 [)CC.HOBT/ 74% 45 20g 46 10.0g i)TFA salmon calcitonin ii)piperidin Example 3 Biological assay of salmon calcitonin Hypocalcaemic effect of salmon calcitonin was measured in rats by comparing with standard(NIBSC: National Institute for Biological Standards and Control). 30 rats of the same sex weighing up to 225g were divided into 6 groups. After deprive for 1 day, 3 groups are injected by standard preparation(1 ,3,9mlU/0.25mL of albumin solution, rat/ 100g of body weight), the other groups synthetic one. Exactly 1 hr after injection, a sample of blood was taken, the plasma of it was separated from cells. Then the calcium content of each sample was determined by atomic absorption spectroscopy, and the relationship between the calcium concentration and the logarithm of the dose was calculated by standard statistical methods. subcutaneously injected concentration biological activity compared (mlU / 1009 body weight) with standard preparation 9 99.75 % 3 98.65 % 1 98.75 % It is demonstrated that according to this invention, target peptide can be prepared by using new amino acid derivatives which are very stable under coupling and deblocking with good yield and in high purity, which shows high bilogical activity.