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构象驱动的蛋白酶催化肽段剪接:V8蛋白酶介导源自嗜热菌蛋白酶和核糖核酸酶A的片段合成

Conformationally driven protease-catalyzed splicing of peptide segments: V8 protease-mediated synthesis of fragments derived from thermolysin and ribonuclease A.

作者信息

Kumaran S, Datta D, Roy R P

机构信息

National Institute of Immunology, New Delhi, India.

出版信息

Protein Sci. 1997 Oct;6(10):2233-41. doi: 10.1002/pro.5560061018.

DOI:10.1002/pro.5560061018
PMID:9336846
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2143560/
Abstract

We have studied the conformation as well as V8 protease-mediated synthesis of peptide fragments, namely amino acid residues 295-316 (TC-peptide) of thermolysin and residues 1-20 (S-peptide) of ribonuclease A, to examine whether "conformational trapping" of the product can facilitate reverse proteolysis. The circular dichroism study showed cosolvent-mediated cooperative helix formation in TC-peptide with attainment of about 30-35% helicity in the presence of 40% 1-propanol and 2-propanol solutions at pH 6 and 4 degrees C. The thermal melting profiles of TC-peptide in the above cosolvents were very similar. V8 protease catalyzed the synthesis of TC-peptide from a 1:1 mixture of the non-interacting complementary fragments (TC295-302 and TC303-316) in the presence of the above cosolvents at pH 6 and 4 degrees C. In contrast, V8 protease did not catalyze the ligation of S1-9 and S10-20, although S-peptide could assume helical conformation in the presence of the cosolvent used for the semisynthetic reaction. V8 protease was able to synthesize an analog of S-peptide (SA-peptide) in which residues 10-14 were substituted (RQHMD-->VAAAK). While S-peptide exhibited helical conformation in the presence of aqueous propanol solutions, SA-peptide displayed predominantly beta-sheet conformation. SA-peptide showed enhanced resistance to proteolysis as compared with S-peptide. Thus, failure of semisynthesis of S-peptide may be a consequence of high flexibility around the 9-10 peptide bond due to its proximity to the helix stop signal. The results suggest that protease-mediated ligations may be achieved by design and manipulation of the conformational aspects of the product.

摘要

我们研究了嗜热菌蛋白酶的构象以及V8蛋白酶介导的肽片段合成,即嗜热菌蛋白酶的氨基酸残基295 - 316(TC - 肽)和核糖核酸酶A的残基1 - 20(S - 肽),以检验产物的“构象捕获”是否能促进逆蛋白酶解。圆二色性研究表明,在pH 6和4℃条件下,在40% 1 - 丙醇和2 - 丙醇溶液存在时,共溶剂介导TC - 肽中形成协同螺旋,螺旋度达到约30 - 35%。TC - 肽在上述共溶剂中的热熔解曲线非常相似。在pH 6和4℃条件下,在上述共溶剂存在时,V8蛋白酶催化由非相互作用的互补片段(TC295 - 302和TC303 - 316)的1:1混合物合成TC - 肽。相反,尽管S - 肽在用于半合成反应的共溶剂存在时可呈现螺旋构象,但V8蛋白酶并未催化S1 - 9和S10 - 20的连接。V8蛋白酶能够合成一种S - 肽类似物(SA - 肽),其中残基10 - 14被取代(RQHMD→VAAAK)。当S - 肽在丙醇水溶液存在时呈现螺旋构象,而SA - 肽主要呈现β - 折叠构象。与S - 肽相比,SA - 肽对蛋白酶解的抗性增强。因此,S - 肽半合成失败可能是由于其9 - 10肽键靠近螺旋终止信号而具有高柔韧性的结果。结果表明,蛋白酶介导的连接可通过设计和操纵产物的构象方面来实现。

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引用本文的文献

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Product-conformation-driven ligation of peptides by V8 protease.V8蛋白酶介导的肽段的产物构象驱动连接反应
Protein Sci. 2002 Jun;11(6):1384-92. doi: 10.1110/ps.0201302.
2
An enigmatic peptide ligation reaction: protease-catalyzed oligomerization of a native protein segment in neat aqueous solution.一种神秘的肽连接反应:蛋白酶催化的天然蛋白质片段在纯水溶液中的寡聚化。
Protein Sci. 2000 Apr;9(4):734-41. doi: 10.1110/ps.9.4.734.
3
Chemistry of the "molecular trap" of protease-catalyzed splicing reaction of complementary segments of alpha-subunit of hemoglobin A.
J Protein Chem. 1998 Oct;17(7):669-78. doi: 10.1007/BF02780969.

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