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丝氨酸蛋白酶的催化机制:对α-裂解蛋白酶催化三联体中组氨酸1J13C2-H耦合常数pH依赖性的重新审视。

Catalytic mechanism of serine proteases: reexamination of the pH dependence of the histidyl 1J13C2-H coupling constant in the catalytic triad of alpha-lytic protease.

作者信息

Bachovchin W W, Kaiser R, Richards J H, Roberts J D

出版信息

Proc Natl Acad Sci U S A. 1981 Dec;78(12):7323-6. doi: 10.1073/pnas.78.12.7323.

Abstract

L-Histidine, 90% 13C enriched at the C2 position, was incorporated into the catalytic triad of alpha-lytic protease (EC 3.4.21.12) with the aid of histidine-requiring mutant of Lysobacter enzymogenes (ATC 29487), and the pH dependence of the coupling constant between this carbon atom and its directly bonded proton was reinvestigated. The high degree of specific 13C isotopic enrichment attainable with the auxotroph permits direct observation and measurement of this coupling constant in proton-coupled 13C NMR spectra at 67.89 MHz and at 15.1 MHz. In contrast to the earlier study, the present study indicate that this coupling constant does respond to a microscopic ionization with pKa near 7.0; moreover, the magnitude of the values of 1JC-H observed are in accord with those expected for titration of the histidyl residue. We conclude that the original measurement must be in error and that this coupling constant now also supports a histidyl residue that titrates more or less normally as a component of the catalytic triad of serine proteases.

摘要

L-组氨酸在C2位置有90%的13C富集,在产酶溶杆菌(ATC 29487)的组氨酸需求突变体的帮助下被掺入α-裂解蛋白酶(EC 3.4.21.12)的催化三联体中,并且重新研究了该碳原子与其直接相连质子之间耦合常数的pH依赖性。利用营养缺陷型可实现的高度特异性13C同位素富集,允许在67.89 MHz和15.1 MHz的质子耦合13C NMR谱中直接观察和测量该耦合常数。与早期研究相反,本研究表明该耦合常数确实对pKa接近7.0的微观电离有响应;此外,观察到的1JC-H值的大小与组氨酸残基滴定预期的值一致。我们得出结论,原来的测量一定有误,并且该耦合常数现在也支持一个作为丝氨酸蛋白酶催化三联体组成部分的组氨酸残基,其滴定或多或少是正常的。

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