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人α-凝血酶蛋白水解衍生物的酶学性质

Enzymatic properties of proteolytic derivatives of human alpha-thrombin.

作者信息

Hofsteenge J, Braun P J, Stone S R

机构信息

Friedrich Miescher Institut, Basel, Switzerland.

出版信息

Biochemistry. 1988 Mar 22;27(6):2144-51. doi: 10.1021/bi00406a049.

DOI:10.1021/bi00406a049
PMID:3378050
Abstract

The use of derivatives of alpha-thrombin obtained by limited proteolysis, that have only a single peptide bond cleaved, allowed the unequivocal correlation between the change in covalent structure and alteration of the enzymatic properties. beta T-Thrombin contains a single cleavage in the surface loop corresponding to residues 65-83 of alpha-chymotrypsin [Birktoft, J. J., & Blow, D. M. (1972) J. Mol. Biol. 68, 187-240]. Compared with alpha-thrombin, this modification had a minor effect on the following: (1) The Michaelis constant (Km) for two tripeptidyl p-nitroanilide substrates increased 2-3 fold, whereas the catalytic constant (k cat) remained unaltered. (2) A 2-3 fold increase in the binding constant (KI) of a tripeptidyl chloromethane inhibitor was observed, but the inactivation rate constant (k i) was the same, which indicated that the nucleophilicity of the active-site histidyl residue had not changed. (3) The second-order rate constant for the inhibition by antithrombin III decreased 2-fold. Heparin accelerated the inactivation, and the degree of acceleration was similar to that obtained with alpha-thrombin. Pronounced effects of the cleavage of this loop were found. (1) The cleavage of fibrinogen was approximately 80-fold slower than that with alpha-thrombin. This was mainly due to a 40-fold decrease in k cat. In contrast, only a 1.9-fold increase in the Michaelis constant was observed. (2) The affinity for thrombomodulin had decreased 39-fold compared to alpha-thrombin. epsilon-Thrombin contains a single cleaved peptide bond in the loop corresponding to residues 146-150 in alpha-chymotrypsin.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过有限蛋白水解获得的α-凝血酶衍生物,其仅有一个肽键被切割,这使得共价结构的变化与酶学性质的改变之间建立了明确的关联。βT-凝血酶在对应于α-胰凝乳蛋白酶65 - 83位残基的表面环中含有一个单一切割位点[伯克托夫特,J. J.,& 布洛,D. M.(1972年)《分子生物学杂志》68卷,187 - 240页]。与α-凝血酶相比,这种修饰对以下方面有较小影响:(1)两种三肽基对硝基苯胺底物的米氏常数(Km)增加了2 - 3倍,而催化常数(k cat)保持不变。(2)观察到三肽基氯甲烷抑制剂的结合常数(KI)增加了2 - 3倍,但失活速率常数(k i)相同,这表明活性位点组氨酸残基的亲核性没有改变。(3)抗凝血酶III抑制的二级速率常数降低了2倍。肝素加速了失活,加速程度与α-凝血酶相似。发现该环切割有显著影响。(1)纤维蛋白原的切割比α-凝血酶慢约80倍。这主要是由于k cat降低了40倍。相比之下,米氏常数仅增加了1.9倍。(2)与α-凝血酶相比,对血栓调节蛋白的亲和力降低了39倍。ε-凝血酶在对应于α-胰凝乳蛋白酶146 - 150位残基的环中含有一个单一切割的肽键。(摘要截短于250字)

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