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尿激酶对人α-凝血酶进行有限的蛋白水解会产生一种无凝血活性的酶。

Limited proteolysis of human alpha-thrombin by urokinase yields a non-clotting enzyme.

作者信息

Bezeaud A, de Raucourt E, Miyata T, Bouton M C, Angles-Cano E, Guillin M C

机构信息

Laboratoire de Recherche sur l'Hémostase et la Thrombose, Faculté Xavier Bichat, Paris, France.

出版信息

Thromb Haemost. 1995 Feb;73(2):275-80.

PMID:7792743
Abstract

Limited proteolysis of human alpha-thrombin by various proteases has been efficiently used to demonstrate the importance of two insertion loops located on the surface of this molecule. In the present study, we demonstrate that two-chain urokinase (tcu-PA) specifically cleaves the B chain of alpha-thrombin giving rise to a transient derivative, consisting of two non-covalently linked subunits. Although the thrombin derivative conserves its activity towards the synthetic substrate S-2238 (Km = 8.4 microM and kcat = 145 s-1 versus respectively 4.5 microM and 149 s-1 for alpha-thrombin), most of its coagulant activity is lost (140 NIH u/mg versus 3000 NIH u/mg) and its ability to activate platelets is considerably reduced (threshold for full platelet aggregation 2.5 nM versus 0.25 nM). The thrombin fragments were separated by HPLC and after reduction and S-carboxyamidemethylation were digested with a lysylendopeptidase; the resulting peptides were separated by HPLC and sequenced. One fragment corresponded to B chain fragment 1-73 and the second to B chain fragment 74-259 covalently linked to the A chain, indicating that tcu-PA cleaves selectively the peptide bond Arg 73-Asn 74 in the B chain. The proteolytic derivative obtained, designated beta u-thrombin, is therefore identical to the transient proteolytic derivative, beta 1-thrombin, produced by trypsin. Prolonged incubation with tcu-PA resulted in further conversion in a derivative analogous to gamma t-thrombin.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

多种蛋白酶对人α-凝血酶的有限蛋白水解已被有效用于证明该分子表面两个插入环的重要性。在本研究中,我们证明双链尿激酶(tcu-PA)特异性切割α-凝血酶的B链,产生一种由两个非共价连接亚基组成的瞬时衍生物。尽管凝血酶衍生物保留了对合成底物S-2238的活性(Km = 8.4 microM,kcat = 145 s-1,而α-凝血酶分别为4.5 microM和149 s-1),但其大部分凝血活性丧失(140 NIH u/mg对3000 NIH u/mg),其激活血小板的能力也大大降低(完全血小板聚集阈值为2.5 nM对0.25 nM)。通过HPLC分离凝血酶片段,还原和S-羧酰胺甲基化后用赖氨酰内肽酶消化;所得肽通过HPLC分离并测序。一个片段对应于B链片段1-73,第二个片段对应于与A链共价连接的B链片段74-259,表明tcu-PA选择性切割B链中的肽键Arg 73-Asn 74。因此,获得的蛋白水解衍生物βu-凝血酶与胰蛋白酶产生的瞬时蛋白水解衍生物β1-凝血酶相同。与tcu-PA长时间孵育导致进一步转化为类似于γt-凝血酶的衍生物。(摘要截短至250字)

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