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配体与阴离子结合外位调节凝血酶的构象特性。

Ligand binding to anion-binding exosites regulates conformational properties of thrombin.

机构信息

Chemistry Department, University of Louisville, Louisville, Kentucky 40292.

Chemistry Department, University of Louisville, Louisville, Kentucky 40292.

出版信息

J Biol Chem. 2013 Mar 22;288(12):8667-8678. doi: 10.1074/jbc.M112.410829. Epub 2013 Feb 1.

Abstract

Thrombin participates in coagulation, anticoagulation, and initiation of platelet activation. To fulfill its diverse roles and maintain hemostasis, this serine protease is regulated via the extended active site region and anion-binding exosites (ABEs) I and II. For the current project, amide proton hydrogen-deuterium exchange coupled with MALDI-TOF mass spectrometry was used to characterize ligand binding to individual exosites and to investigate the presence of exosite-active site and exosite-exosite interactions. PAR3(44-56) and PAR1(49-62) were observed to bind to thrombin ABE I and then to exhibit long range effects over to ABE II. By contrast, Hirudin(54-65) focused more on ABE I and did not transmit influences over to ABE II. Although these three ligands were each directed to ABE I, they did not promote the same conformational consequences. D-Phe-Pro-Arg-chloromethyl ketone inhibition at the thrombin active site led to further local and long range consequences to thrombin-ABE I ligand complexes with the autolysis loop often most affected. When Hirudin(54-65) was bound to ABE I, it was still possible to bind GpIbα(269-286) or fibrinogen γ'(410-427) to ABE II. Each ligand exerted its predominant influences on thrombin and also allowed interexosite communication. The results obtained support the proposal that thrombin is a highly dynamic protein. The transmission of ligand-specific local and long range conformational events is proposed to help regulate this multifunctional enzyme.

摘要

凝血酶参与凝血、抗凝和血小板激活的启动。为了发挥其多种作用并维持止血,这种丝氨酸蛋白酶通过扩展的活性位点区域和阴离子结合外位(ABE)I 和 II 进行调节。在当前项目中,酰胺质子氘交换与 MALDI-TOF 质谱联用用于表征配体与单个外位的结合,并研究外位-活性位点和外位-外位相互作用的存在。PAR3(44-56) 和 PAR1(49-62) 观察到与凝血酶 ABE I 结合,然后在 ABE II 上表现出长程效应。相比之下,水蛭素(54-65) 更专注于 ABE I,并且不会将影响传递到 ABE II。尽管这三种配体都被定向到 ABE I,但它们并没有促进相同的构象后果。凝血酶活性位点的 D-Phe-Pro-Arg-氯甲基酮抑制导致与自溶环经常受影响的凝血酶-ABE I 配体复合物的进一步局部和长程后果。当水蛭素(54-65)与 ABE I 结合时,仍然可以将 GpIbα(269-286)或纤维蛋白原γ'(410-427)结合到 ABE II。每种配体对凝血酶都有其主要影响,并且允许外位间通讯。所得结果支持凝血酶是一种高度动态蛋白的观点。配体特异性局部和长程构象事件的传递被认为有助于调节这种多功能酶。

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