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蛋白磷酸酶1对caspase 3切割的PAK2活性的负调控

Negative regulation of caspase 3-cleaved PAK2 activity by protein phosphatase 1.

作者信息

Wang JinJun, Wang ZhiXin

机构信息

National Laboratory of Biomacromolecules, Institute of Biophysics, Chinese Academy of Sciences, Beijing 100101, China.

出版信息

Sci China C Life Sci. 2008 Jan;51(1):1-11. doi: 10.1007/s11427-008-0006-z.

DOI:10.1007/s11427-008-0006-z
PMID:18176785
Abstract

The p21-activated kinase 2 (PAK2) is activated by binding of small G proteins, Cdc42 and Rac, or through proteolytic cleavage by caspases or caspase-like proteases. Activation by both small G protein and caspase requires autophosphorylation at Thr-402 of PAK2. Although activation of PAK2 has been investigated for nearly a decade, the mechanism of PAK2 downregulation is unclear. In this study, we have applied the kinetic theory of substrate reaction during modification of enzyme activity to study the regulation mechanism of PAK2 activity by the catalytic subunit of protein phosphatase 1 (PP1alpha). On the basis of the kinetic equation of the substrate reaction during the reversible phosphorylation of PAK2, all microscopic kinetic constants for the free enzyme and enzyme-substrate(s) complexes have been determined. The results indicate that (1) PP1alpha can act directly on phosphorylated Thr-402 in the activation loop of PAK2 and down-regulate its kinase activity; (2) binding of the exogenous protein/peptide substrates at the active site of PAK2 decreases both the rates of PAK2 autoactivation and inactivation. The present method provides a novel approach for studying reversible phosphorylation reactions. The advantage of this method is not only its usefulness in study of substrate effects on enzyme modification but also its convenience in study of modification reaction directly involved in regulation of enzyme activity. This initial study should provide a foundation for future structural and mechanistic work of protein kinases and phosphatases.

摘要

p21激活激酶2(PAK2)可通过与小G蛋白Cdc42和Rac结合,或通过半胱天冬酶或半胱天冬酶样蛋白酶的蛋白水解切割而被激活。小G蛋白和半胱天冬酶的激活均需要PAK2的苏氨酸-402位点发生自磷酸化。尽管对PAK2的激活已经研究了近十年,但其下调机制仍不清楚。在本研究中,我们应用酶活性修饰过程中底物反应的动力学理论,研究了蛋白磷酸酶1催化亚基(PP1α)对PAK2活性的调节机制。基于PAK2可逆磷酸化过程中底物反应的动力学方程,确定了游离酶和酶-底物复合物的所有微观动力学常数。结果表明:(1)PP1α可直接作用于PAK2激活环中磷酸化的苏氨酸-402,并下调其激酶活性;(2)外源性蛋白质/肽底物在PAK2活性位点的结合降低了PAK2自激活和失活的速率。本方法为研究可逆磷酸化反应提供了一种新途径。该方法的优点不仅在于其在研究底物对酶修饰的影响方面有用,还在于其在研究直接参与酶活性调节的修饰反应方面的便利性。这项初步研究应为未来蛋白激酶和磷酸酶的结构和机制研究奠定基础。

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Negative regulation of caspase 3-cleaved PAK2 activity by protein phosphatase 1.蛋白磷酸酶1对caspase 3切割的PAK2活性的负调控
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