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RhoE的功能受ROCK I介导的磷酸化作用调控。

RhoE function is regulated by ROCK I-mediated phosphorylation.

作者信息

Riento Kirsi, Totty Nick, Villalonga Priam, Garg Ritu, Guasch Rosa, Ridley Anne J

机构信息

Ludwig Institute for Cancer Research, Royal Free and University College School of Medicine, London, UK.

出版信息

EMBO J. 2005 Mar 23;24(6):1170-80. doi: 10.1038/sj.emboj.7600612. Epub 2005 Mar 3.

Abstract

The Rho GTPase family member RhoE regulates actin filaments partly by binding to and inhibiting ROCK I, a serine/threonine kinase that induces actomyosin contractility. Here, we show that ROCK I can phosphorylate multiple residues on RhoE in vitro. In cells, ROCK I-phosphorylated RhoE localizes in the cytosol, whereas unphosphorylated RhoE is primarily associated with membranes. Phosphorylation has no effect on RhoE binding to ROCK I, but instead increases RhoE protein stability. Using phospho-specific antibodies, we show that ROCK phosphorylates endogenous RhoE at serine 11 upon cell stimulation with platelet-derived growth factor, and that this phosphorylation requires an active protein kinase C signalling pathway. In addition, we demonstrate that phosphorylation of RhoE correlates with its activity in inducing stress fibre disruption and inhibiting Ras-induced transformation. This is the first demonstration of an endogenous Rho family member being phosphorylated in vivo and indicates that phosphorylation is an important mechanism to control the stability and function of this GTPase-deficient Rho protein.

摘要

Rho GTP酶家族成员RhoE部分通过与丝氨酸/苏氨酸激酶ROCK I结合并抑制其活性来调节肌动蛋白丝,ROCK I可诱导肌动球蛋白收缩。在此,我们表明ROCK I在体外可磷酸化RhoE上的多个位点。在细胞中,ROCK I磷酸化的RhoE定位于胞质溶胶,而未磷酸化的RhoE主要与膜相关。磷酸化对RhoE与ROCK I的结合没有影响,但会增加RhoE蛋白的稳定性。使用磷酸化特异性抗体,我们发现用血小板衍生生长因子刺激细胞后,ROCK会在丝氨酸11位点磷酸化内源性RhoE,且这种磷酸化需要活性蛋白激酶C信号通路。此外,我们证明RhoE的磷酸化与其诱导应力纤维破坏和抑制Ras诱导的转化的活性相关。这是首次证明内源性Rho家族成员在体内被磷酸化,表明磷酸化是控制这种缺乏GTP酶的Rho蛋白稳定性和功能的重要机制。

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