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活化的Ras蛋白通过使盘基网柄菌DdCAD-1去磷酸化来改变细胞黏附。

An activated Ras protein alters cell adhesion by dephosphorylating Dictyostelium DdCAD-1.

作者信息

Secko David M, Siu Chi-Hung, Spiegelman George B, Weeks Gerald

机构信息

Department of Microbiology and Immunology, University of British Columbia, Life Sciences Centre, 2350 Health Sciences Mall, Vancouver, British Columbia V6T 1Z4, Canada.

Banting and Best Department of Medical Research, and Department of Biochemistry, University of Toronto, Toronto, Ontario M5G 1L6, Canada.

出版信息

Microbiology (Reading). 2006 May;152(Pt 5):1497-1505. doi: 10.1099/mic.0.28709-0.

Abstract

RasG-regulated signal transduction has been linked to a variety of growth-specific processes and appears to also play a role in the early development of Dictyostelium discoideum. In an attempt to uncover some of the molecular components involved in Ras-mediated signalling, several proteins have been described previously, including the cell adhesion molecule DdCAD-1, whose phosphorylation state was affected by the expression of the constitutively activated RasG, RasG(G12T). Here it has been shown that a cadA null strain lacks the phosphoproteins that were tentatively identified as DdCAD-1, confirming its previous designation. Further investigation revealed that cells expressing RasG(G12T) exhibited increased cell-cell cohesion, concomitant with reduced levels of DdCAD-1 phosphorylation. This increased cohesion was DdCAD-1-dependent and was correlated with increased localization of DdCAD-1 at the cell surface. DdCAD-1 phosphorylation was also found to decrease during Dictyostelium aggregation. These results revealed a possible role for protein phosphorylation in regulating DdCAD-1-mediated cell adhesion during early development. In addition, the levels of DdCAD-1 protein were substantially reduced in a rasG null cell line. These results indicate that RasG affects both the expression and dephosphorylation of DdCAD-1 during early development.

摘要

RasG调节的信号转导与多种生长特异性过程相关,并且似乎在盘基网柄菌的早期发育中也发挥作用。为了揭示Ras介导的信号传导中涉及的一些分子成分,之前已经描述了几种蛋白质,包括细胞粘附分子DdCAD-1,其磷酸化状态受组成型激活的RasG即RasG(G12T)表达的影响。本文表明,cadA基因敲除菌株缺乏初步鉴定为DdCAD-1的磷蛋白,证实了其先前的命名。进一步研究发现,表达RasG(G12T)的细胞表现出细胞间凝聚力增加,同时DdCAD-1磷酸化水平降低。这种增加的凝聚力依赖于DdCAD-1,并且与DdCAD-1在细胞表面的定位增加相关。还发现盘基网柄菌聚集过程中DdCAD-1磷酸化减少。这些结果揭示了蛋白质磷酸化在早期发育过程中调节DdCAD-1介导的细胞粘附方面可能发挥的作用。此外,在rasG基因敲除细胞系中DdCAD-1蛋白水平大幅降低。这些结果表明,RasG在早期发育过程中影响DdCAD-1的表达和去磷酸化。

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