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Roco 蛋白 GbpC 在粘菌中的多种调控机制。

Multiple regulatory mechanisms for the Dictyostelium Roco protein GbpC.

机构信息

Department of Cell Biochemistry, University of Groningen, Nijenborgh 7, 9747 AG Groningen, The Netherlands.

出版信息

J Biol Chem. 2012 Jan 20;287(4):2749-58. doi: 10.1074/jbc.M111.315739. Epub 2011 Nov 26.

DOI:10.1074/jbc.M111.315739
PMID:22119747
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3268432/
Abstract

GbpC is a multidomain Roco protein in Dictyostelium, involved in transduction of intracellular cGMP that is produced by chemotactic signals. We have shown previously that cGMP binding to GbpC induces an intramolecular signaling cascade by activating subsequently the GEF, Ras, and kinase domains. In this study, we report on the cellular localization of GbpC. In resting cells, the protein is present in the cytoplasm, but GbpC rapidly translocates to the cell boundary upon stimulation with the chemoattractant cAMP. Also, during the formation of cell-cell streams and osmotic shock, the protein localizes toward the plasma membrane and actin cytoskeleton. The translocation upon cAMP stimulation occurs downstream of heterotrimeric G proteins but is independent of guanylyl cyclases and the previously identified cGMP-induced intramolecular signaling cascade in GbpC. Mutations in the GRAM domain of GbpC lead to disturbed membrane association and inactivation of GbpC function during chemotaxis in vivo. Furthermore, we show that the GRAM domain itself associates with cellular membranes and binds various phospholipids in vitro. Together, the results show that GbpC receives multiple input signals that are both required for functional activity in vivo. cAMP-stimulation induces a cGMP-dependent signaling cascade, leading to activation of kinase activity, and, independently, cAMP induces a GRAM-dependent translocation of GbpC toward the plasma membrane and cell cortex, where it may locally phosphorylate effector proteins, which are needed for proper biological activity.

摘要

GbpC 是一种在盘基网柄菌中具有多个结构域的 Roco 蛋白,参与由趋化信号产生的细胞内 cGMP 的转导。我们之前已经表明,cGMP 与 GbpC 结合通过随后激活 GEF、Ras 和激酶结构域来诱导分子内信号级联。在这项研究中,我们报告了 GbpC 的细胞定位。在静止细胞中,该蛋白存在于细胞质中,但在受到趋化剂 cAMP 刺激时,GbpC 会迅速向细胞膜边界转移。此外,在细胞-细胞流和渗透冲击形成过程中,该蛋白定位于质膜和肌动蛋白细胞骨架。cAMP 刺激引起的易位发生在异三聚体 G 蛋白的下游,但不依赖于鸟苷酸环化酶和 GbpC 中先前鉴定的 cGMP 诱导的分子内信号级联。GbpC 的 GRAM 结构域中的突变导致在体内趋化过程中膜结合受到干扰和 GbpC 功能失活。此外,我们还表明,GRAM 结构域本身与细胞膜结合,并在体外结合各种磷脂。总之,结果表明 GbpC 接收多个输入信号,这些信号对于体内功能活性都是必需的。cAMP 刺激诱导 cGMP 依赖性信号级联,导致激酶活性的激活,并且独立地,cAMP 诱导 GbpC 向质膜和细胞皮质的 GRAM 依赖性易位,其可能在局部磷酸化效应蛋白,这对于适当的生物活性是必需的。

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