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蛋白激酶 A 依赖性磷酸化 Rap1 调节其膜定位和细胞迁移。

Protein kinase A-dependent phosphorylation of Rap1 regulates its membrane localization and cell migration.

机构信息

From the Vollum Institute, and.

出版信息

J Biol Chem. 2013 Sep 27;288(39):27712-23. doi: 10.1074/jbc.M113.466904. Epub 2013 Aug 14.

Abstract

The small G protein Rap1 can mediate "inside-out signaling" by recruiting effectors to the plasma membrane that signal to pathways involved in cell adhesion and cell migration. This action relies on the membrane association of Rap1, which is dictated by post-translational prenylation as well as by a stretch of basic residues within its carboxyl terminus. One feature of this stretch of acidic residues is that it lies adjacent to a functional phosphorylation site for the cAMP-dependent protein kinase PKA. This phosphorylation has two effects on Rap1 action. One, it decreases the level of Rap1 activity as measured by GTP loading and the coupling of Rap1 to RapL, a Rap1 effector that couples Rap1 GTP loading to integrin activation. Two, it destabilizes the membrane localization of Rap1, promoting its translocation into the cytoplasm. These two actions, decreased GTP loading and decreased membrane localization, are related, as the translocation of Rap1-GTP into the cytoplasm is associated with its increased GTP hydrolysis and inactivation. The consequences of this phosphorylation in Rap1-dependent cell adhesion and cell migration were also examined. Active Rap1 mutants that lack this phosphorylation site had a minimal effect on cell adhesion but strongly reduced cell migration, when compared with an active Rap1 mutant that retained the phosphorylation site. This suggests that optimal cell migration is associated with cycles of Rap1 activation, membrane egress, and inactivation, and requires the regulated phosphorylation of Rap1 by PKA.

摘要

小分子 G 蛋白 Rap1 可以通过招募效应物到质膜上来介导“内向外信号转导”,这些效应物信号通路参与细胞黏附和细胞迁移。这种作用依赖于 Rap1 的膜结合,这由翻译后修饰的异戊烯基化以及其羧基末端的一段碱性残基决定。这段酸性残基的一个特征是它紧邻 cAMP 依赖性蛋白激酶 PKA 的功能性磷酸化位点。这种磷酸化对 Rap1 作用有两个影响。一,它降低了 Rap1 活性的水平,如通过 GTP 加载和 Rap1 与 RapL 的偶联来衡量,RapL 是一种将 Rap1 GTP 加载偶联到整合素激活的 Rap1 效应物。二,它使 Rap1 的膜定位不稳定,促进其易位到细胞质中。这两个作用,即 GTP 加载的减少和膜定位的减少是相关的,因为 Rap1-GTP 易位到细胞质中与其 GTP 水解和失活的增加有关。还研究了这种磷酸化在 Rap1 依赖性细胞黏附和细胞迁移中的作用。与保留磷酸化位点的活性 Rap1 突变体相比,缺乏该磷酸化位点的活性 Rap1 突变体对细胞黏附的影响最小,但强烈降低了细胞迁移。这表明最佳的细胞迁移与 Rap1 的激活、膜输出和失活循环有关,并且需要 PKA 对 Rap1 的调节性磷酸化。

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