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Nuclear Localization of the ERK MAP Kinase Mediated by Drosophila αPS2βPS Integrin and Importin-7

机译:果蝇αPS2βPS整合素和Importin-7介导的ERK MAP激酶的核定位。

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The control of gene expression by the mitogen-activated protein (MAP) kinase extracellular signal-regulated kinase (ERK) requires its translocation into the nucleus. In Drosophila S2 cells nuclear accumulation of diphospho-ERK (dpERK) is greatly reduced by interfering double-stranded RNA against Drosophila importin-7 (DIM-7) or by the expression of integrin mutants, either during active cell spreading or after stimulation by insulin. In both cases, total ERK phosphorylation (on Westerns) is not significantly affected, and ERK accumulates in a perinuclear ring. Tyrosine phosphorylation of DIM-7 is reduced in cells expressing integrin mutants, indicating a mechanistic link between these components. DIM-7 and integrins localize to the same actin-containing peripheral regions in spreading cells, but DIM-7 is not concentrated in paxillin-positive focal contacts or stable focal adhesions. The Corkscrew (SHP-2) tyrosine phosphatase binds DIM-7, and Corkscrew is required for the cortical localization of DIM-7. These data suggest a model in which ERK phosphorylation must be spatially coupled to integrin-mediated DIM-7 activation to make a complex that can be imported efficiently. Moreover, dpERK nuclear import can be restored in DIM-7–deficient cells by Xenopus Importin-7, demonstrating that ERK import is an evolutionarily conserved function of this protein.
机译:有丝分裂原激活蛋白(MAP)激酶细胞外信号调节激酶(ERK)对基因表达的控制要求其易位到细胞核中。在果蝇S2细胞中,通过干扰果蝇importin-7(DIM-7)的双链RNA或通过整联蛋白突变体的表达(在活性细胞扩散过程中或在胰岛素刺激下)大大降低了二磷酸ERK(dpERK)的核积累。在这两种情况下,总ERK磷酸化(在Westerns上)均未受到明显影响,并且ERK积累在核周环中。在表达整联蛋白突变体的细胞中,DIM-7的酪氨酸磷酸化降低,表明这些组件之间存在机械联系。 DIM-7和整联蛋白位于铺展细胞中相同的含肌动蛋白的外围区域,但DIM-7并不集中在帕西林阳性的焦点接触或稳定的粘连中。开瓶器(SHP-2)酪氨酸磷酸酶结合DIM-7,而DIM-7的皮质定位需要开瓶器。这些数据提示了一个模型,其中ERK磷酸化必须在空间上与整联蛋白介导的DIM-7激活偶联,以形成可以有效导入的复合物。此外,非洲爪蟾Importin-7可以在DIM-7缺陷细胞中恢复dpERK核的导入,表明ERK导入是该蛋白的进化保守功能。

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