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Epac1 interacts with importin β1 and controls neurite outgrowth independently of cAMP and Rap1

机译:EPAC1与Importinβ1相互作用,独立于营地和RAP1控制神经突遗传

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Exchange protein directly activated by cAMP-1 (Epac1) is a cAMP sensor that regulates multiple cellular functions including cellular migration, proliferation and differentiation. Classically, Epac1 is thought to exert its effects through binding of cAMP leading to a conformational change in Epac1 and its accumulation at the plasma membrane (PM) where it activates Rap1. In search for regulators of Epac1 activity, we show here that importin β1 (impβ1) is an Epac1 binding partner that prevents PM accumulation of Epac1. We demonstrate that in the absence of impβ1, endogenous as well as overexpressed Epac1 accumulate at the PM. Moreover, agonist-induced PM translocation of Epac1 leads to dissociation of Epac1 from impβ1. Localization of Epac1 at the PM in the absence of impβ1, requires residue R82 in its DEP domain. Notably, the PM accumulation of Epac1 in the absence of impβ1 does not require binding of cAMP to Epac1 and does not result in Rap1 activation. Functionally, PM accumulation of Epac1, an Epac1 mutant deficient in cAMP binding, or an Epac1 mutant tethered to the PM, is sufficient to inhibit neurite outgrowth. In conclusion, we uncover a cAMP-independent function of Epac1 at the PM and demonstrate that impβ1 controls subcellular localization of Epac1.
机译:CAMP-1(EPAC1)直接激活的交换蛋白是调节多个细胞功能,包括细胞迁移,增殖和分化的阵营传感器。经典上,EPAC1被认为通过CAMP的结合导致EPAC1的构象变化及其在血浆膜(PM)中的积累来发挥其效果,在那里它激活RAP1。为了寻找EPAC1活性的调节剂,我们在此显示Importinβ1(IMPβ1)是一种ePAC1结合伴侣,其防止PM积累EPAC1。我们证明在没有IMPβ1的情况下,内源性以及过表达EPAC1在PM积聚。此外,激动剂诱导的PM易位EPAC1易位导致来自IMPβ1的EPAC1的解离。在没有IMPβ1的情况下PM在PM的局部化需要其DEP结构域中的残留物R82。值得注意的是,在没有IMPβ1的情况下,ePac1的PM积累不需要将阵营的结合到EPAC1,并且不会导致RAP1激活。在功能上,PM ePAC1的累积,胰蛋白酶结合的EPAC1突变体,或持续到PM的EPAC1突变体足以抑制神经突的过度。总之,我们在PM揭示了ePAC1的营养函数,并证明了IMPβ1控制EPAC1的亚细胞定位。

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