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Gα Subunit Gpa2 Recruits Kelch Repeat Subunits That Inhibit Receptor-G Protein Coupling during cAMP-induced Dimorphic Transitions in Saccharomyces cerevisiae

机译:Gα亚基Gpa2招募克尔奇重复亚基,该亚基在cAMP诱导的酿酒酵母双态转化过程中抑制受体G蛋白偶联。

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摘要

All eukaryotic cells sense extracellular stimuli and activate intracellular signaling cascades via G protein-coupled receptors (GPCR) and associated heterotrimeric G proteins. The Saccharomyces cerevisiae GPCR Gpr1 and associated Gα subunit Gpa2 sense extracellular carbon sources (including glucose) to govern filamentous growth. In contrast to conventional Gα subunits, Gpa2 forms an atypical G protein complex with the kelch repeat Gβ mimic proteins Gpb1 and Gpb2. Gpb1/2 negatively regulate cAMP signaling by inhibiting Gpa2 and an as yet unidentified target. Here we show that Gpa2 requires lipid modifications of its N-terminus for membrane localization but association with the Gpr1 receptor or Gpb1/2 subunits is dispensable for membrane targeting. Instead, Gpa2 promotes membrane localization of its associated Gβ mimic subunit Gpb2. We also show that the Gpa2 N-terminus binds both to Gpb2 and to the C-terminal tail of the Gpr1 receptor and that Gpb1/2 binding interferes with Gpr1 receptor coupling to Gpa2. Our studies invoke novel mechanisms involving GPCR-G protein modules that may be conserved in multicellular eukaryotes.
机译:所有的真核细胞都通过G蛋白偶联受体(GPCR)和相关的异三聚体G蛋白感知细胞外刺激并激活细胞内信号传导级联。酿酒酵母GPCR Gpr1和相关的Gα亚基Gpa2感知细胞外碳源(包括葡萄糖)来控制丝状生长。与常规的Gα亚基相反,Gpa2与海藻重复Gβ模仿蛋白Gpb1和Gpb2形成非典型的G蛋白复合物。 Gpb1 / 2通过抑制Gpa2和一个尚未确定的靶标来负调控cAMP信号传导。在这里,我们显示Gpa2需要对其N末端进行脂质修饰以进行膜定位,但与Gpr1受体或Gpb1 / 2亚基缔合对于膜靶向而言是必不可少的。相反,Gpa2促进其相关的Gβ模拟亚基Gpb2的膜定位。我们还显示,Gpa2 N末端与Gpb2和Gpr1受体的C末端尾部都结合,并且Gpb1 / 2结合会干扰Gpr1受体与Gpa2的偶联。我们的研究提出了涉及GPCR-G蛋白模块的新机制,该机制可能在多细胞真核生物中得以保守。

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  • 作者单位
  • 年度 2005
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  • 原文格式 PDF
  • 正文语种 en
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  • 入库时间 2022-08-31 15:23:34

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