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Molecular assembly of rhodopsin with G protein-coupled receptor kinases

机译:视紫红质与G蛋白偶联受体激酶的分子组装

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摘要

G protein-coupled receptor kinases (GRKs) play pivotal roles in desensitizing GPCR signaling but little is known about how GRKs recognize and phosphorylate GPCRs due to the technical difficulties in detecting the highly dynamic GPCR/GRK interaction. By combining a genetic approach with multiple biochemical assays, we identified the key determinants for the assembly of the prototypical GPCR rhodopsin with its kinase GRK1. Our work reveals that the regulatory G-protein signaling homology (RH) domain of GRKs is the primary binding site to GPCRs and an active conformation of the GRK1 kinase domain is required for efficient interaction with rhodopsin. In addition, we provide a mechanistic solution for the longstanding puzzle about the gain-of-function Q41L mutation in GRK5. This mutation is in the RH domain and increases the capacity of the GRK mutant to interact with and to desensitize GPCRs. Finally we present the principal architecture of a rhodopsin/GRK complex through negative stain electron microscopy reconstruction. Together, these data define the key components for the rhodopsin/GRK1 interaction and provide a framework for understanding GRK-mediated desensitization of GPCRs.
机译:G蛋白偶联受体激酶(GRK)在使GPCR信号减敏中起关键作用,但由于检测高动态GPCR / GRK相互作用的技术困难,人们对GRK如何识别和磷酸化GPCR知之甚少。通过将遗传学方法与多种生化分析相结合,我们确定了原型GPCR视紫红质及其激酶GRK1装配的关键决定因素。我们的工作表明,GRK的调节性G蛋白信号同源性(RH)域是GPCR的主要结合位点,而GRK1激酶域的有效构象是与视紫红质有效相互作用所必需的。此外,我们为有关GRK5中功能获得Q41L突变的长期难题提供了一种机械解决方案。此突变在RH域中,并增加了GRK突变体与GPCR相互作用并使它们脱敏的能力。最后,我们通过负染色电子显微镜重建介绍了视紫红质/ GRK复合物的主要结构。这些数据共同定义了视紫红质/ GRK1相互作用的关键成分,并为理解GRK介导的GPCR脱敏提供了框架。

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