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工程化的蛋白质与肌动蛋白的连接模拟了G蛋白偶联受体的PDZ依赖性循环,但不模拟其受Hrs的调节。

Engineered protein connectivity to actin mimics PDZ-dependent recycling of G protein-coupled receptors but not its regulation by Hrs.

作者信息

Lauffer Benjamin E L, Chen Stanford, Melero Cristina, Kortemme Tanja, von Zastrow Mark, Vargas Gabriel A

机构信息

Program in Pharmaceutical Sciences and Pharmacogenomics, Department of Psychiatry, University of California, San Francisco, California 94158-2140, USA.

出版信息

J Biol Chem. 2009 Jan 23;284(4):2448-58. doi: 10.1074/jbc.M806370200. Epub 2008 Nov 10.

Abstract

Many G protein-coupled receptors (GPCRs) recycle after agonist-induced endocytosis by a sequence-dependent mechanism, which is distinct from default membrane flow and remains poorly understood. Efficient recycling of the beta2-adrenergic receptor (beta2AR) requires a C-terminal PDZ (PSD-95/Discs Large/ZO-1) protein-binding determinant (PDZbd), an intact actin cytoskeleton, and is regulated by the endosomal protein Hrs (hepatocyte growth factor-regulated substrate). The PDZbd is thought to link receptors to actin through a series of protein interaction modules present in NHERF/EBP50 (Na+/H+ exchanger 3 regulatory factor/ezrin-binding phosphoprotein of 50 kDa) family and ERM (ezrin/radixin/moesin) family proteins. It is not known, however, if such actin connectivity is sufficient to recapitulate the natural features of sequence-dependent recycling. We addressed this question using a receptor fusion approach based on the sufficiency of the PDZbd to promote recycling when fused to a distinct GPCR, the delta-opioid receptor, which normally recycles inefficiently in HEK293 cells. Modular domains mediating actin connectivity promoted receptor recycling with similarly high efficiency as the PDZbd itself, and recycling promoted by all of the domains was actin-dependent. Regulation of receptor recycling by Hrs, however, was conferred only by the PDZbd and not by downstream interaction modules. These results suggest that actin connectivity is sufficient to mimic the core recycling activity of a GPCR-linked PDZbd but not its cellular regulation.

摘要

许多G蛋白偶联受体(GPCRs)在激动剂诱导的内吞作用后通过一种序列依赖性机制进行再循环,这种机制不同于默认的膜流动,目前仍知之甚少。β2肾上腺素能受体(β2AR)的有效再循环需要一个C末端PDZ(PSD-95/盘状大蛋白/ZO-1)蛋白结合决定簇(PDZbd)、完整的肌动蛋白细胞骨架,并受内体蛋白Hrs(肝细胞生长因子调节底物)调控。PDZbd被认为通过存在于NHERF/EBP50(Na+/H+交换体3调节因子/50 kDa埃兹蛋白结合磷蛋白)家族和ERM(埃兹蛋白/根蛋白/莫西蛋白)家族蛋白中的一系列蛋白相互作用模块将受体与肌动蛋白连接起来。然而,尚不清楚这种肌动蛋白连接是否足以重现序列依赖性再循环的自然特征。我们使用一种受体融合方法解决了这个问题,该方法基于PDZbd与一种不同的GPCR(δ阿片受体)融合时促进再循环的能力,δ阿片受体在HEK293细胞中通常再循环效率低下。介导肌动蛋白连接的模块化结构域促进受体再循环的效率与PDZbd本身相似,并且所有结构域促进的再循环都依赖于肌动蛋白。然而,Hrs对受体再循环的调节仅由PDZbd赋予,而不是由下游相互作用模块赋予。这些结果表明,肌动蛋白连接足以模拟GPCR连接的PDZbd的核心再循环活性,但不能模拟其细胞调节。

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