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异源三聚体G蛋白与小窝蛋白之间存在调控相互作用的证据。

Evidence for a regulated interaction between heterotrimeric G proteins and caveolin.

作者信息

Li S, Okamoto T, Chun M, Sargiacomo M, Casanova J E, Hansen S H, Nishimoto I, Lisanti M P

机构信息

Whitehead Institute for Biomedical Research, Cambridge, Massachusetts 02142-1479, USA.

出版信息

J Biol Chem. 1995 Jun 30;270(26):15693-701. doi: 10.1074/jbc.270.26.15693.

DOI:10.1074/jbc.270.26.15693
PMID:7797570
Abstract

Caveolae are flask-shaped plasma membrane specializations. A 22-kDa protein, caveolin, is a principal component of caveolar membranes in vivo. As recent evidence suggests that caveolae may participate in G protein-coupled signaling events, we have investigated the potential interaction of caveolin with heterotrimeric G proteins. Using cell fractionation techniques, we found that mutational or pharmacologic activation of Gs alpha prevents its cofractionation with caveolin. In a second independent approach, we directly examined the interaction of G proteins with caveolin. For this purpose, we recombinantly expressed caveolin as a glutathione S-transferase fusion protein. Using an in vitro binding assay, we found that caveolin interacts with G protein alpha subunits (Gs, Go, and Gi). Mutational or pharmacologic activation (with guanosine 5'-O-(thiotriphosphate)) of G alpha subunits prevents this interaction, indicating that the inactive GDP-bound form of G alpha subunits preferentially interacts with caveolin. This G protein binding activity is located within a 41-amino acid region of caveolin's cytoplasmic N-terminal domain (residues 61-101). Further functional analysis shows that a polypeptide derived from this region of caveolin (residues 82-101) effectively suppresses the basal activity of purified G proteins, apparently by inhibiting GDP/GTP exchange. This caveolin sequence is homologous to a region of the Rab GDP dissociation inhibitor, a known inhibitor of GDP/GTP exchange for Rab proteins. These data suggest that caveolin could function to negatively regulate the activation state of heterotrimeric G proteins.

摘要

小窝是烧瓶状的质膜特化结构。一种22 kDa的蛋白质——小窝蛋白,是体内小窝膜的主要成分。由于最近有证据表明小窝可能参与G蛋白偶联信号事件,我们研究了小窝蛋白与异源三聚体G蛋白之间的潜在相互作用。使用细胞分级分离技术,我们发现Gsα的突变激活或药物激活会阻止其与小窝蛋白的共分级分离。在第二种独立方法中,我们直接检测了G蛋白与小窝蛋白的相互作用。为此,我们将小窝蛋白重组表达为谷胱甘肽S-转移酶融合蛋白。使用体外结合试验,我们发现小窝蛋白与G蛋白α亚基(Gs、Go和Gi)相互作用。Gα亚基的突变激活或药物激活(用鸟苷5'-O-(硫代三磷酸))会阻止这种相互作用,这表明Gα亚基的无活性GDP结合形式优先与小窝蛋白相互作用。这种G蛋白结合活性位于小窝蛋白胞质N端结构域的一个41个氨基酸区域内(第61 - 101位氨基酸)。进一步的功能分析表明,源自小窝蛋白该区域的一种多肽(第82 - 101位氨基酸)能有效抑制纯化的G蛋白的基础活性,显然是通过抑制GDP / GTP交换来实现的。这个小窝蛋白序列与Rab GDP解离抑制剂的一个区域同源,Rab GDP解离抑制剂是一种已知的Rab蛋白GDP / GTP交换抑制剂。这些数据表明,小窝蛋白可能起到负调节异源三聚体G蛋白激活状态的作用。

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