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Ras与小窝蛋白(一种小窝微区的整合膜蛋白)的共纯化及直接相互作用。无去污剂纯化小窝微区。

Co-purification and direct interaction of Ras with caveolin, an integral membrane protein of caveolae microdomains. Detergent-free purification of caveolae microdomains.

作者信息

Song K S, Okamoto T, Quilliam L A, Sargiacomo M, Lisanti M P

机构信息

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

出版信息

J Biol Chem. 1996 Apr 19;271(16):9690-7. doi: 10.1074/jbc.271.16.9690.

DOI:10.1074/jbc.271.16.9690
PMID:8621645
Abstract

Caveolae are plasma membrane specializations that have been implicated in signal transduction. Caveolin, a 21-24-kDa integral membrane protein, is a principal structural component of caveolae membranes in vivo. G protein alpha subunits are concentrated in purified preparations of caveolae membranes, and caveolin interacts directly with multiple G protein alpha subunits, including G(s), G(o), and G(i2). Mutational or pharmacologic activation of G alpha subunits prevents the interaction of caveolin with G proteins, indicating that inactive G alpha subunits preferentially interact with caveolin. Here, we show that caveolin interacts with another well characterized signal transducer, Ras. Using a detergent-free procedure for purification of caveolin-rich membrane domains and a polyhistidine tagged form of caveolin, we find that Ras and other classes of lipid-modified signaling molecules co-fractionate and co-elute with caveolin. The association of Ras with caveolin was further evaluated using two distinct in vitro binding assays. Wild-type H-Ras interacted with glutathione S-transferase (GST)-caveolin fusion proteins but not with GST alone. Using a battery of GST fusion proteins encoding distinct regions of caveolin, Ras binding activity was localized to a 41-amino acid membrane proximal region of the cytosolic N-terminal domain of caveolin. In addition, reconstituted caveolin-rich membranes (prepared with purified recombinant caveolin and purified lipids) interacted with a soluble form of wild-type H-Ras but failed to interact with mutationally activated soluble H-Ras (G12V). Thus, a single amino acid change (G12V) that constitutively activates Ras prevents or destabilizes this interaction. These results clearly indicate that (i) caveolin is sufficient to recruit soluble Ras onto lipid membranes and (ii) membrane-bound caveolin preferentially interacts with inactive Ras proteins. In direct support of these in vitro studies, we also show that recombinant overexpression of caveolin in intact cells is sufficient to functionally recruit a nonfarnesylated mutant of Ras (C186S) onto membranes, overcoming the normal requirement for lipid modification of Ras. Taken together, these observations suggest that caveolin may function as a scaffolding protein to localize or sequester certain caveolin-interacting proteins, such as wild-type Ras, within caveolin-rich microdomains of the plasma membrane.

摘要

小窝是质膜特化结构,与信号转导有关。小窝蛋白是一种21 - 24 kDa的整合膜蛋白,是体内小窝膜的主要结构成分。G蛋白α亚基集中在纯化的小窝膜制剂中,小窝蛋白直接与多种G蛋白α亚基相互作用,包括G(s)、G(o)和G(i2)。Gα亚基的突变激活或药物激活会阻止小窝蛋白与G蛋白的相互作用,这表明无活性的Gα亚基优先与小窝蛋白相互作用。在此,我们表明小窝蛋白与另一种特征明确的信号转导分子Ras相互作用。使用无去污剂的方法纯化富含小窝蛋白的膜结构域以及一种多组氨酸标签形式的小窝蛋白,我们发现Ras和其他类别的脂质修饰信号分子与小窝蛋白共分级分离并共洗脱。使用两种不同的体外结合试验进一步评估了Ras与小窝蛋白的结合。野生型H-Ras与谷胱甘肽S-转移酶(GST)-小窝蛋白融合蛋白相互作用,但不与单独的GST相互作用。使用一系列编码小窝蛋白不同区域的GST融合蛋白,Ras结合活性定位于小窝蛋白胞质N端结构域的一个41个氨基酸的膜近端区域。此外,重组的富含小窝蛋白的膜(用纯化的重组小窝蛋白和纯化的脂质制备)与野生型H-Ras的可溶性形式相互作用,但不与突变激活的可溶性H-Ras(G12V)相互作用。因此,组成性激活Ras的单个氨基酸变化(G12V)会阻止或破坏这种相互作用。这些结果清楚地表明:(i)小窝蛋白足以将可溶性Ras募集到脂质膜上;(ii)膜结合的小窝蛋白优先与无活性的Ras蛋白相互作用。作为这些体外研究的直接支持,我们还表明在完整细胞中重组过表达小窝蛋白足以在功能上将Ras的非法尼基化突变体(C186S)募集到膜上,克服了Ras脂质修饰的正常需求。综上所述,这些观察结果表明小窝蛋白可能作为一种支架蛋白,在质膜富含小窝蛋白的微结构域内定位或隔离某些与小窝蛋白相互作用的蛋白,如野生型Ras。

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