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酵母PalA/AIP1/Alix同源物Rim20p与一个类PEST区域相关联,并且是其蛋白水解切割所必需的。

Yeast PalA/AIP1/Alix homolog Rim20p associates with a PEST-like region and is required for its proteolytic cleavage.

作者信息

Xu W, Mitchell A P

机构信息

Department of Microbiology, Integrated Program in Cellular, Molecular, and Biophysical Studies, Columbia University, 701 West 168th Street, New York, NY 10032, USA.

出版信息

J Bacteriol. 2001 Dec;183(23):6917-23. doi: 10.1128/JB.183.23.6917-6923.2001.

Abstract

The Saccharomyces cerevisiae zinc finger protein Rim101p is activated by cleavage of its C-terminal region, which resembles PEST regions that confer susceptibility to proteolysis. Here we report that Rim20p, a member of the broadly conserved PalA/AIP1/Alix family, is required for Rim101p cleavage. Two-hybrid and coimmunoprecipitation assays indicate that Rim20p binds to Rim101p, and a two-hybrid assay shows that the Rim101p PEST-like region is sufficient for Rim20p binding. Rim101p-Rim20p interaction is conserved in Candida albicans, supporting the idea that interaction is functionally significant. Analysis of Rim20p mutant proteins indicates that some of its broadly conserved regions are required for processing of Rim101p and for stability of Rim20p itself but are not required for interaction with Rim101p. A recent genome-wide two-hybrid study (T. Ito, T. Chiba, R. Ozawa, M. Yoshida, M. Hattori, and Y. Sakaki, Proc. Natl. Acad. Sci. USA 98:4569-4574, 2000) indicates that Rim20p interacts with Snf7p and that Snf7p interacts with Rim13p, a cysteine protease required for Rim101p proteolysis. We suggest that Rim20p may serve as part of a scaffold that places Rim101p and Rim13p in close proximity.

摘要

酿酒酵母锌指蛋白Rim101p通过其C端区域的切割而被激活,该C端区域类似于赋予蛋白水解敏感性的PEST区域。在此我们报道,广泛保守的PalA/AIP1/Alix家族成员Rim20p是Rim101p切割所必需的。双杂交和免疫共沉淀分析表明Rim20p与Rim101p结合,并且双杂交分析表明Rim101p的PEST样区域足以与Rim20p结合。Rim101p与Rim20p的相互作用在白色念珠菌中保守,这支持了这种相互作用具有功能重要性的观点。对Rim20p突变蛋白的分析表明,其一些广泛保守的区域是Rim101p加工和Rim20p自身稳定性所必需的,但不是与Rim101p相互作用所必需的。最近一项全基因组双杂交研究(T. Ito、T. Chiba、R. Ozawa、M. Yoshida、M. Hattori和Y. Sakaki,《美国国家科学院院刊》98:4569 - 4574,2000)表明Rim20p与Snf7p相互作用,并且Snf7p与Rim13p相互作用,Rim13p是Rim101p蛋白水解所需的一种半胱氨酸蛋白酶。我们认为Rim20p可能作为一种支架的一部分,使Rim101p和Rim13p紧密靠近。

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