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人晶状体βB2-晶体蛋白的结构域相互作用位点

Domain interaction sites of human lens betaB2-crystallin.

作者信息

Liu Bing-Fen, Liang Jack J-N

机构信息

Center for Ophthalmic Research/Surgery, Brigham and Women's Hospital, and Department of Ophthalmology, Harvard Medical School, Boston, Massachusetts 02115, USA.

出版信息

J Biol Chem. 2006 Feb 3;281(5):2624-30. doi: 10.1074/jbc.M509017200. Epub 2005 Nov 29.

DOI:10.1074/jbc.M509017200
PMID:16319073
Abstract

betaB2-crystallin, the major component of beta-crystallin, is a dimer at low concentrations but can form oligomers under physiological conditions. The interaction domains have been speculated to be the beta-sheets, each of which is formed by two or more beta-strands. betaB2-crystallin consists of 16 beta-strands, 8 in the N-terminal domain and 8 in the C-terminal domain. Domain interaction sites may be removed by destroying the beta-strands, which can be done by site-specific mutations, substituting the beta-formers (Val, Phe, Leu) with Glu or Asn, strong beta-breakers. We have cloned the following beta-strand-deleted mutants, I20E, L34E, V54E, V60E, V73E, L97E, I109E, I124E, V144E, V152E, L162E, L165E, and V187E and their corresponding X --> Asn mutants. We also made two mutants, V46E and V129E, that were not on the beta-strand as controls. Disruption of protein-protein interactions was screened by a mammalian two-hybrid system assay. Protein-protein interactions decreased for all beta-strand-deleted mutants except I20E, L34E, and L162E mutants; this effect was not seen in the two mutant controls, V46E and V129E. The sequences around Val-54, Val-60, Val-73, and Leu-97 in the N-terminal region and Ile-109, Ile-124, Val-144, Val-152, Leu-165, and Val-187 in the C-terminal region that formed beta-strands appear to be important in dimerization. Some selected mutant proteins that showed strong (V46E and V129E) and reduced (V60E, V144E, V60N, and V144N) interactions were expressed in bacterial culture and were studied with spectroscopy and chromatography. The V60E and V144E mutants were found to be partially unfolded and incapable of forming a complete dimer.

摘要

βB2-晶状体蛋白是β-晶状体蛋白的主要成分,在低浓度时为二聚体,但在生理条件下可形成寡聚体。推测其相互作用结构域为β折叠片层,每个β折叠片层由两条或更多条β链组成。βB2-晶状体蛋白由16条β链组成,N端结构域有8条,C端结构域有8条。通过破坏β链可去除结构域相互作用位点,这可通过位点特异性突变来实现,即将β链形成者(缬氨酸、苯丙氨酸、亮氨酸)替换为谷氨酸或天冬酰胺,它们是强效的β链破坏者。我们克隆了以下β链缺失突变体:I20E、L34E、V54E、V60E、V73E、L97E、I109E、I124E、V144E、V152E、L162E、L165E和V187E以及它们相应的X→天冬酰胺突变体。我们还制备了两个不在β链上的突变体V46E和V129E作为对照。通过哺乳动物双杂交系统测定筛选蛋白质-蛋白质相互作用的破坏情况。除I20E、L34E和L162E突变体外,所有β链缺失突变体的蛋白质-蛋白质相互作用均降低;在两个突变体对照V46E和V129E中未观察到这种效应。N端区域中缬氨酸-54、缬氨酸-60、缬氨酸-73和亮氨酸-97以及C端区域中异亮氨酸-109、异亮氨酸-124、缬氨酸-144、缬氨酸-152、亮氨酸-165和缬氨酸-187周围形成β链的序列似乎在二聚化中起重要作用。一些显示出强相互作用(V

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