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综述:分子伴侣介导的稳定蛋白质聚集体解聚与重折叠机制

Review: mechanisms of disaggregation and refolding of stable protein aggregates by molecular chaperones.

作者信息

Ben-Zvi A P, Goloubinoff P

机构信息

Department of Plant Sciences, A Silberman Institute of Life Sciences, The Hebrew University of Jerusalem, Jerusalem, 91904, Israel.

出版信息

J Struct Biol. 2001 Aug;135(2):84-93. doi: 10.1006/jsbi.2001.4352.

DOI:10.1006/jsbi.2001.4352
PMID:11580258
Abstract

Molecular chaperones are essential for the correct folding of proteins in the cell under physiological and stress conditions. Two activities have been traditionally attributed to molecular chaperones: (1) preventing aggregation of unfolded polypeptides and (2) assisting in the correct refolding of chaperone-bound denatured polypeptides. We discuss here a novel function of molecular chaperones: catalytic solubilization and refolding of stable protein aggregates. In Escherichia coli, disaggregation is carried out by a network of ATPase chaperones consisting of a DnaK core, assisted by the cochaperones DnaJ, GrpE, ClpB, and GroEL-GroES. We suggest a sequential mechanism in which (a) ClpB exposes new DnaK-binding sites on the surface of the stable protein aggregates; (b) DnaK binds the aggregate surfaces and, by doing so, melts the incorrect hydrophobic associations between aggregated polypeptides; (c) ATP hydrolysis and DnaK release allow local intramolecular refolding of native domains, leading to a gradual weakening of improper intermolecular links; (d) DnaK and GroEL complete refolding of solubilized polypeptide chains into native proteins. Thus, active disaggregation by the chaperone network can serve as a central cellular tool for the recovery of native proteins from stress-induced aggregates and actively remove disease-causing toxic aggregates, such as polyglutamine-rich proteins, amyloid plaques, and prions.

摘要

分子伴侣对于细胞中蛋白质在生理和应激条件下的正确折叠至关重要。传统上认为分子伴侣具有两种活性:(1)防止未折叠多肽聚集;(2)协助与分子伴侣结合的变性多肽正确重折叠。我们在此讨论分子伴侣的一种新功能:稳定蛋白质聚集体的催化溶解和重折叠。在大肠杆菌中,解聚由一个由DnaK核心组成的ATPase分子伴侣网络进行,辅伴侣DnaJ、GrpE、ClpB和GroEL-GroES协助。我们提出一种顺序机制,其中:(a)ClpB在稳定蛋白质聚集体表面暴露新的DnaK结合位点;(b)DnaK结合聚集体表面,从而破坏聚集多肽之间不正确的疏水缔合;(c)ATP水解和DnaK释放允许天然结构域进行局部分子内重折叠,导致分子间不正确连接逐渐减弱;(d)DnaK和GroEL将溶解的多肽链完全重折叠成天然蛋白质。因此,分子伴侣网络的活性解聚可作为一种核心细胞工具,用于从应激诱导的聚集体中恢复天然蛋白质,并积极清除致病的毒性聚集体,如富含多聚谷氨酰胺的蛋白质、淀粉样斑块和朊病毒。

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