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粗糙脉孢菌的热休克蛋白80,一种真核应激90家族的胞质分子伴侣,直接与热休克蛋白70相互作用。

Heat shock protein 80 of Neurospora crassa, a cytosolic molecular chaperone of the eukaryotic stress 90 family, interacts directly with heat shock protein 70.

作者信息

Freitag D G, Ouimet P M, Girvitz T L, Kapoor M

机构信息

Department of Biological Sciences, University of Calgary, Calgary, Alberta, Canada T2N 1N4.

出版信息

Biochemistry. 1997 Aug 19;36(33):10221-9. doi: 10.1021/bi963030g.

DOI:10.1021/bi963030g
PMID:9254620
Abstract

The subunit structure of Hsp80, the most abundant heat-shock protein of Neurospora crassa, was examined by chemical cross-linking of the purified protein in vitro. Resolution of glutaraldehyde-treated Hsp80 by sodium dodecyl sulfate-polyacrylamide gel electrophoresis SDS-PAGE suggests that the native state of this protein is a tetramer; the relative proportion of cross-linked species, estimated by the fraction of protein recovered in each category, is consistent with a dimer-of-dimer structure. Upon interaction with nucleotides, higher order cross-linked oligomers were detected, indicating ligand-induced conformational changes. The effect of nucleotides was also monitored by following tryptophan fluorescence: CTP, UTP, and NAD led to fluorescence quenching, the effect of CTP being the most pronounced. As individual molecular chaperones often act in concert with cochaperones, interaction between the two major cytosolic stress proteins--Hsp80 and Hsp70--was examined. Purified Hsp70 was immobilized on ATP-agarose and purified Hsp80 was applied to the Hsp70-saturated matrix; while Hsp80 did not bind to ATP-agarose by itself, it was bound strongly by immobilized Hsp70. The [Hsp70-Hsp80] complex was eluted with ATP and coelution of both proteins was confirmed by Western blot analysis, using specific polyclonal antibodies raised against each protein. The physical association of stress-inducible Hsp70 and Hsp80 was verified by interprotein cross-linking in vitro followed by immunoblot analysis and by immunoprecipitation.

摘要

粗糙脉孢菌中最丰富的热休克蛋白Hsp80的亚基结构,通过体外对纯化蛋白进行化学交联来检测。经十二烷基硫酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)分析戊二醛处理后的Hsp80,结果表明该蛋白的天然状态是四聚体;通过每一类中回收的蛋白比例估算交联物种的相对比例,与二聚体-二聚体结构一致。与核苷酸相互作用时,检测到更高阶的交联寡聚体,表明配体诱导的构象变化。还通过跟踪色氨酸荧光监测核苷酸的作用:CTP、UTP和NAD导致荧光猝灭,其中CTP的作用最为明显。由于单个分子伴侣通常与共伴侣协同作用,因此研究了两种主要的胞质应激蛋白——Hsp80和Hsp70之间的相互作用。将纯化的Hsp70固定在ATP-琼脂糖上,并将纯化的Hsp80应用于Hsp70饱和的基质;虽然Hsp80自身不与ATP-琼脂糖结合,但它能与固定化的Hsp70强烈结合。用ATP洗脱[Hsp70-Hsp80]复合物,并用针对每种蛋白产生的特异性多克隆抗体通过蛋白质印迹分析确认两种蛋白的共洗脱。通过体外蛋白间交联,随后进行免疫印迹分析和免疫沉淀,验证了应激诱导型Hsp70和Hsp80的物理缔合。

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