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GroEL顶端结构域构象变化的停流荧光分析:顶端结构域运动与GroEL四级结构之间的关系。

Stopped-flow fluorescence analysis of the conformational changes in the GroEL apical domain: relationships between movements in the apical domain and the quaternary structure of GroEL.

作者信息

Taniguchi Masaaki, Yoshimi Tatsunari, Hongo Kunihiro, Mizobata Tomohiro, Kawata Yasushi

机构信息

Department of Biotechnology, Faculty of Engineering, Insitute of Regenerative Medicine and Biofunction, Graduate School of Medical Sciences, Tottori University, Tottori, Japan.

出版信息

J Biol Chem. 2004 Apr 16;279(16):16368-76. doi: 10.1074/jbc.M311806200. Epub 2004 Jan 20.

Abstract

GroEL undergoes numerous conformational alterations in the course of facilitating the folding of various proteins, and the specific movements of the GroEL apical domain are of particular importance in the molecular mechanism. In order to monitor in detail the numerous movements of the GroEL apical domain, we have constructed a mutant chaperonin (GroEL R231W) with wild type-like function and a fluorescent probe introduced into the apical domain. By monitoring the tryptophan fluorescence changes of GroEL R231W upon ATP addition in the presence and absence of the co-chaperonin GroES, we detected a total of four distinct kinetic phases that corresponded to conformational changes of the apical domain and GroES binding. By introducing this mutation into a single ring variant of GroEL (GroEL SR-1), we determined the extent of inter-ring cooperation that was involved in apical domain movements. Surprisingly, we found that the apical domain movements of GroEL were affected only slightly by the change in quaternary structure. Our experiments provide a number of novel insights regarding the dynamic movements of this protein.

摘要

在促进各种蛋白质折叠的过程中,GroEL会经历众多构象变化,而GroEL顶端结构域的特定运动在分子机制中尤为重要。为了详细监测GroEL顶端结构域的众多运动,我们构建了一个具有野生型样功能且在顶端结构域引入荧光探针的突变伴侣蛋白(GroEL R231W)。通过在存在和不存在共伴侣蛋白GroES的情况下监测添加ATP后GroEL R231W的色氨酸荧光变化,我们总共检测到四个不同的动力学阶段,它们对应于顶端结构域的构象变化和GroES结合。通过将此突变引入GroEL的单环变体(GroEL SR - 1)中,我们确定了参与顶端结构域运动的环间协作程度。令人惊讶的是,我们发现GroEL的顶端结构域运动仅受到四级结构变化的轻微影响。我们的实验提供了关于这种蛋白质动态运动的许多新见解。

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