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GrpE通过缔合置换机制加速分子伴侣DnaK的核苷酸交换。

GrpE accelerates nucleotide exchange of the molecular chaperone DnaK with an associative displacement mechanism.

作者信息

Packschies L, Theyssen H, Buchberger A, Bukau B, Goody R S, Reinstein J

机构信息

Abteilung Physikalische Biochemie, Max-Planck-Institut für Molekulare Physiologie, Dortmund, Germay.

出版信息

Biochemistry. 1997 Mar 25;36(12):3417-22. doi: 10.1021/bi962835l.

DOI:10.1021/bi962835l
PMID:9131990
Abstract

The ATP hydrolysis and protein-binding and release cycle of the molecular chaperone DnaK is regulated by the accessory proteins GrpE and DnaJ. Here we describe a study of the formation of complexes between the molecular chaperone DnaK, its nucleotide exchange factor GrpE, and the fluorescent ADP analog N8-[4-[(N'-methylanthraniloyl)amino]butyl]-8-aminoadenosine 5'-diphosphate (MABA-ADP) by equilibrium and stopped flow kinetic experiments. The catalytic cycle of the GrpE-stimulated nucleotide exchange involves a ternary DnaK x GrpE x ADP complex as well as the binary DnaK x GrpE and DnaK x ADP complexes. The equilibrium data of the interaction of GrpE with DnaK x ADP and the nucleotide-free DnaK can be described by a simple equilibrium system where GrpE reduces the affinity of ADP for DnaK 200-fold. However, transient kinetic studies revealed that the functional cycle of GrpE in addition includes at least two distinct ternary DnaK x GrpE x ADP complexes. Our data indicate that the initial weak binding of GrpE to DnaK x ADP is followed by an isomerization of the ternary complex which leads to weakening of nucleotide binding and finally to its rapid dissociation. The maximal stimulation for nucleotide exchange brought about by GrpE was found to be 5000-fold. We propose that this kinetically observed isomerization represents a structural change (opening) of the nucleotide binding pocket of DnaK that allows for fast nucleotide exchange.

摘要

分子伴侣DnaK的ATP水解以及蛋白质结合与释放循环受辅助蛋白GrpE和DnaJ的调控。在此,我们通过平衡和停流动力学实验描述了一项关于分子伴侣DnaK、其核苷酸交换因子GrpE与荧光ADP类似物N8-[4-[(N'-甲基邻氨基苯甲酰基)氨基]丁基]-8-氨基腺苷5'-二磷酸(MABA-ADP)之间复合物形成的研究。GrpE刺激的核苷酸交换催化循环涉及三元DnaK x GrpE x ADP复合物以及二元DnaK x GrpE和DnaK x ADP复合物。GrpE与DnaK x ADP以及无核苷酸DnaK相互作用的平衡数据可以用一个简单的平衡系统来描述,其中GrpE将ADP对DnaK的亲和力降低了200倍。然而,瞬态动力学研究表明,GrpE的功能循环还至少包括两种不同的三元DnaK x GrpE x ADP复合物。我们的数据表明,GrpE与DnaK x ADP最初的弱结合之后是三元复合物的异构化,这导致核苷酸结合减弱并最终使其快速解离。发现GrpE对核苷酸交换的最大刺激为5000倍。我们提出,这种动力学观察到的异构化代表了DnaK核苷酸结合口袋的结构变化(开放),从而允许快速的核苷酸交换。

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