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Back to GroEL-Assisted Protein Folding: GroES Binding-Induced Displacement of Denatured Proteins from GroEL to Bulk Solution

机译:返回到GroEL辅助的蛋白质折叠:GroES结合引起的变性蛋白质从GroEL到大体积溶液的置换

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摘要

The main events in chaperone-assisted protein folding are the binding and ligand-induced release of substrate proteins. Here, we studied the location of denatured proteins previously bound to the GroEL chaperonin resulting from the action of the GroES co-chaperonin in the presence of Mg-ATP. Fluorescein-labeled denatured proteins (α-lactalbumin, lysozyme, serum albumin, and pepsin in the presence of thiol reagents at neutral pH, as well as an early refolding intermediate of malate dehydrogenase) were used to reveal the effect of GroES on their interaction with GroEL. Native electrophoresis has demonstrated that these proteins tend to be released from the GroEL-GroES complex. With the use of biotin- and fluorescein-labeled denatured proteins and streptavidin fused with luciferase aequorin (the so-called streptavidin trap), the presence of denatured proteins in bulk solution after GroES and Mg-ATP addition has been confirmed. The time of GroES-induced dissociation of a denatured protein from the GroEL surface was estimated using the stopped-flow technique and found to be much shorter than the proposed time of the GroEL ATPase cycle.
机译:伴侣蛋白折叠中的主要事件是底物蛋白的结合和配体诱导的释放。在这里,我们研究了在Mg-ATP存在下,GroES伴侣蛋白的作用导致先前与GroEL伴侣蛋白结合的变性蛋白的位置。荧光素标记的变性蛋白(α-乳清蛋白,溶菌酶,血清白蛋白和胃蛋白酶,在中性pH下存在硫醇试剂的情况下,以及苹果酸脱氢酶的早期重折叠中间体)用于揭示GroES对它们与蛋白相互作用的影响GroEL。天然电泳表明,这些蛋白质倾向于从GroEL-GroES复合物中释放。通过使用生物素和荧光素标记的变性蛋白以及与荧光素酶水母发光蛋白融合的链霉亲和素(所谓的链霉亲和素陷阱),已证实在添加GroES和Mg-ATP后散装溶液中存在变性蛋白。使用停止流技术估算了GroES诱导的变性蛋白质从GroEL表面解离的时间,发现该时间比拟议的GroEL ATPase循环时间短得多。

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