首页> 美国卫生研究院文献>The EMBO Journal >DnaK DnaJ and GrpE form a cellular chaperone machinery capable of repairing heat-induced protein damage.
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DnaK DnaJ and GrpE form a cellular chaperone machinery capable of repairing heat-induced protein damage.

机译:DnaKDnaJ和GrpE形成了一种细胞伴侣分子机制能够修复热诱导的蛋白质损伤。

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摘要

Members of the conserved Hsp70 chaperone family are assumed to constitute a main cellular system for the prevention and the amelioration of stress-induced protein damage, though little direct evidence exists for this function. We investigated the roles of the DnaK (Hsp70), DnaJ and GrpE chaperones of Escherichia coli in prevention and repair of thermally induced protein damage using firefly luciferase as a test substrate. In vivo, luciferase was rapidly inactivated at 42 degrees C, but was efficiently reactivated to 50% of its initial activity during subsequent incubation at 30 degrees C. DnaK, DnaJ and GrpE did not prevent luciferase inactivation, but were essential for its reactivation. In vitro, reactivation of heat-inactivated luciferase to 80% of its initial activity required the combined activity of DnaK, DnaJ and GrpE as well as ATP, but not GroEL and GroES. DnaJ associated with denatured luciferase, targeted DnaK to the substrate and co-operated with DnaK to prevent luciferase aggregation at 42 degrees C, an activity that was required for subsequent reactivation. The protein repair function of DnaK, GrpE and, in particular, DnaJ is likely to be part of the role of these proteins in regulation of the heat shock response.
机译:保守的Hsp70伴侣家族成员被认为构成了预防和改善应激诱导的蛋白质损伤的主要细胞系统,尽管很少有直接证据表明该功能。我们调查了萤火虫荧光素酶作为测试底物,大肠杆菌的DnaK(Hsp70),DnaJ和GrpE分子伴侣在预防和修复热诱导蛋白质损伤中的作用。在体内,萤光素酶在42摄氏度下迅速失活,但在随后于30摄氏度的孵育过程中被有效地重新活化至其初始活性的50%。DnaK,DnaJ和GrpE不能阻止萤光素酶的失活,但对其重新活化至关重要。在体外,将热灭活的荧光素酶重新激活至其初始活性的80%,需要DnaK,DnaJ和GrpE以及ATP的组合活性,但不需要GroEL和GroES。与变性的萤光素酶相关的DnaJ将DnaK靶向底物,并与DnaK协同作用以防止萤光素酶在42摄氏度下聚集,这是后续重新激活所必需的活性。 DnaK,GrpE尤其是DnaJ的蛋白质修复功能可能是这些蛋白质在调节热激反应中所起的作用的一部分。

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