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热休克蛋白90(Hsp90)ATP结合特性的评估

Assessment of the ATP binding properties of Hsp90.

作者信息

Jakob U, Scheibel T, Bose S, Reinstein J, Buchner J

机构信息

Institut für Biophysik und Physikalische Biochemie, Universität Regensburg, 93040 Regensburg, Federal Republic of Germany.

出版信息

J Biol Chem. 1996 Apr 26;271(17):10035-41. doi: 10.1074/jbc.271.17.10035.

DOI:10.1074/jbc.271.17.10035
PMID:8626558
Abstract

Hsp90, one of the most prominent proteins in eucaryotic cells under physiological and stress conditions, chaperones protein folding reactions in an ATP-independent way. Surprisingly, ATP binding and ATPase activity of Hsp90 has been reported by several groups. To clarify this important issue, we have reinvestigated the potential ATP binding properties and ATPase activity of highly purified Hsp90 using a number of different techniques. Hsp90 was compared to the well characterized ATP-binding chaperone Hsc70 and to two control proteins, immunoglobulin G and bovine serum albumin, that are known to not bind ATP. Hsp90 behaved very similarly to the non-ATP-binding proteins and very differently from the ATP-binding protein Hsc70. Like bovine serum albumin and immunoglobulin G, Hsp90 (i) did not bind to immobilized ATP, (ii) could not be specifically photocross-linked with azido-ATP, (iii) failed to exhibit significant changes in intrinsic protein fluorescence upon ATP addition, and (iv) did not bind to three fluorescent ADP analogues. In contrast, Hsc70 strongly bound ATP and ADP, specifically cross-linked with azido-ATP, and exhibited major shifts in fluorescence upon addition of ATP. Finally, reexamination of the amino acid sequence of Hsp90 failed to reveal any significant homologies to known ATP-binding motifs. Taken together, we conclude that highly purified Hsp90 does not bind ATP. Weak ATPase activities associated with Hsp90 preparations may be due to minor impurities or kinases copurifying with Hsp90.

摘要

Hsp90是真核细胞在生理和应激条件下最显著的蛋白质之一,它以不依赖ATP的方式协助蛋白质折叠反应。令人惊讶的是,有几个研究小组报道了Hsp90具有ATP结合和ATP酶活性。为了阐明这个重要问题,我们使用多种不同技术重新研究了高度纯化的Hsp90的潜在ATP结合特性和ATP酶活性。将Hsp90与已明确其ATP结合特性的伴侣蛋白Hsc70以及两种已知不结合ATP的对照蛋白(免疫球蛋白G和牛血清白蛋白)进行比较。Hsp90的行为与非ATP结合蛋白非常相似,与ATP结合蛋白Hsc70则有很大不同。与牛血清白蛋白和免疫球蛋白G一样,Hsp90:(i)不与固定化ATP结合;(ii)不能与叠氮基ATP特异性光交联;(iii)添加ATP后其内在蛋白质荧光没有显著变化;(iv)不与三种荧光ADP类似物结合。相比之下,Hsc70能强烈结合ATP和ADP,能与叠氮基ATP特异性交联,添加ATP后荧光有显著变化。最后,对Hsp90氨基酸序列的重新检查未能发现与已知ATP结合基序有任何显著同源性。综上所述,我们得出结论:高度纯化的Hsp90不结合ATP。与Hsp90制剂相关的微弱ATP酶活性可能是由于与Hsp90共纯化的少量杂质或激酶所致。

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