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通过质谱法探究共伴侣蛋白GroES和gp31的热激活

Thermal activation of the co-chaperonins GroES and gp31 probed by mass spectrometry.

作者信息

Geels Rimco B J, Calmat Stephane, Heck Albert J R, van der Vies Saskia M, Heeren Ron M A

机构信息

FOM Institute for Atomic and Molecular Physics, Kruislaan 407, 1098 SJ Amsterdam, The Netherlands.

出版信息

Rapid Commun Mass Spectrom. 2008 Nov;22(22):3633-41. doi: 10.1002/rcm.3782.

DOI:10.1002/rcm.3782
PMID:18972453
Abstract

Many biological active proteins are assembled in protein complexes. Understanding the (dis)assembly of such complexes is therefore of major interest. Here we use mass spectrometry to monitor the disassembly induced by thermal activation of the heptameric co-chaperonins GroES and gp31. We use native electrospray ionization mass spectrometry (ESI-MS) on a Fourier transform ion cyclotron resonance (FT-ICR) mass spectrometer to monitor the stoichiometry of the chaperonins. A thermally controlled electrospray setup was employed to analyze conformational and stoichiometric changes of the chaperonins at varying temperature. The native ESI-MS data agreed well with data obtained from fluorescence spectroscopy as the measured thermal dissociation temperatures of the complexes were in good agreement. Furthermore, we observed that thermal denaturing of GroES and gp31 proceeds via intermediate steps of all oligomeric forms, with no evidence of a transiently stable unfolded heptamer. We also evaluated the thermal dissociation of the chaperonins in the gas phase using infrared multiphoton dissociation (IRMPD) for thermal activation. Using gas-phase activation the smaller (2-4) oligomers were not detected, only down to the pentamer, whereafter the complex seemed to dissociate completely. These results demonstrate clearly that conformational changes of GroES and gp31 due to heating in solution and in the gas phase are significantly different.

摘要

许多生物活性蛋白是在蛋白质复合物中组装而成的。因此,了解此类复合物的(解)组装过程具有重大意义。在此,我们使用质谱法监测由七聚体共伴侣蛋白GroES和gp31的热激活诱导的解组装过程。我们在傅里叶变换离子回旋共振(FT-ICR)质谱仪上使用原生电喷雾电离质谱(ESI-MS)来监测伴侣蛋白的化学计量。采用热控电喷雾装置分析伴侣蛋白在不同温度下的构象和化学计量变化。原生ESI-MS数据与荧光光谱获得的数据吻合良好,因为测得的复合物热解离温度吻合度很高。此外,我们观察到GroES和gp31的热变性通过所有寡聚形式的中间步骤进行,没有证据表明存在瞬时稳定的未折叠七聚体。我们还使用红外多光子解离(IRMPD)进行热激活,评估了气相中伴侣蛋白的热解离。使用气相激活时,未检测到较小的(2-4)寡聚体,仅检测到五聚体,此后复合物似乎完全解离。这些结果清楚地表明,GroES和gp31在溶液中和气相中因加热而发生的构象变化显著不同。

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