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人碳酸酐酶II的自旋标记变体与GroEL之间相互作用的电子顺磁共振图谱:相互作用导致疏水核心灵活性增加的证据。

EPR mapping of interactions between spin-labeled variants of human carbonic anhydrase II and GroEL: evidence for increased flexibility of the hydrophobic core by the interaction.

作者信息

Persson M, Hammarström P, Lindgren M, Jonsson B H, Svensson M, Carlsson U

机构信息

IFM-Department of Chemistry, Linköping University, Sweden.

出版信息

Biochemistry. 1999 Jan 5;38(1):432-41. doi: 10.1021/bi981442e.

Abstract

Human carbonic anhydrase II (HCA II) interacts weakly with GroEL at room temperature. To further investigate this interaction we used electron paramagnetic resonance (EPR) spectroscopy to study HCA II cysteine mutants spin-labeled at selected positions. From our results it is evident that protein-protein interactions can be specifically mapped by site-directed spin-labeling and EPR measurements. HCA II needs to be unfolded to about the same extent as a GuHCl-induced molten-globule intermediate of the enzyme to interact with GroEL. The interaction with GroEL includes interactions with outer parts of the HCA II molecule, such as peripheral beta-strands and the N-terminal domain, which have previously been shown to be rather unstable. As a result of the interaction, the rigid and compact hydrophobic core exhibits higher flexibility than in the molten globule, which is likely to facilitate rearrangements of misfolded structure during the folding process. The degree of binding to GroEL and accompanying inactivation of the enzyme depend on the stability of the HCA II variant, and nonspecific hydrophobic interactions appear to be most important in stabilizing the GroEL-substrate complex.

摘要

人碳酸酐酶II(HCA II)在室温下与GroEL的相互作用较弱。为了进一步研究这种相互作用,我们使用电子顺磁共振(EPR)光谱来研究在选定位置进行自旋标记的HCA II半胱氨酸突变体。从我们的结果可以明显看出,蛋白质-蛋白质相互作用可以通过定点自旋标记和EPR测量来特异性地绘制。HCA II需要展开到与该酶的盐酸胍诱导的熔球中间体大致相同的程度才能与GroEL相互作用。与GroEL的相互作用包括与HCA II分子外部部分的相互作用,例如外周β链和N端结构域,这些部分先前已被证明相当不稳定。由于这种相互作用,刚性且紧密的疏水核心表现出比熔球更高的灵活性,这可能有助于在折叠过程中重排错误折叠的结构。与GroEL的结合程度以及伴随的酶失活程度取决于HCA II变体的稳定性,并且非特异性疏水相互作用似乎在稳定GroEL-底物复合物中最为重要。

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