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CXXC 基序:活性位点中的变阻器

The CXXC motif: a rheostat in the active site.

作者信息

Chivers P T, Prehoda K E, Raines R T

机构信息

Department of Biochemistry, University of Wisconsin-Madison, 53706, USA.

出版信息

Biochemistry. 1997 Apr 8;36(14):4061-6. doi: 10.1021/bi9628580.

Abstract

The active-site CXXC motif of thiol:disulfide oxidoreductases is essential for their catalysis of redox reactions. Changing the XX residues can perturb the reduction potential of the active-site disulfide bond of the Escherichia coli enzymes thioredoxin (Trx; CGPC) and DsbA (CPHC). The reduction potential is correlated with the acidity of the N-terminal cysteine residue of the CXXC motif. As the pKa is lowered, the disulfide bond becomes more easy to reduce. A change in pKa can account fully for a change in reduction potential in well-characterized CXXC motifs of DsbA but not of Trx. Formal analysis of the Nernst equation reveals that reduction potential contains both pH-dependent and pH-independent components. Indeed, the difference between the reduction potentials of wild-type Trx and wild-type DsbA cannot be explained solely by differences in thiol pKa values. Structural data for thiol:disulfide oxidoreductases reveal no single factor that determines the pH-independent component of the reduction potential. In addition, the pH-dependent component is complex when the redox state of the CXXC motif affects the titration of residues other than the thiols. These intricacies enable CXXC motifs to vary widely in their capacity to assist electron flow, and thereby engender a family of thiol:disulfide oxidoreductases that play diverse roles in biochemistry.

摘要

硫醇

二硫键氧化还原酶的活性位点CXXC基序对其催化氧化还原反应至关重要。改变XX残基会扰乱大肠杆菌酶硫氧还蛋白(Trx;CGPC)和DsbA(CPHC)活性位点二硫键的还原电位。还原电位与CXXC基序N端半胱氨酸残基的酸度相关。随着pKa降低,二硫键变得更容易还原。pKa的变化可以完全解释DsbA中特征明确的CXXC基序还原电位的变化,但不能解释Trx的变化。对能斯特方程的形式分析表明,还原电位包含pH依赖和pH独立成分。事实上,野生型Trx和野生型DsbA还原电位的差异不能仅用硫醇pKa值的差异来解释。硫醇:二硫键氧化还原酶的结构数据显示,没有单一因素能决定还原电位的pH独立成分。此外,当CXXC基序的氧化还原状态影响除硫醇以外的残基滴定时,pH依赖成分很复杂。这些复杂性使得CXXC基序在协助电子流动的能力上有很大差异,从而产生了一类在生物化学中发挥不同作用的硫醇:二硫键氧化还原酶。

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