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人硫氧还蛋白中结构半胱氨酸残基的诱变及其对硒代二谷胱甘肽调节活性的影响。

Mutagenesis of structural half-cystine residues in human thioredoxin and effects on the regulation of activity by selenodiglutathione.

作者信息

Ren X, Björnstedt M, Shen B, Ericson M L, Holmgren A

机构信息

Department of Biochemistry I, Medical Nobel Institute, Karolinska Institutet, Stockholm, Sweden.

出版信息

Biochemistry. 1993 Sep 21;32(37):9701-8. doi: 10.1021/bi00088a023.

Abstract

A human thioredoxin cDNA was modified to optimize Escherichia coli expression and subcloned into the plasmid pACA, a vector for T7 RNA polymerase-directed expression. The substitution of structural (noncatalytic) half-cystines in human thioredoxin (hTrx) was made by site-directed mutagenesis. The recombinant wild-type (wt) hTrx and its mutant C61S, C72S, and C61S/C72S were expressed and purified to homogeneity. Characterization of the wt and mutant hTrx was done with respect to redox activity with thioredoxin reductase (TR), tryptophan fluorescence, and effects of incubation with GS-Se-SG, which is believed to be the major metabolite of inorganic selenium compounds in mammalian tissues. The Km and kcat of wild-type hTrx for human placenta thioredoxin reductase (HP-TR) at pH 7.0 were 2.0 microM and 2800 min-1, respectively. The mutant proteins C61S, C72S, and C61S/C72S had Km and kcat values similar to those of the wt thioredoxin. Tryptophan fluorescence measurements showed that the wt and mutant proteins had similar stability to a denaturing agent. Incubation of fully reduced thioredoxin with 0.1 molar equivalent of GS-Se-SG resulted in continued oxidation of SH groups. After 3.5 h only 0.5 of initially 4.6 SH groups/thioredoxin remained. With the oxidized protein, a pronounced lag phase in thioredoxin reductase-dependent insulin disulfide reduction was present. Disulfide-linked dimers of the protein were present. The results clearly showed that noncatalytic cysteine residues in hTrx were oxidized accompanied by dimerization and inactivation. The activities of the mutant proteins C72S and C61S/C72S were unchanged after 3 h of incubation with GS-Se-SG. No dimer appeared of the C72S thioredoxin.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

对人硫氧还蛋白cDNA进行修饰以优化其在大肠杆菌中的表达,并亚克隆到质粒pACA中,pACA是一种用于T7 RNA聚合酶指导表达的载体。通过定点诱变对人硫氧还蛋白(hTrx)中的结构(非催化)半胱氨酸进行替换。表达并纯化重组野生型(wt)hTrx及其突变体C61S、C72S和C61S/C72S,使其达到均一性。对wt和突变体hTrx进行了表征,涉及与硫氧还蛋白还原酶(TR)的氧化还原活性、色氨酸荧光以及与GS-Se-SG孵育的影响,GS-Se-SG被认为是哺乳动物组织中无机硒化合物的主要代谢产物。野生型hTrx对人胎盘硫氧还蛋白还原酶(HP-TR)在pH 7.0时的Km和kcat分别为2.0 microM和2800 min-1。突变蛋白C61S、C72S和C61S/C72S的Km和kcat值与wt硫氧还蛋白相似。色氨酸荧光测量表明,wt和突变蛋白对变性剂具有相似的稳定性。将完全还原的硫氧还蛋白与0.1摩尔当量的GS-Se-SG孵育导致SH基团持续氧化。3.5小时后,最初每个硫氧还蛋白4.6个SH基团中仅剩下0.5个。对于氧化型蛋白,在硫氧还蛋白还原酶依赖性胰岛素二硫键还原过程中存在明显的延迟期。该蛋白存在二硫键连接的二聚体。结果清楚地表明,hTrx中的非催化半胱氨酸残基被氧化并伴随二聚化和失活。与GS-Se-SG孵育3小时后,突变蛋白C72S和C61S/C72S的活性未改变。C72S硫氧还蛋白未出现二聚体。(摘要截短为250字)

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