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用硒代半胱氨酸替代催化性半胱氨酸41可增强在大肠杆菌中表达的植物磷脂氢过氧化物谷胱甘肽过氧化物酶的酶活性。

Substituting selenocysteine for catalytic cysteine 41 enhances enzymatic activity of plant phospholipid hydroperoxide glutathione peroxidase expressed in Escherichia coli.

作者信息

Hazebrouck S, Camoin L, Faltin Z, Strosberg A D, Eshdat Y

机构信息

Department of Fruit Tree Breeding and Molecular Genetics, Agricultural Research Organization, The Volcani Center, 50250 Bet-Dagan, Israel.

出版信息

J Biol Chem. 2000 Sep 15;275(37):28715-21. doi: 10.1074/jbc.M004985200.

DOI:10.1074/jbc.M004985200
PMID:10874045
Abstract

The citrus phospholipid hydroperoxide glutathione peroxidase (cit-PHGPx) was the first plant peroxidase demonstrated to exhibit PHGPx-specific enzymatic activity, although it was 500-fold weaker than that of the pig heart analog. This relatively low activity is accounted for the catalytic residue of cit-PHGPx, which was found to be cysteine and not the rare selenocysteine (Sec) present in animal enzymes. Sec incorporation into proteins is encoded by a UGA codon, usually a STOP codon, which, in prokaryotes, is suppressed by an adjacent downstream mRNA stem-loop structure, the Sec insertion sequence (SECIS). By performing appropriate nucleotide substitutions into the gene encoding cit-PHGPx, we introduced bacterial-type SECIS elements that afforded the substitution of the catalytic Cys(41) by Sec, as established by mass spectrometry, while preserving the functional integrity of the peroxidase. The recombinant enzyme, whose synthesis is selenium-dependent, displayed a 4-fold enhanced peroxidase activity as compared with the Cys-containing analog, thus confirming the higher catalytic power of Sec compared with Cys in cit-PHGPx active site. The study led also to refinement of the minimal sequence requirements of the bacterial-type SECIS, and, for the first time, to the heterologous expression in Escherichia coli of a eukaryotic selenoprotein containing a SECIS in its open reading frame.

摘要

柑橘磷脂氢过氧化物谷胱甘肽过氧化物酶(cit-PHGPx)是首个被证明具有PHGPx特异性酶活性的植物过氧化物酶,尽管其活性比猪心同类酶弱500倍。这种相对较低的活性是由cit-PHGPx的催化残基造成的,该催化残基被发现是半胱氨酸,而非动物酶中存在的稀有硒代半胱氨酸(Sec)。Sec掺入蛋白质是由UGA密码子编码的,UGA通常是一个终止密码子,在原核生物中,它会被相邻的下游mRNA茎环结构即Sec插入序列(SECIS)所抑制。通过对编码cit-PHGPx的基因进行适当的核苷酸替换,我们引入了细菌型SECIS元件,质谱分析证实这些元件使得催化性的半胱氨酸(Cys41)被Sec取代,同时保持了过氧化物酶的功能完整性。这种合成依赖于硒的重组酶与含半胱氨酸的类似物相比,过氧化物酶活性提高了4倍,从而证实了在cit-PHGPx活性位点中,Sec的催化能力高于Cys。该研究还细化了细菌型SECIS的最小序列要求,并且首次在大肠杆菌中实现了在开放阅读框中含有SECIS的真核硒蛋白的异源表达。

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