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巨大脱硫弧菌尼尔雷德oxin的分子特征分析,一种参与厌氧菌氧气解毒的蛋白质。

Molecular characterization of Desulfovibrio gigas neelaredoxin, a protein involved in oxygen detoxification in anaerobes.

作者信息

Silva G, LeGall J, Xavier A V, Teixeira M, Rodrigues-Pousada C

机构信息

Instituto de Tecnologia Química e Biológica, Universidade Nova de Lisboa, 2781-901 Oeiras, Portugal.

出版信息

J Bacteriol. 2001 Aug;183(15):4413-20. doi: 10.1128/JB.183.4.4413-4420.2001.

Abstract

Desulfovibrio gigas neelaredoxin is an iron-containing protein of 15 kDa, having a single iron site with a His(4)Cys coordination. Neelaredoxins and homologous proteins are widespread in anaerobic prokaryotes and have superoxide-scavenging activity. To further understand its role in anaerobes, its genomic organization and expression in D. gigas were studied and its ability to complement Escherichia coli superoxide dismutase deletion mutant was assessed. In D. gigas, neelaredoxin is transcribed as a monocistronic mRNA of 500 bases as revealed by Northern analysis. Putative promoter elements resembling sigma(70) recognition sequences were identified. Neelaredoxin is abundantly and constitutively expressed, and its expression is not further induced during treatment with O(2) or H(2)O(2). The neelaredoxin gene was cloned by PCR and expressed in E. coli, and the protein was purified to homogeneity. The recombinant neelaredoxin has spectroscopic properties identical to those observed for the native one. Mutations of Cys-115, one of the iron ligands, show that this ligand is essential for the activity of neelaredoxin. In an attempt to elucidate the function of neelaredoxin within the cell, it was expressed in an E. coli mutant deficient in cytoplasmic superoxide dismutases (sodA sodB). Neelaredoxin suppresses the deleterious effects produced by superoxide, indicating that it is involved in oxygen detoxification in the anaerobe D. gigas.

摘要

巨大脱硫弧菌的尼尔红氧还蛋白是一种15千道尔顿的含铁蛋白,具有一个由4个组氨酸和1个半胱氨酸配位的单一铁位点。尼尔红氧还蛋白及其同源蛋白广泛存在于厌氧原核生物中,并具有超氧化物清除活性。为了进一步了解其在厌氧菌中的作用,研究了它在巨大脱硫弧菌中的基因组组织和表达,并评估了其对大肠杆菌超氧化物歧化酶缺失突变体的互补能力。通过Northern分析发现,在巨大脱硫弧菌中,尼尔红氧还蛋白转录为一个500个碱基的单顺反子mRNA。鉴定出了类似于σ⁷⁰识别序列的推定启动子元件。尼尔红氧还蛋白大量且组成性表达,在用氧气或过氧化氢处理期间其表达不会进一步诱导。通过PCR克隆了尼尔红氧还蛋白基因并在大肠杆菌中表达,该蛋白被纯化至同质。重组尼尔红氧还蛋白具有与天然蛋白相同的光谱性质。铁配体之一的半胱氨酸-115的突变表明该配体对尼尔红氧还蛋白的活性至关重要。为了阐明尼尔红氧还蛋白在细胞内的功能,将其在缺乏细胞质超氧化物歧化酶(sodA sodB)的大肠杆菌突变体中表达。尼尔红氧还蛋白抑制了超氧化物产生的有害影响,表明它参与了厌氧菌巨大脱硫弧菌中的氧解毒过程。

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