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不同抗氧化防御机制存在缺陷的大肠杆菌菌株细胞DNA中8-氧代鸟嘌呤的形成。

Formation of 8-oxoguanine in cellular DNA of Escherichia coli strains defective in different antioxidant defences.

作者信息

Alhama J, Ruiz-Laguna J, Rodriguez-Ariza A, Toribio F, López-Barea J, Pueyo C

机构信息

Departamento de Bioquímica y Biología Molecular, Universidad de Córdoba, España.

出版信息

Mutagenesis. 1998 Nov;13(6):589-94. doi: 10.1093/mutage/13.6.589.

DOI:10.1093/mutage/13.6.589
PMID:9862189
Abstract

This paper examines the relationship in Escherichia coli between the in vivo content of 8-oxoguanine (8-oxoG) in chromosomal DNA and deficiencies of various key antioxidant defences. The structural genes for catalases (katG and katE), cytosolic superoxide dismutases (sodA and sodB) or formamidopyrimidine-DNA glycosylase (fpg) were inactivated to obtain bacterial strains lacking the scavenger enzymes for H2O2 or O2.- or the DNA repair protein for 8-oxoG. Wild-type bacteria showed 5-fold increased sensitivity to both lethality and mutagenesis by H2O2 in K medium (1% casamino acids and 1% glucose), as compared with nutrient broth. This higher sensitivity was associated with increased chromosomal oxidative damage, estimated as the 8-oxodG content, and with a marked decrease in both catalase and SOD activities. Bacteria lacking both cytosolic SODs (sodA sodB mutant) displayed increased 8-oxodG content in chromosomal DNA (2.8-fold that of the wild-type) when grown under standard aerated conditions. Comparatively, no significant difference in 8-oxodG content was observed in cells grown without aeration. Bacteria totally devoid of catalase activity (katG katE mutant) showed wild-type contents of 8-oxodG in chromosomal DNA when grown under aerated conditions. Nevertheless, the protective role of catalase in preventing formation of 8-oxodG in chromosomal DNA became evident under oxidative stress conditions: growth under hyperoxygenation and, particularly, following H2O2 exposure. Catalase deficiency resulted in a dramatic decrease in viability after H2O2 exposure. A deficiency of Fpg protein also sensitized E.coli to H2O2 lethality, though to lesser extent than a deficiency of catalase activity. However, the scavenger enzyme and the DNA repair protein protected equally against 8-oxoG formed in vivo upon H2O2 treatment.

摘要

本文研究了大肠杆菌染色体DNA中8-氧代鸟嘌呤(8-oxoG)的体内含量与各种关键抗氧化防御缺陷之间的关系。过氧化氢酶(katG和katE)、胞质超氧化物歧化酶(sodA和sodB)或甲酰胺嘧啶-DNA糖基化酶(fpg)的结构基因被灭活,以获得缺乏H2O2或O2-清除酶或8-oxoG DNA修复蛋白的细菌菌株。与营养肉汤相比,野生型细菌在K培养基(1%酪蛋白氨基酸和1%葡萄糖)中对H2O2的致死性和致突变性的敏感性增加了5倍。这种更高的敏感性与染色体氧化损伤增加(以8-氧代脱氧鸟苷含量估计)以及过氧化氢酶和超氧化物歧化酶活性的显著降低有关。在标准通气条件下生长时,缺乏两种胞质超氧化物歧化酶的细菌(sodA sodB突变体)染色体DNA中的8-氧代脱氧鸟苷含量增加(是野生型的2.8倍)。相比之下,在无通气条件下生长的细胞中,8-氧代脱氧鸟苷含量没有显著差异。完全缺乏过氧化氢酶活性的细菌(katG katE突变体)在通气条件下生长时,染色体DNA中的8-氧代脱氧鸟苷含量显示为野生型水平。然而,在氧化应激条件下,过氧化氢酶在防止染色体DNA中8-氧代脱氧鸟苷形成方面的保护作用变得明显:在高氧条件下生长,特别是在暴露于H2O2后。过氧化氢酶缺乏导致暴露于H2O2后活力急剧下降。Fpg蛋白缺乏也使大肠杆菌对H2O2致死性敏感,尽管程度低于过氧化氢酶活性缺乏。然而,清除酶和DNA修复蛋白对H2O2处理后体内形成的8-oxoG具有同等的保护作用。

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