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Role of narK2X and narGHJI inHypoxic Upregulation of Nitrate Reduction by Mycobacteriumtuberculosis

亚硝酸盐还原酶 硝酸还原酶 生物 操纵子 亚硝酸盐 突变体 硝酸盐 微生物学 生物化学 大肠杆菌 还原酶 结核分枝杆菌 分子生物学 基因 肺结核 病理 医学 生态学
作者
Charles D. Sohaskey,Lawrence G. Wayne
出处
期刊:Journal of Bacteriology [American Society for Microbiology]
卷期号:185 (24): 7247-7256 被引量:167
标识
DOI:10.1128/jb.185.24.7247-7256.2003
摘要

ABSTRACT Mycobacterium tuberculosis is one of the strongest reducers of nitrate in the genus Mycobacterium . Under microaerobic conditions, whole cells exhibit upregulation of activity, producing approximately eightfold more nitrite than those of aerobic cultures of the same age. Assays of cell extracts from aerobic cultures and hypoxic cultures yielded comparable nitrate reductase activities. Mycobacterium bovis produced only low levels of nitrite, and this activity was not induced by hypoxia. M . tuberculosis has two sets of genes, narGHJI and narX of the narK2X operon, that exhibit some degree of homology to prokaryotic dissimilatory nitrate reductases. Each of these were knocked out by insertional inactivation. The narG mutant showed no nitrate reductase activity in whole culture or in cell-free assays, while the narX mutant showed wild-type levels in both assays. A knockout of the putative nitrite transporter narK2 gene produced a strain that had aerobic levels of nitrate reductase activity but failed to show hypoxic upregulation. Insertion of the M. tuberculosis narGHJI into a nitrate reductase Escherichia coli mutant allowed anaerobic growth in the presence of nitrate. Under aerobic and hypoxic conditions, transcription of narGHJI was constitutive, while the narK2X operon was induced under hypoxia, as measured with a lacZ reporter system and by quantitative real-time reverse PCR. This indicates that nitrate reductase activity in M . tuberculosis is due to the narGHJI locus with no detectable contribution from narX and that the hypoxic upregulation of activity is associated with the induction of the nitrate and nitrite transport gene narK2 .
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