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Mutants of Mycobacterium smegmatis impaired in stationary-phase survival

机译:分枝杆菌的突变体在固定相存活中受损

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A bank of 600 insertional mutants of Mycobacterium smegmatis was screened for mutants defective in stationary-phase survival. Of 74 mutants picked by the initial screen, 21 had stationary-phase survival defects and 7 of these were studied in more detail. In general, mutants survived stationary phase significantly less well in rich medium than under carbon-starvation conditions. In all cases the loss of viability in stationary phase was not complete even after prolonged incubation. All mutants showed an initial decrease in viability, during the first 40?d in stationary phase, followed by an increase in viable counts that returned viability close to the levels of the wild-type. Southern hybridization experiments showed that recovery of viability was not a consequence of precise excision or movement of the transposon. Two of the survival mutants differed from the wild-type in their colony morphology, and recovery of their viability in stationary phase was coincident with the return of wild-type colony morphology. It is possible that second-site suppressor mutations accumulate that alleviate the effects of the original mutation. For five of the mutants the DNA flanking the site of transposition was amplified by ligation-mediated PCR and sequenced to identify the disrupted locus. In each case, homologous genes were identified in the Mycobacterium tuberculosis genome, three of which have clearly predicted functions in M. tuberculosis as a penicillin-binding protein, in biotin biosynthesis and as a polyketide synthase. This is the first identification of genes implicated in the stationary-phase survival of mycobacteria.
机译:筛选突变体在固定相存活中缺血的突变体的600分枝杆菌的突变体。在初始筛选的74个突变体中,21例具有固定相存活缺陷,其中7个更详细地研究了其中7个。通常,突变体在富含碳饥饿条件下的富含培养基中的固定相活得少得多。在所有情况下,即使在长时间孵化后,固定阶段的活力损失也没有完成。在固定阶段的前40℃期间,所有突变体均显示活力的初始降低,然后增加可行计数的可行性,返回接近野生型水平的活力。 Southern杂交实验表明,存活率的回收率不是经过试位器的精确切除或运动的结果。两种存活突变体与群体形态的野生类型不同,并且在固定阶段的活力恢复与野生型菌落形态的回归是一致的。第二位点抑制突变可能积累,以减轻原始突变的影响。对于五个突变体,侧翼的DNA通过连接介导的PCR扩增,并测序以鉴定破坏的基因座。在每种情况下,在结核分枝杆菌基因组中鉴定了同源基因,其中三个在生物素生物合成中具有清晰地预测在M.结核中作为青霉素结合蛋白和聚酮合成蛋白的功能。这是第一次鉴定涉及分枝杆菌的固定相存活的基因。

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