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SOS gene induction and possible mutagenic effects of freeze-drying in Escherichia coli and Salmonella typhimurium

机译:大肠杆菌和鼠伤寒沙门氏菌的SOS基因诱导和冻干可能的诱变作用

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摘要

We report the results of a study of the potential negative effects of the freeze-drying process, normally considered a benign means for long-term conservation of living cells and the golden standard in bacterial preservation. By monitoring gene induction using a whole-cell Escherichia coli bioreporter panel, in which diverse stress-responsive gene promoters are fused to luminescent or fluorescent reporting systems, we have demonstrated that DNA repair genes belonging to the SOS operon (recA, sulA, uvrA, umuD, and lexA) were induced upon resuscitation from the freeze-dried state, whereas other stress-responsive promoters such as grpE, katG, phoA, soxS, and sodA were not affected. This observation was confirmed by the UMU-chromotest (activation of the umuD gene promoter) in Salmonella typhimurium, as well as by real-time PCR analyses of selected E. coli SOS genes. We further show that a functional SOS operon is important in viability maintenance following resuscitation, but that at the same time, this repair system may introduce significantly higher mutation rates, comparable to those induced by high concentrations of a known mutagen. Our results also indicate that the entire freeze-drying process, rather than either freezing or drying separately, is instrumental in the induction of DNA damage.
机译:我们报告了冷冻干燥过程的潜在负面影响的研究结果,该过程通常被认为是长期保存活细胞和细菌保存的黄金标准的良性手段。通过使用全细胞大肠杆菌生物报告专家组监测基因诱导,其中各种应激反应基因启动子与发光或荧光报告系统融合,我们证明了属于SOS操纵子的DNA修复基因(recA,sulA,uvrA,在从冷冻干燥状态复苏后,诱导了umuD和lexA),而其他压力响应性启动子(如grpE,katG,phoA,soxS和sodA)不受影响。鼠伤寒沙门氏菌中的UMU色谱测试(激活umuD基因启动子),以及对选定的大肠杆菌SOS基因进行实时PCR分析,证实了这一观察结果。我们进一步表明,功能性SOS操纵子在复苏后的生存能力维持中很重要,但是与此同时,与高浓度的已知诱变剂诱导的突变率相比,该修复系统可能会引入更高的突变率。我们的结果还表明,整个冷冻干燥过程(而不是单独冷冻或干燥)有助于诱导DNA损伤。

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