首页> 美国卫生研究院文献>Journal of Bacteriology >Complexity of the ultraviolet mutation frequency response curve in Escherichia coli B/r: SOS induction one-lesion and two-lesion mutagenesis.
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Complexity of the ultraviolet mutation frequency response curve in Escherichia coli B/r: SOS induction one-lesion and two-lesion mutagenesis.

机译:大肠杆菌B / r中紫外线突变频率响应曲线的复杂性:SOS诱导一个病变和两个病变的诱变。

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摘要

Three distinct sections of the ultraviolet mutation frequency response (MFR) curve toward tryptophan prototrophy have been demonstrated in Excherichia coli B/r WP2 trp thy and its uvrA derivative in log-phase growth in minimal medium. The initial section, which appears fluence-squared, may reflect the necessity, if mutation is to result, for induction of two lesions, one located within the potentially mutated genetic locus and the other damaging deoxyribonucleic acid replication and resulting in inducation of the error-prone SOS repair function. A second linear section is ascribed to the continued induction, after exposure above that sufficient for complete SOS expression, of isolated lesions which lead to mutation in potentially mutated loci. The third section demonstrates an increased rate of mutagenesis and suggests the induction of two lesions in proximity which result in additional mutations. Split-exposure studies support the inducible nature of the SOS function and suggest that mutation frequency decline (MFD) is due to exicion resulting from or related to the prevention of SOS induction by inhibition of protein synthesis. Preirradiation tryptophan starvation of the uvr+ strain for 30 min decrease MFR in the first and second sections of the curve. Reduction of MFR in the third section requires more prestarvation time and is blocked by nalidixic acid. The decreased MFR of the first and second sections ascribed to promotion of postirradiation MFD based on excision and that of third section to completion of the chromosome during the prestarvation period.
机译:已在基本培养基中以对数生长期在大肠杆菌B / r WP2 trp thy和其uvrA衍生物中证明了向色氨酸原营养型的紫外线突变频率响应(MFR)曲线的三个截然不同的部分。初始部分显示为通量平方,如果要导致突变,则可能反映出诱导两个病变的必要性,一个病变位于可能突变的遗传基因座内,另一个损坏脱氧核糖核酸复制并导致错误提示。容易出现SOS修复功能。在暴露于足以完成SOS表达的充分暴露之后,第二个线性部分归因于持续诱导分离的病变,从而导致潜在突变的基因座发生突变。第三部分证明了诱变的速率增加,并提出了在附近诱发两个病变的诱因,这导致了额外的突变。分体暴露研究支持SOS功能的可诱导性质,并表明突变频率下降(MFD)是由于抑制蛋白合成而阻止SOS诱导或与之相关的兴奋。 uvr +菌株的辐射前色氨酸饥饿30分钟可降低曲线第一部分和第二部分的MFR。在第三部分中降低MFR需要更多的预饥饿时间,并且被萘啶酸所阻止。第一部分和第二部分的MFR降低归因于在饥饿前期基于切除的照射后MFD的促进,第三部分的MFR促进了染色体的完成。

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