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umuDC、mucAB和samAB操纵子对大肠杆菌化学诱变突变特异性的影响:II. 碱基替换诱变

Effects of the umuDC, mucAB, and samAB operons on the mutational specificity of chemical mutagenesis in Escherichia coli: II. Base substitution mutagenesis.

作者信息

Watanabe M, Nohmi T, Ohta T

机构信息

Institute of Environmental Toxicology, Tokyo, Japan.

出版信息

Mutat Res. 1994 Jan;314(1):39-49. doi: 10.1016/0921-8777(94)90059-0.

Abstract

Mutational spectra induced by different classes of chemical mutagens including two ultraviolet-mimetic mutagens, an alkylating agent, intercalators, a crosslinking agent, and base analogs were characterized by means of a set of mutant lacZ genes in E. coli. These strains can be used to detect each of two types of transition and four types of transversion, simply by measuring the number of Lac+ revertant colonies. 4-Nitroquinoline 1-oxide induced G.C-->A.T, G.C-->C.G, or G.C-->T.A changes almost equally, whereas furylfuramide and mitomycin C induced only G.C-->A.T transitions and G.C-->T.A transversions, respectively. No base substitutional mutations were detected by the treatment with 9-aminoacridine. A weak stimulation of G.C-->A.T transitions by ICR-191 was observed. Both the G.C-->A.T and A.T-->G.C transitions were induced by N-methyl-N'-nitro-N-nitrosoguanidine and N4-aminocytidine. 5-Azacytidine was a specific inducer of G.C-->C.G transversions. In addition, a comparative study of mutational specificity was performed in the strains bearing either the umuDC, mucAB, or the samAB operon on a multicopy plasmid. Regardless of the kind of mutagen, G.C-->T.A transversions were greatly potentiated by the introduction of plasmids in the order of pGW1700 (mucAB) > pSE117 (umuDC) > or = pYG8011 (samAB). Besides G.C-->T.A transversions, the introduction of pGW1700, but not pSE117 and pYG8011, enhanced the mutations of A.T-->C.G and A.T-->T.A transversions. The mucAB plasmid also enhanced the G.C-->A.T transitions and G.C-->C.G transversions induced by some mutagens.

摘要

利用一组大肠杆菌中的突变型lacZ基因,对包括两种紫外线模拟诱变剂、一种烷化剂、嵌入剂、一种交联剂和碱基类似物在内的不同类化学诱变剂诱导的突变谱进行了表征。这些菌株可通过简单地测量Lac + 回复菌落的数量,用于检测两种类型的转换和四种类型的颠换。4-硝基喹啉1-氧化物几乎同等程度地诱导G.C→A.T、G.C→C.G或G.C→T.A变化,而呋喃基糠酰胺和丝裂霉素C分别仅诱导G.C→A.T转换和G.C→T.A颠换。用9-氨基吖啶处理未检测到碱基置换突变。观察到ICR-191对G.C→A.T转换有微弱刺激作用。N-甲基-N'-硝基-N-亚硝基胍和N4-氨基胞苷诱导了G.C→A.T和A.T→G.C转换。5-氮杂胞苷是G.C→C.G颠换的特异性诱导剂。此外,在多拷贝质粒上携带umuDC、mucAB或samAB操纵子的菌株中进行了突变特异性的比较研究。无论诱变剂种类如何,通过引入质粒,G.C→T.A颠换按pGW1700(mucAB)> pSE117(umuDC)> 或 = pYG8011(samAB)的顺序得到极大增强。除了G.C→T.A颠换外,引入pGW1700而非pSE117和pYG8011可增强A.T→C.G和A.T→T.A颠换的突变。mucAB质粒还增强了某些诱变剂诱导的G.C→A.T转换和G.C→C.G颠换。

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