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通过基因转化选择酿酒酵母中一种核尿嘧啶-DNA-糖基化酶缺陷型突变体。

Selection by genetic transformation of a Saccharomyces cerevisiae mutant defective for the nuclear uracil-DNA-glycosylase.

作者信息

Burgers P M, Klein M B

出版信息

J Bacteriol. 1986 Jun;166(3):905-13. doi: 10.1128/jb.166.3.905-913.1986.

Abstract

A coliphage M13 chimer containing the Saccharomyces cerevisiae TRP1 gene and ARS1 replication origin (mPY2) was grown on an ung- dut- strain of Escherichia coli. The resulting single-stranded phage DNA had 13% of thymine residues substituted by uracil. This DNA failed to transform a delta trp1 yeast strain to prototrophy. However, when a mutagenized yeast stock was transformed with uracil-containing single-stranded mPY2 DNA, unstable transformants were obtained. After plasmid segregation, about half of these were retransformed at a high frequency by uracil-containing single-stranded mPY2 DNA. In vitro, these mutants were defective for uracil-DNA-glycosylase activity. They were designated ung1. Strains containing the ung1 mutation have an increased sensitivity to sodium bisulfite and sodium nitrite but a wild-type sensitivity to methyl methanesulfonate, UV light, and drugs that cause depletion of the thymidylate pool. They have a moderate mutator phenotype for nuclear but not for mitochondrial genes. A low mitochondrial uracil-DNA-glycosylase activity was demonstrated in the mutant strains.

摘要

一种含有酿酒酵母TRP1基因和ARS1复制起点的大肠杆菌噬菌体M13嵌合体(mPY2)在大肠杆菌的ung - dut - 菌株上生长。所得的单链噬菌体DNA中有13%的胸腺嘧啶残基被尿嘧啶取代。这种DNA无法将δtrp1酵母菌株转化为原养型。然而,当用含尿嘧啶的单链mPY2 DNA转化诱变的酵母菌株时,获得了不稳定的转化体。在质粒分离后,其中约一半被含尿嘧啶的单链mPY2 DNA高频重新转化。在体外,这些突变体的尿嘧啶-DNA-糖基化酶活性有缺陷。它们被命名为ung1。含有ung1突变的菌株对亚硫酸氢钠和亚硝酸钠的敏感性增加,但对甲基磺酸甲酯、紫外线和导致胸苷酸池耗尽的药物具有野生型敏感性。它们对于核基因具有中等的诱变表型,但对于线粒体基因则没有。在突变菌株中证明了低水平的线粒体尿嘧啶-DNA-糖基化酶活性。

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