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3 - 5 Exonucleases of DNA Polymerases ε and δ Correct Base Analog Induced DNA Replication Errors on opposite DNA Strands in Saccharomyces Cerevisiae

机译:DNA聚合酶ε和δ的3- 5核酸外切酶正确酿酒酵母酿酒酵母中相反DNA链上的正确碱基类似物诱导的DNA复制错误。

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摘要

The base analog 6-N-hydroxylaminopurine (HAP) induces bidirectional GC -> AT and AT -> GC transitions that are enhanced in DNA polymerase ε and δ 3' -> 5' exonuclease-deficient yeast mutants, pol2-4 and pol3-01, respectively. We have constructed a set of isogenic strains to determine whether the DNA polymerases δ and ε contribute equally to proofreading of replication errors provoked by HAP during leading and lagging strand DNA synthesis. Site-specific GC -> AT and AT -> GC transitions in a Pol(+), pol2-4 or pol3-01 genetic background were scored as reversions of ura3 missense alleles. At each site, reversion was increased in only one proofreading-deficient mutant, either pol2-4 or pol3-01, depending on the DNA strand in which HAP incorporation presumably occurred. Measurement of the HAP-induced reversion frequency of the ura3 alleles placed into chromosome III near to the defined active replication origin ARS306 in two orientations indicated that DNA polymerases ε and δ correct HAP-induced DNA replication errors on opposite DNA strands.
机译:碱基类似物6-N-羟基氨基嘌呤(HAP)诱导双向GC-> AT和AT-> GC转化,DNA转化酶ε和δ3'-> 5'核酸外切酶缺陷型酵母突变体pol2-4和pol3-分别为01。我们已经构建了一套等基因菌株,以确定DNA聚合酶δ和ε是否同样有助于校正在领先和落后链DNA合成过程中HAP引起的复制错误。特定地点的GC-> AT和AT-> GC在Pol(+),pol2-4或pol3-01遗传背景下的转变被计为ura3错义等位基因的回复。在每个位点,只有一个校对缺陷的突变体pol2-4或pol3-01的逆转录增加,这取决于可能发生HAP掺入的DNA链。 HAP诱导的ura3等位基因在两个方向上靠近定义的活性复制起点ARS306的ura3等位基因的HAP诱导的回复频率的测量表明,DNA聚合酶ε和δ可纠正HAP诱导的相反DNA链上的DNA复制错误。

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