The mutT Defect Does Not Elevate Chromosomal Fragmentation in Escherichia coli Because of the Surprisingly Low Levels of MutM/MutY-Recognized DNA Modifications

Ella Rotman; Andrei Kuzminov

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The mutT Defect Does Not Elevate Chromosomal Fragmentation in Escherichia coli Because of the Surprisingly Low Levels of MutM/MutY-Recognized DNA Modifications

机译：由于MutM / MutY识别的DNA修饰水平过低，mutT缺陷不会增加大肠杆菌中的染色体片段

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Nucleotide pool sanitizing enzymes Dut (dUTPase), RdgB (dITPase), and MutT (8-oxo-dGTPase) of Escherichia coli hydrolyze noncanonical DNA precursors to prevent incorporation of base analogs into DNA. Previous studies reported dramatic AT→CG mutagenesis in mutT mutants, suggesting a considerable density of 8-oxo-G in DNA that should cause frequent excision and chromosomal fragmentation, irreparable in the absence of RecBCD-catalyzed repair and similar to the lethality of dut recBC and rdgB recBC double mutants. In contrast, we found mutT recBC double mutants viable with no signs of chromosomal fragmentation. Overproduction of the MutM and MutY DNA glycosylases, both acting on DNA containing 8-oxo-G, still yields no lethality in mutT recBC double mutants. Plasmid DNA, extracted from mutT mutM double mutant cells and treated with MutM in vitro, shows no increased relaxation, indicating no additional 8-oxo-G modifications. Our ΔmutT allele elevates the AT→CG transversion rate 27,000-fold, consistent with published reports. However, the rate of AT→CG transversions in our mutT+ progenitor strain is some two orders of magnitude lower than in previous studies, which lowers the absolute rate of mutagenesis in ΔmutT derivatives, translating into less than four 8-oxo-G modifications per genome equivalent, which is too low to cause the expected effects. Introduction of various additional mutations in the ΔmutT strain or treatment with oxidative agents failed to increase the mutagenesis even twofold. We conclude that, in contrast to the previous studies, there is not enough 8-oxo-G in the DNA of mutT mutants to cause elevated excision repair that would trigger chromosomal fragmentation.

机译：大肠埃希氏菌的核苷酸池消毒酶Dut（dUTPase），RdgB（dITPase）和MutT（8-oxo-dGTPase）水解非规范DNA前体，以防止碱基类似物掺入DNA。先前的研究报道了 mutT 突变体中发生了戏剧性的AT→CG诱变，表明DNA中的8-oxo-G密度相当高，应该引起频繁的切除和染色体片段化，这在没有RecBCD催化的修复和修复的情况下是无法修复的。与 dut recBC 和 rdgB recBC 双重突变体的致死性相似。相反，我们发现 mutT recBC 双重突变体是可行的，没有染色体片段化的迹象。 Mutm和MutY DNA糖基化酶的过量生产都作用于含有8-oxo-G的DNA，但在 mutT recBC 双重突变体中仍然没有致死性。从 mutT mutM 双突变细胞中提取的质粒DNA并在体外用MutM处理后，质粒DNA的松弛度没有增加，表明没有其他8-oxo-G修饰。我们的Δ mutT 等位基因将AT→CG的转化率提高了27,000倍，与已发表的报道一致。但是，我们的 mutT + 祖细胞株中AT→CG的转化率比以前的研究低两个数量级，这降低了Δ的绝对诱变率 mutT 衍生物，每个基因组当量转化为少于四个8-oxo-G修饰，该修饰太低而无法产生预期的效果。在Δ mutT 菌株中引入各种其他突变或用氧化剂处理均无法使诱变增加两倍。我们得出的结论是，与以前的研究相反， mutT 突变体的DNA中没有足够的8-oxo-G引起升高的切除修复，从而引发染色体断裂。 展开▼

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《Journal of bacteriology》 |2007年第19期|共13页

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Ella Rotman; Andrei Kuzminov;
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专利

1. Interactions among the Escherichia coli mutT, mutM, and mutY damage prevention pathways. [J] . Fowler RG, White SJ, Koyama C, DNA repair . 2003,第2期

机译：大肠杆菌mutT，mutM和mutY损害预防途径之间的相互作用。

2. Functional cooperation of MutT, MutM and MutY proteins in preventing mutations caused by spontaneous oxidation of guanine nucleotide in Escherichia coli. [J] . Tajiri T, Maki H, Sekiguchi M Mutation Research: International Journal on Mutagenesis, Chromosome Breakage and Related Subjects . 1995,第3期

机译：MutT，MutM和MutY蛋白在防止大肠杆菌中鸟嘌呤核苷酸的自发氧化引起的突变中的功能配合。

3. Escherichia coli DNA polymerase III is responsible for the high level of spontaneous mutations in mutT strains [J] . Molecular Microbiology . 2012,第6期

机译：大肠杆菌DNA聚合酶III导致mutT菌株中高水平的自发突变

4. Reconstitution of in vitro inactivation and reactivation systems of DnaA protein for the control of chromosomal replication initiation in Escherichia coli [C] . Masayuki Suetsugu, Kazuyuki Fujimitsu, Tsutomu Katayama IEEE International Symposium on Micro-NanoMechatronics and Human Science . 2006

机译：DNAA蛋白体外灭活和再活化系统的重组，用于控制大肠杆菌染色体复制术

5. Chromosomal fragmentation in Escherichia coli: Its absence in mutT mutants and its mechanisms in seqA mutants. [D] . Rotman, Ella Rose. 2009

机译：大肠杆菌中的染色体片段化：mutT突变体中不存在其片段及其seqA突变体中的机制。

6. The mutT Defect Does Not Elevate Chromosomal Fragmentation in Escherichia coli Because of the Surprisingly Low Levels of MutM/MutY-Recognized DNA Modifications [O] . Ella Rotman, Andrei Kuzminov 2007

机译：由于MutM / MutY识别的DNA修饰水平过低mutT缺陷不会提高大肠杆菌中的染色体片段

7. The mutT Defect Does Not Elevate Chromosomal Fragmentation in Escherichia coli Because of the Surprisingly Low Levels of MutM/MutY-Recognized DNA Modifications▿ [O] . Rotman, Ella, Kuzminov, Andrei 2007

机译：由于MutM / MutY识别的DNA修饰水平过低，mutT缺陷不会提高大肠杆菌中的染色体片段

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机译：基于VTvaf17基因治疗DNA载体的基因治疗DNA载体，其携带选自ANG，ANGPT1，VEGFA，FGF1，HIF1α，HGF，SDF1，KLK4，PDGFC，PROK1，PROK2的靶基因以增加这些靶标的表达水平基因，方法的制备和使用，大肠杆菌菌株SCS110-AF / VTvaf17-ANG或大肠杆菌SCS110-AF / VTvaf17-ANGPT1或大肠杆菌SCS110-AF / VTvaf17-VEGFA或大肠杆菌SCS110-AF / VTvaf17-Fichia-SC110 AF /VTvaf17-HIF1α或大肠杆菌SCS110-AF / VTvaf17-HGF或大肠杆菌SCS110-AF / VTvaf17-SDF1或大肠杆菌SCS110-AF / VTvaf17-KLK4或大肠杆菌SCS110-AF / VTviFi10 S1携带基因治疗DNA载体的大肠杆菌SCS110-AF / VTvaf17-PROK2，其制备方法，工业生产基因治疗DNA载体的方法

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The mutT Defect Does Not Elevate Chromosomal Fragmentation in Escherichia coli Because of the Surprisingly Low Levels of MutM/MutY-Recognized DNA Modifications

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