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Mismatch-induced lethality due to a defect in Escherichia coli RecQ. helicase in exonuclease-deficient background: Dependence on MutS and UvrD functions

机译：由于大肠杆菌RecQ中的缺陷而导致错配诱导的致死性。核酸外切酶缺陷型背景下的解旋酶：对MutS和UvrD功能的依赖

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Escherichia coli DNA-unwinding protein RecQ. has roles in the regulation of general recombination and the processing of stalled replication forks. In this study, we found that knockout of the recQ. gene in combination with xonA xseA recj mutations, which inhibit methyl-directed mismatch repair (MMR), caused about 100-fold increase in sensitivity to a purine analog 2-aminopurine (2AP). Intriguingly, inactivation of a MMR initiator due to the either mutation mutS or uvrD completely suppressed the 2AP sensitivity caused by recQxonA xseA recj mutations, suggesting that RecQ. helicase might act on the DNA structures that are generated by the processing of DNA by the MutSLH complex and UvrD helicase. Moreover, the recQ. gene knockout in combination with xonA xseA recj mutations enhanced 2AP-induced filament formation, and increased by twofold the rate of spontaneous forward mutations in the thy A locus but did not increase the rate of rifampicin-resistant mutations. We discuss about the possible interplay between E. coli RecQ helicase and mismatch recognition factors.

机译：大肠杆菌DNA解链蛋白RecQ。在常规重组和停滞的复制叉的处理中发挥作用。在这项研究中，我们发现recQ的敲除。该基因与xonA xseA recj突变相结合，可抑制甲基定向错配修复（MMR），对嘌呤类似物2-氨基嘌呤（2AP）的敏感性提高约100倍。有趣的是，由于mutS或uvrD突变而导致的MMR引发剂的失活完全抑制了recQxonA xseA recj突变引起的2AP敏感性，这提示了RecQ。解旋酶可能作用于由MutSLH复合物和UvrD解旋酶对DNA进行处理而生成的DNA结构。此外，recQ。基因敲除与xonA xseA recj突变结合可增强2AP诱导的细丝形成，并在thy A基因座中自发正向突变的速率增加两倍，但不会增加对利福平耐药的突变的速率。我们讨论了大肠杆菌RecQ解旋酶和错配识别因子之间可能的相互作用。

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来源
《Plasmid: An International Journal Devoted to Extrachromosomal Gene Systems》 |2010年第3期|共9页
作者
Yoshimasa Yamana; Shuji Sonezaki; Hiroaki I. Ogawa; Kohji Kusano;
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原文格式 PDF
正文语种 eng
中图分类医学遗传学;
关键词
RecQ; Exonuclease; Mismatch repair; SOS response;

机译：RecQ;核酸外切酶;错配修复;SOS反应;

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1. Mismatch-induced lethality due to a defect in Escherichia coli RecQ. helicase in exonuclease-deficient background: Dependence on MutS and UvrD functions [J] . Yoshimasa Yamana, Shuji Sonezaki, Hiroaki I. Ogawa, Plasmid: An International Journal Devoted to Extrachromosomal Gene Systems . 2010,第3期

机译：由于大肠杆菌RecQ中的缺陷而导致错配诱导的致死性。核酸外切酶缺陷型背景下的解旋酶：对MutS和UvrD功能的依赖
2. em>Escherichia coli/em> and em>Neisseria gonorrhoeae/em> UvrD helicase unwinds G4 DNA structures [J] . Kaustubh Shukla, Roshan Singh Thakur, Debayan Ganguli, The Biochemical Journal . 2017,第21期

机译：＆ em>大肠杆菌＆ / em> neisseria jonorrhoeae＆ / em> UVRD Helicase展开G4 DNA结构
3. RecF recombination pathway in Escherichia coli cells lacking RecQ, UvrD and HelD helicases [J] . Buljuba?i?M., ReparJ., ZahradkaK., DNA repair . 2012,第4期

机译：缺乏RecQ，UvrD和HelD解旋酶的大肠杆菌细胞中的RecF重组途径
4. Isolation and Identification of Helicase from Escherichia coli for Biotechnology Processes [C] . S.Sasidharan, S.Yamuna, O. Eugene International Conference on Biotechnology and Food Science . 2012

机译：脑卒中大肠杆菌对生物技术过程的螺旋酶的分离与鉴定
5. Molecular mechanisms underlying the deoxyribonucleic acid helicase activity of Escherichia coli RecQ. [D] . Zittel, Morgan C. 2007

机译：大肠杆菌RecQ的脱氧核糖核酸解旋酶活性的分子机制。
6. Double helicase II (uvrD)-helicase IV (helD) deletion mutants are defective in the recombination pathways of Escherichia coli. [O] . V M Mendonca, K Kaiser-Rogers, S W Matson 2017

机译：双重解旋酶II（uvrD）-解旋酶IV（helD）缺失突变体在大肠杆菌的重组途径中存在缺陷。
7. UvrD helicase, unlike Rep helicase, dismantles RecA nucleoprotein filaments in Escherichia coli [O] . Veaute, Xavier, Delmas, Stéphane, Selva, Marjorie, 2004

机译：与Rep解旋酶不同，UvrD解旋酶可拆卸大肠杆菌中的RecA核蛋白丝

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