Functional and physical interaction between Sgs1 and Top3 and Sgs1-independent function of Top3 in DNA recombination repair
スポンサーリンク
概要
- 論文の詳細を見る
A mutant allele of SGS1 of Saccharomyces cerevisiae was identified as a suppressor of the slow-growth phenotype of top3 mutants. We previously reported the involvement of Top3 via the interaction with the N-terminal region of Sgs1 in the complementation of methylmethanesulfonate (MMS) sensitivity and the suppression of hyper recombination of a sgs1 mutant. In this study, we found that several amino acids residues in the N-terminal region of Sgs1 between residues 4 and 33 were responsible for binding to Top3 and essential for complementing the sensitivity to MMS of sgs1 cells. Two-hybrid assays suggested that the region of Top3 responsible for the binding to Sgs1 was bipartite, with portion in the N- and C-terminal domains. Although disruption of the SGS1 gene suppressed the semi-lethality of the top3 mutant of strain MR, the sgs1-top3 double mutant grew more slowly and was more sensitive to MMS than the sgs1 single mutant, indicating that Top3 plays some role independently of Sgs1. The DNA topoisomerase activity of Top3 was required for the Top3 function to repair DNA damages induced by MMS, as shown by the fact that the TOP3 gene carrying a mutation (Phe for Tyr) at the amino acid residue essential for its activity (residue 356) failed to restore the MMS sensitivity of sgs1-top3 to the level of that of the sgs1 single mutant. Epistatic analysis using the sgs1-top3 double mutant, rad52 mutant and sgs1-top3-rad52 triple mutant indicated that TOP3 belongs to the RAD52 recombinational repair pathway.
- 日本遺伝学会の論文
著者
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MIYAJIMA Atsuko
Division of Pharmacology, National Institute of Health Sciences
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Miyajima A
Division Of Pharmacology Biological Safety Research Center National Institute Of Health Sciences
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Miyajima Atsuko
東北大学 薬研究 遺伝子薬
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Miyajima Atsuko
Division Of Pharmacology Biological Safety Research Center National Institute Of Health Sciences
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ONODERA Ryoko
Molecular Cell Biology Laboratory, Graduate School of Pharmaceutical Sciences, Tohoku University
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SEKI Masayuki
Molecular Cell Biology Laboratory, Graduate School of Pharmaceutical Sciences, Tohoku University
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UI Ayako
Molecular Cell Biology Laboratory, Graduate School of Pharmaceutical Sciences, Tohoku University
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SATOH Yurie
Molecular Cell Biology Laboratory, Graduate School of Pharmaceutical Sciences, Tohoku University
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ONODA Fumitoshi
Molecular Cell Biology Laboratory, Graduate School of Pharmaceutical Sciences, Tohoku University
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ENOMOTO Takemi
Molecular Cell Biology Laboratory, Graduate School of Pharmaceutical Sciences, Tohoku University
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Ui Ayako
Molecular Cell Biology Laboratory Graduate School Of Pharmaceutical Sciences Tohoku University
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Satoh Yurie
Molecular Cell Biology Laboratory Graduate School Of Pharmaceutical Sciences Tohoku University
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Seki Masayuki
Molecular Cell Biology Laboratory Graduate School Of Pharmaceutical Sciences Tohoku University
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Enomoto Takemi
Molecular Cell Biology Laboratory Graduate School Of Pharmaceutical Sciences Tohoku University
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Enomoto T
Tohoku Univ. Miyagi
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Onodera Ryoko
Molecular Cell Biology Laboratory Graduate School Of Pharmaceutical Sciences Tohoku University
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Onoda Fumitoshi
Molecular Cell Biology Laboratory Graduate School Of Pharmaceutical Sciences Tohoku University
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Enomoto T
Molecular Cell Biology Laboratory Graduate School Of Pharmaceutical Sciences Tohoku University
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Enomoto Takemi
Cell Biology Laboratory Graduate School Of Pharmaceutical Sciences Tohoku University
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Seki M
Nissin Kogyo Co. Ltd. Tobu Jpn
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