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  1. 研究・技術・調査報告

Construction of Luciferase Reporter Strains for Functional Analysis of DNA Damage Response Regulators

https://repo.qst.go.jp/records/82298
https://repo.qst.go.jp/records/82298
a8d540af-b895-484e-b1ed-7db3b761fe80
Item type 一般雑誌記事 / Article(1)
公開日 2021-03-19
タイトル
タイトル Construction of Luciferase Reporter Strains for Functional Analysis of DNA Damage Response Regulators
言語
言語 eng
資源タイプ
資源タイプ識別子 http://purl.org/coar/resource_type/c_6501
資源タイプ article
アクセス権
アクセス権 metadata only access
アクセス権URI http://purl.org/coar/access_right/c_14cb
著者 Katsuya, Sato

× Katsuya, Sato

WEKO 937945

Katsuya, Sato

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Sanzen, Toshihiko

× Sanzen, Toshihiko

WEKO 937946

Sanzen, Toshihiko

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Yutaka, Ono

× Yutaka, Ono

WEKO 937947

Yutaka, Ono

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Narumi, Issay

× Narumi, Issay

WEKO 937948

Narumi, Issay

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Katsuya, Sato

× Katsuya, Sato

WEKO 937949

en Katsuya, Sato

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Yutaka, Ono

× Yutaka, Ono

WEKO 937950

en Yutaka, Ono

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抄録
内容記述タイプ Abstract
内容記述 Deinococcus radiodurans is a representative strain of radioresistant bacteria and has extremely high resistance to various DNA damage caused by gamma rays, ultraviolet rays, desiccation, free radical-generating substances, and DNA cross-linkers. The previous studies revealed that the expression of a unique DNA repair-related protein, PprA, was up-regulated by a DNA damage response regulator, PprI, following DNA damage in D. radiodurans. However, the detailed functional site of PprI protein is poorly understood. In an effort to gain an insight into the role of PprI in DNA damage response mechanism in D. radiodurans, we generated luciferase reporter strains that were regulated by pprI expression plasmids. Firstly, we constructed a luciferase reporter DNA cassette consisted of an engineered firefly luciferase gene (FL) and an Escherichia coli spectinomycin resistance gene. Next, this luciferase reporter DNA cassette was integrated into the genome of the wild-type and the pprI-deleted mutant strains, and the resulting FL reporter strains were designated DARP and SIRP, respectively. Consequently, in strain DARP, FL reporter activity was enhanced following 2 kGy gamma irradiation at 2 h post-irradiation time. On the other hand, FL reporter activity in the pprI-deletion strain SIRP was not observed following irradiation. Like strain DARP, the FL reporter activity in the strain SIRP carrying the pprI expression plasmid was enhanced following irradiation by functional complementation with the pprI expression plasmid. This result suggests that the D. radiodurans PprI is a key protein for DNA damage response regulator.
書誌情報 QST Takasaki Annual Report 2019

巻 QST-M-29, p. 96-96, 発行日 2021-03
出版者
出版者 QST
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