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  1. 原著論文

RAC2-P38 MAPK-dependent NADPH oxidase activity is associated with the resistance of quiescent cells to ionizing radiation.

https://repo.qst.go.jp/records/47693
https://repo.qst.go.jp/records/47693
ae38f636-9a72-4db9-8a5a-3b1e4d09a38d
Item type 学術雑誌論文 / Journal Article(1)
公開日 2017-03-27
タイトル
タイトル RAC2-P38 MAPK-dependent NADPH oxidase activity is associated with the resistance of quiescent cells to ionizing radiation.
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 journal 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 Pei, Hailong

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WEKO 478552

Pei, Hailong

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Zhang, Jian

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WEKO 478553

Zhang, Jian

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Nie, Jing

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WEKO 478554

Nie, Jing

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Ding, Nan

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WEKO 478555

Ding, Nan

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Hu, Wentao

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WEKO 478556

Hu, Wentao

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Hua, Junrui

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WEKO 478557

Hua, Junrui

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Hirayama, Ryoichi

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WEKO 478558

Hirayama, Ryoichi

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Furusawa, Yoshiya

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WEKO 478559

Furusawa, Yoshiya

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Liu, Cuihua

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Liu, Cuihua

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Li, Bingyan

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Li, Bingyan

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K, Hei Tom

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K, Hei Tom

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Zhou, Guangming

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WEKO 478563

Zhou, Guangming

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Pei Hailong

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WEKO 478564

en Pei Hailong

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張 健

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WEKO 478565

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Ding Nan

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en Ding Nan

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胡 文涛

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平山 亮一

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古澤 佳也

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劉 翠華

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李 冰燕

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周 光明

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抄録
内容記述タイプ Abstract
内容記述 Our recent study showed that quiescent G0 cells are more resistant to ionizing radiation than G1 cells; however, the underlying mechanism for this increased radioresistance is unknown. Based on the relatively lower DNA damage induced in G0 cells, we hypothesize that these cells are exposed to less oxidative stress during exposure. As a catalytic subunit of NADPH oxidase, Ras-related C3 botulinum toxin substrate 2 (RAC2) may be involved in the cellular response to ionizing radiation. Here, we show that RAC2 was expressed at low levels in G0 cells but increased substantially in G1 cells. Relative to G1 cells, the total antioxidant capacity in G0 phase cells increased upon exposure to X-ray radiation, whereas the intracellular concentration of ROS and malondialdehyde increased only slightly. The induction of DNA single- and double-stranded breaks in G1 cells by X-ray radiation was inhibited by knockdown of RAC2. P38 MAPK interaction with RAC2 resulted in a decrease of functional RAC2. Increased phosphorylation of P38 MAPK in G0 cells also increased cellular radioresistance; however, excessive production of ROS caused P38 MAPK dephosphorylation. P38 MAPK, phosphorylated P38 MAPK, and RAC2 regulated in mutual feedback and negative feedback regulatory pathways, resulting in the radioresistance of G0 cells.
書誌情報 Cell cycle (Georgetown, Tex.)

巻 16, 号 1, p. 113-122, 発行日 2017-01
出版者
出版者 Taylor & Francis
ISSN
収録物識別子タイプ ISSN
収録物識別子 1551-4005
PubMed番号
識別子タイプ PMID
関連識別子 27936335
DOI
識別子タイプ DOI
関連識別子 10.1080/15384101.2016.1259039
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