TRAIP/RNF206 is required for recruitment of RAP80 to sites of DNA damage

Nam Soo Lee; Hee Jin Chung; Hyoung June Kim; Seo Yun Lee; Jae Hoon Ji; Yoojeong Seo; Seung Hun Han; Minji Choi; Miyong Yun; Seok Geun Lee; Kyungjae Myung; Yonghwan Kim; Ho Chul Kang; Hongtae Kim

doi:10.1038/ncomms10463

TRAIP/RNF206 is required for recruitment of RAP80 to sites of DNA damage

Nam Soo Lee, Hee Jin Chung, Hyoung June Kim, Seo Yun Lee, Jae Hoon Ji, Yoojeong Seo, Seung Hun Han, Minji Choi, Miyong Yun, Seok Geun Lee, Kyungjae Myung, Yonghwan Kim, Ho Chul Kang, Hongtae Kim

Research output: Contribution to journal › Article › peer-review

40 Scopus citations

Abstract

RAP80 localizes to sites of DNA insults to enhance the DNA-damage responses. Here we identify TRAIP/RNF206 as a novel RAP80-interacting protein and find that TRAIP is necessary for translocation of RAP80 to DNA lesions. Depletion of TRAIP results in impaired accumulation of RAP80 and functional downstream partners, including BRCA1, at DNA lesions. Conversely, accumulation of TRAIP is normal in RAP80-depleted cells, implying that TRAIP acts upstream of RAP80 recruitment to DNA lesions. TRAIP localizes to sites of DNA damage and cells lacking TRAIP exhibit classical DNA-damage response-defect phenotypes. Biochemical analysis reveals that the N terminus of TRAIP is crucial for RAP80 interaction, while the C terminus of TRAIP is required for TRAIP localization to sites of DNA damage through a direct interaction with RNF20-RNF40. Taken together, our findings demonstrate that the novel RAP80-binding partner TRAIP regulates recruitment of the damage signalling machinery and promotes homologous recombination.

Original language	English (US)
Article number	10463
Journal	Nature communications
Volume	7
DOIs	https://doi.org/10.1038/ncomms10463
State	Published - Jan 19 2016
Externally published	Yes

ASJC Scopus subject areas

General Chemistry
General Biochemistry, Genetics and Molecular Biology
General Physics and Astronomy

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@article{1d27ee19a2234eb7b47800aa48ed4de0,

title = "TRAIP/RNF206 is required for recruitment of RAP80 to sites of DNA damage",

abstract = "RAP80 localizes to sites of DNA insults to enhance the DNA-damage responses. Here we identify TRAIP/RNF206 as a novel RAP80-interacting protein and find that TRAIP is necessary for translocation of RAP80 to DNA lesions. Depletion of TRAIP results in impaired accumulation of RAP80 and functional downstream partners, including BRCA1, at DNA lesions. Conversely, accumulation of TRAIP is normal in RAP80-depleted cells, implying that TRAIP acts upstream of RAP80 recruitment to DNA lesions. TRAIP localizes to sites of DNA damage and cells lacking TRAIP exhibit classical DNA-damage response-defect phenotypes. Biochemical analysis reveals that the N terminus of TRAIP is crucial for RAP80 interaction, while the C terminus of TRAIP is required for TRAIP localization to sites of DNA damage through a direct interaction with RNF20-RNF40. Taken together, our findings demonstrate that the novel RAP80-binding partner TRAIP regulates recruitment of the damage signalling machinery and promotes homologous recombination.",

author = "{Soo Lee}, Nam and {Jin Chung}, Hee and Kim, {Hyoung June} and {Yun Lee}, Seo and Ji, {Jae Hoon} and Yoojeong Seo and {Hun Han}, Seung and Minji Choi and Miyong Yun and Lee, {Seok Geun} and Kyungjae Myung and Yonghwan Kim and {Chul Kang}, Ho and Hongtae Kim",

note = "Funding Information: We thank the members of Hongtae Kim{\textquoteright}s laboratory for critical discussions, and Dr Anderson Wang (AstraZeneca, UK) for critical reading of the manuscript. The DSB reporter cell line (U2OS) was provided by S. Janicki and D. Spector (Wistar Institute and Cold Spring Harbor Laboratories, respectively) and HR repair cell line (U2OS) was provided by J. Stark. This work was supported by IBS-R015-D1, by a grant from the National R&D Program for Cancer Control, Ministry for Health, Welfare and Family Affairs, Republic of Korea (HI11C1596 and No.1420090) and National Research Foundation of Korea (NRF) grant funded by the Korea government (MEST; No. 20110030831).",

year = "2016",

month = jan,

day = "19",

doi = "10.1038/ncomms10463",

language = "English (US)",

volume = "7",

journal = "Nature communications",

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T1 - TRAIP/RNF206 is required for recruitment of RAP80 to sites of DNA damage

AU - Soo Lee, Nam

AU - Jin Chung, Hee

AU - Kim, Hyoung June

AU - Yun Lee, Seo

AU - Ji, Jae Hoon

AU - Seo, Yoojeong

AU - Hun Han, Seung

AU - Choi, Minji

AU - Yun, Miyong

AU - Lee, Seok Geun

AU - Myung, Kyungjae

AU - Kim, Yonghwan

AU - Chul Kang, Ho

AU - Kim, Hongtae

N1 - Funding Information: We thank the members of Hongtae Kim’s laboratory for critical discussions, and Dr Anderson Wang (AstraZeneca, UK) for critical reading of the manuscript. The DSB reporter cell line (U2OS) was provided by S. Janicki and D. Spector (Wistar Institute and Cold Spring Harbor Laboratories, respectively) and HR repair cell line (U2OS) was provided by J. Stark. This work was supported by IBS-R015-D1, by a grant from the National R&D Program for Cancer Control, Ministry for Health, Welfare and Family Affairs, Republic of Korea (HI11C1596 and No.1420090) and National Research Foundation of Korea (NRF) grant funded by the Korea government (MEST; No. 20110030831).

PY - 2016/1/19

Y1 - 2016/1/19

N2 - RAP80 localizes to sites of DNA insults to enhance the DNA-damage responses. Here we identify TRAIP/RNF206 as a novel RAP80-interacting protein and find that TRAIP is necessary for translocation of RAP80 to DNA lesions. Depletion of TRAIP results in impaired accumulation of RAP80 and functional downstream partners, including BRCA1, at DNA lesions. Conversely, accumulation of TRAIP is normal in RAP80-depleted cells, implying that TRAIP acts upstream of RAP80 recruitment to DNA lesions. TRAIP localizes to sites of DNA damage and cells lacking TRAIP exhibit classical DNA-damage response-defect phenotypes. Biochemical analysis reveals that the N terminus of TRAIP is crucial for RAP80 interaction, while the C terminus of TRAIP is required for TRAIP localization to sites of DNA damage through a direct interaction with RNF20-RNF40. Taken together, our findings demonstrate that the novel RAP80-binding partner TRAIP regulates recruitment of the damage signalling machinery and promotes homologous recombination.

AB - RAP80 localizes to sites of DNA insults to enhance the DNA-damage responses. Here we identify TRAIP/RNF206 as a novel RAP80-interacting protein and find that TRAIP is necessary for translocation of RAP80 to DNA lesions. Depletion of TRAIP results in impaired accumulation of RAP80 and functional downstream partners, including BRCA1, at DNA lesions. Conversely, accumulation of TRAIP is normal in RAP80-depleted cells, implying that TRAIP acts upstream of RAP80 recruitment to DNA lesions. TRAIP localizes to sites of DNA damage and cells lacking TRAIP exhibit classical DNA-damage response-defect phenotypes. Biochemical analysis reveals that the N terminus of TRAIP is crucial for RAP80 interaction, while the C terminus of TRAIP is required for TRAIP localization to sites of DNA damage through a direct interaction with RNF20-RNF40. Taken together, our findings demonstrate that the novel RAP80-binding partner TRAIP regulates recruitment of the damage signalling machinery and promotes homologous recombination.

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ER -

TRAIP/RNF206 is required for recruitment of RAP80 to sites of DNA damage

Abstract

ASJC Scopus subject areas

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