Global and transcription-coupled repair of 8-oxoG is initiated by nucleotide excision repair proteins

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Namrata Kumar
Arjan F. Theil
Vera Roginskaya
Yasmin Ali
Michael Calderon
Simon C. Watkins
Ryan P. Barnes
Patricia L. Opresko
Alex Pines
Hannes Lans
Wim Vermeulen
Bennett Van Houten
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[1] University of Pittsburgh School of Medicine,Molecular Genetics and Developmental Biology graduate program
[2] UPMC Hillman Cancer Center,Department of Molecular Genetics, Oncode Institute, Erasmus MC
[3] University Medical Center Rotterdam,Department of Pharmacology and Chemical Biology
[4] Dr. Molewaterplein 40,Center for Biologic Imaging
[5] University of Pittsburgh School of Medicine,Department of Environmental and Occupational Health
[6] University of Pittsburgh,undefined
[7] University of Pittsburgh Graduate School of Public Health,undefined
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UV-DDB, consisting of subunits DDB1 and DDB2, recognizes UV-induced photoproducts during global genome nucleotide excision repair (GG-NER). We recently demonstrated a noncanonical role of UV-DDB in stimulating base excision repair (BER) which raised several questions about the timing of UV-DDB arrival at 8-oxoguanine (8-oxoG), and the dependency of UV-DDB on the recruitment of downstream BER and NER proteins. Using two different approaches to introduce 8-oxoG in cells, we show that DDB2 is recruited to 8-oxoG immediately after damage and colocalizes with 8-oxoG glycosylase (OGG1) at sites of repair. 8-oxoG removal and OGG1 recruitment is significantly reduced in the absence of DDB2. NER proteins, XPA and XPC, also accumulate at 8-oxoG. While XPC recruitment is dependent on DDB2, XPA recruitment is DDB2-independent and transcription-coupled. Finally, DDB2 accumulation at 8-oxoG induces local chromatin unfolding. We propose that DDB2-mediated chromatin decompaction facilitates the recruitment of downstream BER proteins to 8-oxoG lesions.
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