Poly(ADP-ribose) polymerase-1 antagonizes DNA resection at double-strand breaks

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作者
Marie-Christine Caron
Ajit K. Sharma
Julia O’Sullivan
Logan R. Myler
Maria Tedim Ferreira
Amélie Rodrigue
Yan Coulombe
Chantal Ethier
Jean-Philippe Gagné
Marie-France Langelier
John M. Pascal
Ilya J. Finkelstein
Michael J. Hendzel
Guy G. Poirier
Jean-Yves Masson
机构
[1] CHU de Québec Research Center,Genome Stability Laboratory
[2] HDQ Pavilion,Department of Molecular Biology, Medical Biochemistry and Pathology
[3] Oncology Division,Department of Oncology, Faculty of Medicine and Dentistry
[4] Laval University Cancer Research Center,Department of Molecular Biosciences
[5] University of Alberta,CHU de Québec Research Center
[6] University of Texas at Austin,Biochemistry and Molecular Medicine
[7] CHUL Pavilion,undefined
[8] Oncology Division,undefined
[9] Université de Montréal,undefined
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摘要
PARP-1 is rapidly recruited and activated by DNA double-strand breaks (DSBs). Upon activation, PARP-1 synthesizes a structurally complex polymer composed of ADP-ribose units that facilitates local chromatin relaxation and the recruitment of DNA repair factors. Here, we identify a function for PARP-1 in DNA DSB resection. Remarkably, inhibition of PARP-1 leads to hyperresected DNA DSBs. We show that loss of PARP-1 and hyperresection are associated with loss of Ku, 53BP1 and RIF1 resection inhibitors from the break site. DNA curtains analysis show that EXO1-mediated resection is blocked by PARP-1. Furthermore, PARP-1 abrogation leads to increased DNA resection tracks and an increase of homologous recombination in cellulo. Our results, therefore, place PARP-1 activation as a critical early event for DNA DSB repair activation and regulation of resection. Hence, our work has direct implications for the clinical use and effectiveness of PARP inhibition, which is prescribed for the treatment of various malignancies.
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