ATM and PRDM9 regulate SPO11-bound recombination intermediates during meiosis Journal Article


Authors: Paiano, J.; Wu, W.; Yamada, S.; Sciascia, N.; Callen, E.; Paola Cotrim, A.; Deshpande, R. A.; Maman, Y.; Day, A.; Paull, T. T.; Nussenzweig, A.
Article Title: ATM and PRDM9 regulate SPO11-bound recombination intermediates during meiosis
Abstract: Meiotic recombination is initiated by SPO11-induced double-strand breaks (DSBs). In most mammals, the methyltransferase PRDM9 guides SPO11 targeting, and the ATM kinase controls meiotic DSB numbers. Following MRE11 nuclease removal of SPO11, the DSB is resected and loaded with DMC1 filaments for homolog invasion. Here, we demonstrate the direct detection of meiotic DSBs and resection using END-seq on mouse spermatocytes with low sample input. We find that DMC1 limits both minimum and maximum resection lengths, whereas 53BP1, BRCA1 and EXO1 play surprisingly minimal roles. Through enzymatic modifications to END-seq, we identify a SPO11-bound meiotic recombination intermediate (SPO11-RI) present at all hotspots. We propose that SPO11-RI forms because chromatin-bound PRDM9 asymmetrically blocks MRE11 from releasing SPO11. In Atm–/– spermatocytes, trapped SPO11 cleavage complexes accumulate due to defective MRE11 initiation of resection. Thus, in addition to governing SPO11 breakage, ATM and PRDM9 are critical local regulators of mammalian SPO11 processing. © 2020, This is a U.S. government work and not under copyright protection in the U.S.; foreign copyright protection may apply.
Keywords: mammalia; gene; gene expression; enzyme; recombination; chemical binding; detection method; induced response
Journal Title: Nature Communications
Volume: 11
ISSN: 2041-1723
Publisher: Nature Publishing Group  
Date Published: 2020-02-12
Start Page: 857
Language: English
DOI: 10.1038/s41467-020-14654-w
PUBMED: 32051414
PROVIDER: scopus
PMCID: PMC7016097
DOI/URL:
Notes: Article -- Export Date: 2 March 2020 -- Source: Scopus
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  1. Shintaro   Yamada
    10 Yamada