DNA-PK and the TRF2 iDDR inhibit MRN-initiated resection at leading-end telomeres

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作者
Logan R. Myler
Beatrice Toia
Cara K. Vaughan
Kaori Takai
Andreea M. Matei
Peng Wu
Tanya T. Paull
Titia de Lange
Francisca Lottersberger
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[1] The Rockefeller University,Laboratory for Cell Biology and Genetics
[2] Linköping University,Department of Biomedical and Clinical Sciences, Faculty of Medicine and Health Sciences
[3] University of Texas at Austin,Department of Molecular Biosciences
[4] Stanford University School of Medicine,Department of Pediatrics
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Telomeres replicated by leading-strand synthesis lack the 3′ overhang required for telomere protection. Surprisingly, resection of these blunt telomeres is initiated by the telomere-specific 5′ exonuclease Apollo rather than the Mre11–Rad50–Nbs1 (MRN) complex, the nuclease that acts at DNA breaks. Without Apollo, leading-end telomeres undergo fusion, which, as demonstrated here, is mediated by alternative end joining. Here, we show that DNA-PK and TRF2 coordinate the repression of MRN at blunt mouse telomeres. DNA-PK represses an MRN-dependent long-range resection, while the endonuclease activity of MRN–CtIP, which could cleave DNA-PK off of blunt telomere ends, is inhibited in vitro and in vivo by the iDDR of TRF2. AlphaFold-Multimer predicts a conserved association of the iDDR with Rad50, potentially interfering with CtIP binding and MRN endonuclease activation. We propose that repression of MRN-mediated resection is a conserved aspect of telomere maintenance and represents an ancient feature of DNA-PK and the iDDR.
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页码:1346 / 1356
页数:10
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