| Literature DB >> 27477910 |
Andres Canela1, Sriram Sridharan1, Nicholas Sciascia1, Anthony Tubbs1, Paul Meltzer2, Barry P Sleckman3, André Nussenzweig4.
Abstract
DNA double-strand breaks (DSBs) arise during physiological transcription, DNA replication, and antigen receptor diversification. Mistargeting or misprocessing of DSBs can result in pathological structural variation and mutation. Here we describe a sensitive method (END-seq) to monitor DNA end resection and DSBs genome-wide at base-pair resolution in vivo. We utilized END-seq to determine the frequency and spectrum of restriction-enzyme-, zinc-finger-nuclease-, and RAG-induced DSBs. Beyond sequence preference, chromatin features dictate the repertoire of these genome-modifying enzymes. END-seq can detect at least one DSB per cell among 10,000 cells not harboring DSBs, and we estimate that up to one out of 60 cells contains off-target RAG cleavage. In addition to site-specific cleavage, we detect DSBs distributed over extended regions during immunoglobulin class-switch recombination. Thus, END-seq provides a snapshot of DNA ends genome-wide, which can be utilized for understanding genome-editing specificities and the influence of chromatin on DSB pathway choice. Published by Elsevier Inc.Entities:
Mesh:
Substances:
Year: 2016 PMID: 27477910 PMCID: PMC6299834 DOI: 10.1016/j.molcel.2016.06.034
Source DB: PubMed Journal: Mol Cell ISSN: 1097-2765 Impact factor: 17.970