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RGEN-seq for highly sensitive amplification-free screen of off-target sites of gene editors

Sci Rep. 2021-12; 
Alexander Kuzin, Brendan Redler, Jaya Onuska, Alexei Slesarev
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Mammalian Expression  Genomic CHO-K1 DNA from the AD49GZ clone was isolated as previously described30; human Hek293 DNA was purchased from Genscript Get A Quote

摘要

Sensitive detection of off-target sites produced by gene editing nucleases is crucial for developing reliable gene therapy platforms. Although several biochemical assays for the characterization of nuclease off-target effects have been recently published, significant technical and methodological issues still remain. Of note, existing methods rely on PCR amplification, tagging, and affinity purification which can introduce bias, contaminants, sample loss through handling, etc. Here we describe a sensitive, PCR-free next-generation sequencing method (RGEN-seq) for unbiased detection of double-stranded breaks generated by RNA-guided CRISPR-Cas9 endonuclease. Through use of novel sequencing adapters, the RGEN-Seq m... More

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