Identifying genome-wide off-target sites of CRISPR RNA–guided nucleases and deaminases with Digenome-seq

染色质 生物 基因组编辑 Cas9 基因组 清脆的 DNA 基因组DNA 计算生物学 遗传学 基因组文库 DNA纳米球测序 基因 核糖核酸 基因组工程 基序列
作者
Daesik Kim,Beum‐Chang Kang,Jin‐Soo Kim
出处
期刊:Nature Protocols [Nature Portfolio]
卷期号:16 (2): 1170-1192 被引量:23
标识
DOI:10.1038/s41596-020-00453-6
摘要

Digested genome sequencing (Digenome-seq) is a highly sensitive, easy-to-carry-out, cell-free method for experimentally identifying genome-wide off-target sites of programmable nucleases and deaminases (also known as base editors). Genomic DNA is digested in vitro using clustered regularly interspaced short palindromic repeats ribonucleoproteins (RNPs; plus DNA-modifying enzymes to cleave both strands of DNA at sites containing deaminated base products, in the case of base editors) and subjected to whole-genome sequencing (WGS) with a typical sequencing depth of 30×. A web-based program is available to map in vitro cleavage sites corresponding to on- and off-target sites. Chromatin DNA, in parallel with histone-free genomic DNA, can also be used to account for the effects of chromatin structure on off-target nuclease activity. Digenome-seq is more sensitive and comprehensive than cell-based methods for identifying off-target sites. Unlike other cell-free methods, Digenome-seq does not involve enrichment of DNA ends through PCR amplification. The entire process other than WGS, which takes ~1–2 weeks, including purification and preparation of RNPs, digestion of genomic DNA and bioinformatic analysis after WGS, takes about several weeks. This protocol describes a cell-free method for experimentally identifying genome-wide off-target sites of CRISPR nucleases and deaminases through in vitro digestion of genomic DNA or chromatin followed by whole-genome sequencing.
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