Precise genomic deletions using paired prime editing

被引:0
|
作者
Junhong Choi
Wei Chen
Chase C. Suiter
Choli Lee
Florence M. Chardon
Wei Yang
Anh Leith
Riza M. Daza
Beth Martin
Jay Shendure
机构
[1] University of Washington,Department of Genome Sciences
[2] Howard Hughes Medical Institute,Molecular Engineering and Sciences Institute
[3] University of Washington,Molecular and Cellular Biology Program
[4] University of Washington,undefined
[5] Brotman Baty Institute for Precision Medicine,undefined
[6] Allen Discovery Center for Cell Lineage Tracing,undefined
来源
Nature Biotechnology | 2022年 / 40卷
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摘要
Current methods to delete genomic sequences are based on clustered regularly interspaced short palindromic repeats (CRISPR)–Cas9 and pairs of single-guide RNAs (sgRNAs), but can be inefficient and imprecise, with errors including small indels as well as unintended large deletions and more complex rearrangements. In the present study, we describe a prime editing-based method, PRIME-Del, which induces a deletion using a pair of prime editing sgRNAs (pegRNAs) that target opposite DNA strands, programming not only the sites that are nicked but also the outcome of the repair. PRIME-Del achieves markedly higher precision than CRISPR–Cas9 and sgRNA pairs in programming deletions up to 10 kb, with 1–30% editing efficiency. PRIME-Del can also be used to couple genomic deletions with short insertions, enabling deletions with junctions that do not fall at protospacer-adjacent motif sites. Finally, extended expression of prime editing components can substantially enhance efficiency without compromising precision. We anticipate that PRIME-Del will be broadly useful for precise, flexible programming of genomic deletions, epitope tagging and, potentially, programming genomic rearrangements.
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页码:218 / 226
页数:8
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