Large DNA deletions occur during DNA repair at 20-fold lower frequency for base editors and prime editors than for Cas9 nucleases

DNA 清脆的 Cas9 分子生物学 生物 计算生物学 遗传学 基因
作者
Gue‐Ho Hwang,Seok‐Hoon Lee,Minsik Oh,Segi Kim,Omer Habib,Hyeon‐Ki Jang,Heon Seok Kim,Youngkuk Kim,Chan Hyuk Kim,Sun Kim,Sangsu Bae
出处
期刊:Nature Biomedical Engineering [Springer Nature]
标识
DOI:10.1038/s41551-024-01277-5
摘要

When used to edit genomes, Cas9 nucleases produce targeted double-strand breaks in DNA. Subsequent DNA-repair pathways can induce large genomic deletions (larger than 100 bp), which constrains the applicability of genome editing. Here we show that Cas9-mediated double-strand breaks induce large deletions at varying frequencies in cancer cell lines, human embryonic stem cells and human primary T cells, and that most deletions are produced by two repair pathways: end resection and DNA-polymerase theta-mediated end joining. These findings required the optimization of long-range amplicon sequencing, the development of a k-mer alignment algorithm for the simultaneous analysis of large DNA deletions and small DNA alterations, and the use of CRISPR-interference screening. Despite leveraging mutated Cas9 nickases that produce single-strand breaks, base editors and prime editors also generated large deletions, yet at approximately 20-fold lower frequency than Cas9. We provide strategies for the mitigation of such deletions. DNA repair after Cas9-mediated double-strand breaks induces large DNA deletions at frequencies 20-fold higher than elicited by base editors and prime editors leveraging Cas9 nickases producing single-strand breaks.
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