Deletion and replacement of long genomic sequences using prime editing

被引:0
|
作者
Tingting Jiang
Xiao-Ou Zhang
Zhiping Weng
Wen Xue
机构
[1] University of Massachusetts Medical School,RNA Therapeutics Institute
[2] University of Massachusetts Medical School,Program in Bioinformatics and Integrative Biology
[3] Tongji University,School of Life Sciences and Technology
[4] University of Massachusetts Medical School,Department of Molecular, Cell and Cancer Biology
[5] University of Massachusetts Medical School,Department of Molecular Medicine
[6] University of Massachusetts Medical School,Li Weibo Institute for Rare Diseases Research
来源
Nature Biotechnology | 2022年 / 40卷
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摘要
Genomic insertions, duplications and insertion/deletions (indels), which account for ~14% of human pathogenic mutations, cannot be accurately or efficiently corrected by current gene-editing methods, especially those that involve larger alterations (>100 base pairs (bp)). Here, we optimize prime editing (PE) tools for creating precise genomic deletions and direct the replacement of a genomic fragment ranging from ~1 kilobases (kb) to ~10 kb with a desired sequence (up to 60 bp) in the absence of an exogenous DNA template. By conjugating Cas9 nuclease to reverse transcriptase (PE-Cas9) and combining it with two PE guide RNAs (pegRNAs) targeting complementary DNA strands, we achieve precise and specific deletion and repair of target sequences via using this PE-Cas9-based deletion and repair (PEDAR) method. PEDAR outperformed other genome-editing methods in a reporter system and at endogenous loci, efficiently creating large and precise genomic alterations. In a mouse model of tyrosinemia, PEDAR removed a 1.38-kb pathogenic insertion within the Fah gene and precisely repaired the deletion junction to restore FAH expression in liver.
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页码:227 / 234
页数:7
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