Precision genome editing using cytosine and adenine base editors in mammalian cells

被引:0
|
作者
Tony P. Huang
Gregory A. Newby
David R. Liu
机构
[1] The Broad Institute of Harvard and MIT,Merkin Institute of Transformative Technologies in Healthcare
[2] Harvard University,Department of Chemistry and Chemical Biology
[3] Harvard University,Howard Hughes Medical Institute
来源
Nature Protocols | 2021年 / 16卷
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摘要
Genome editing has transformed the life sciences and has exciting prospects for use in treating genetic diseases. Our laboratory developed base editing to enable precise and efficient genome editing while minimizing undesired byproducts and toxicity associated with double-stranded DNA breaks. Adenine and cytosine base editors mediate targeted A•T-to-G•C or C•G-to-T•A base pair changes, respectively, which can theoretically address most human disease-associated single-nucleotide polymorphisms. Current base editors can achieve high editing efficiencies—for example, approaching 100% in cultured mammalian cells or 70% in adult mouse neurons in vivo. Since their initial description, a large set of base editor variants have been developed with different on-target and off-target editing characteristics. Here, we describe a protocol for using base editing in cultured mammalian cells. We provide guidelines for choosing target sites, appropriate base editor variants and delivery strategies to best suit a desired application. We further describe standard base-editing experiments in HEK293T cells, along with computational analysis of base-editing outcomes using CRISPResso2. Beginning with target DNA site selection, base-editing experiments in mammalian cells can typically be completed within 1–3 weeks and require only standard molecular biology techniques and readily available plasmid constructs.
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页码:1089 / 1128
页数:39
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