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Efficient precise integration of large DNA sequences with 3′-overhang dsDNA donors using CRISPR/Cas9

Proceedings of the national academy of sciences of the USA. 2023-05; 
Wenjie Han, Zhigang Li, Yijun Guo, Kaining He, Wenqing Li, Caoling Xu, Lishuang Ge, Miao He, Xue Yin, Junxiang Zhou, Chengxu Li, Dongbao Yao, Jianqiang Bao, Haojun Liang
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CRISPR RNAs/Cas9 Proteins(INACTIVE) . The extraction method of Cas9-PCV2 protein was the same as the above, PCV2 gene was synthesized (Sangon Biotech) and Cas9-PCV2 plasmid (sequence in SI Appendix, Table S9) was assembled by Gibson assembly. GenCRISPR Cas9 v1.2 (Genscript) Get A Quote

摘要

CRISPR/Cas9 genome-editing tools have tremendously boosted our capability of manipulating the eukaryotic genomes in biomedical research and innovative biotechnologies. However, the current approaches that allow precise integration of gene-sized large DNA fragments generally suffer from low efficiency and high cost. Herein, we developed a versatile and efficient approach, termed LOCK (Long dsDNA with 3'-Overhangs mediated CRISPR Knock-in), by utilizing specially designed 3'-overhang double-stranded DNA (odsDNA) donors harboring 50-nt homology arm. The length of the 3'-overhangs of odsDNA is specified by the five consecutive phosphorothioate modifications. Compared with existing methods, LOCK allows highly effici... More

關鍵詞

3′-overhangs dsDNA; CRISPR knock-in; double-stranded break; off-target effect; phosphorothioate modification
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