Efficient and risk-reduced genome editing using double nicks enhanced by bacterial recombination factors in multiple species

Author:

He Xiaozhen1,Chen Wenfeng1,Liu Zhen2,Yu Guirong1,Chen Youbang1,Cai Yi-Jun2,Sun Ling1,Xu Wanli1,Zhong Lili1,Gao Caixi1,Chen Jishen1,Zhang Minjie1,Yang Shengxi1,Yao Yizhou1,Zhang Zhiping1,Ma Fujun1,Zhang Chen-Chen2,Lu Hui-Ping2,Yu Bin2,Cheng Tian-Lin2,Qiu Juhui3,Sheng Qing4,Zhou Hai-Meng45,Lv Zhi-Rong5,Yan Junjun6,Zhou Yongjian7,Qiu Zilong2,Cui Zongbin6,Zhang Xi1,Meng Anming3,Sun Qiang2,Yang Yufeng1ORCID

Affiliation:

1. Institute of Life Sciences, Fuzhou University, Fuzhou, Fujian 350108, China

2. Institute of Neuroscience, CAS Center for Excellence in Brain Science and Intelligence Technology, State Key Laboratory of Neuroscience, CAS Key Laboratory of Primate Neurobiology, Chinese Academy of Sciences, Shanghai 200031, China

3. State Key Laboratory of Biomembrane and Membrane Engineering, Tsinghua-Peking Center for Life Sciences, School of Life Sciences, Tsinghua University, Beijing 100084, China

4. College of Life Sciences, Zhejiang Sci-Tech University, Hangzhou, Zhejiang 310018, China

5. Zhejiang Provincial Key Laboratory of Applied Enzymology, Yangtze Delta Region Institute of Tsinghua University, Jiaxing, Zhejiang 314006, China

6. State Key Laboratory of Freshwater Ecology and Biotechnology, Institute of Hydrobiology, Chinese Academy of Sciences, Wuhan, Hubei 430072, China

7. Department of Gastric Surgery, Union Hospital of Fujian Medical University, Fuzhou, Fujian 350001, China

Abstract

Abstract Site-specific DNA double-strand breaks have been used to generate knock-in through the homology-dependent or -independent pathway. However, low efficiency and accompanying negative impacts such as undesirable indels or tumorigenic potential remain problematic. In this study, we present an enhanced reduced-risk genome editing strategy we named as NEO, which used either site-specific trans or cis double-nicking facilitated by four bacterial recombination factors (RecOFAR). In comparison to currently available approaches, NEO achieved higher knock-in (KI) germline transmission frequency (improving from zero to up to 10% efficiency with an average of 5-fold improvement for 8 loci) and ‘cleaner’ knock-in of long DNA fragments (up to 5.5 kb) into a variety of genome regions in zebrafish, mice and rats. Furthermore, NEO yielded up to 50% knock-in in monkey embryos and 20% relative integration efficiency in non-dividing primary human peripheral blood lymphocytes (hPBLCs). Remarkably, both on-target and off-target indels were effectively suppressed by NEO. NEO may also be used to introduce low-risk unrestricted point mutations effectively and precisely. Therefore, by balancing efficiency with safety and quality, the NEO method reported here shows substantial potential and improves the in vivo gene-editing strategies that have recently been developed.

Funder

Fujian Province Min-River Scholar

National Natural Science Foundation of China

Fuzhou University Sci-Tech Innovation

Shanghai Municipal Government Bureau of Science

National Key Research and Development Program of China

Fuzhou University

Fujian Natural Science Foundation

Education and Scientific Research Projects of Young Teachers in Fujian Province

National Basic Research Program of China

CAS Strategic Priority Research Program

Publisher

Oxford University Press (OUP)

Subject

Genetics

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