Engineered circular guide RNAs boost CRISPR/Cas12a-and CRISPR/Cas13d-based DNA and RNA editing

被引:8
|
作者
Zhang, Xin [1 ,2 ]
Wang, Xinlong [2 ]
Lv, Jie [2 ]
Huang, Hongxin [3 ]
Wang, Jiahong [2 ]
Zhuo, Ma [2 ]
Tan, Zhihong [2 ]
Huang, Guanjie [2 ]
Liu, Jiawei [2 ]
Liu, Yuchen [2 ]
Li, Mengrao [2 ]
Lin, Qixiao [2 ]
Li, Lian [2 ]
Ma, Shufeng [2 ,4 ]
Huang, Tao [2 ]
Lin, Ying [2 ]
Zhao, Xiaoyang [5 ]
Rong, Zhili [1 ,2 ,3 ]
机构
[1] Southern Med Univ, Affiliated Dongguan Hosp, Dongguan Inst Clin Canc Res, Dongguan 523058, Peoples R China
[2] Southern Med Univ, Canc Res Inst, Natl Clin Res Ctr Kidney Dis, Key Lab Organ Failure Res,Minist Educ,State Key La, Guangzhou 510515, Peoples R China
[3] Southern Med Univ, Dermatol Hosp, Guangzhou 510091, Peoples R China
[4] Southern Med Univ, Shenzhen Hosp, Dept Nephrol, Shenzhen 518110, Peoples R China
[5] Southern Med Univ, Natl Clin Res Ctr Kidney Dis, State Key Lab Organ Failure Res, Dept Dev,Sch Basic Med Sci,Key Lab Organ Failure R, Guangzhou 510515, Peoples R China
来源
GENOME BIOLOGY | 2023年 / 24卷 / 01期
基金
中国博士后科学基金; 中国国家自然科学基金;
关键词
cgRNA; Engineered circular gRNA; Cas12a; Cas13d; Gene activation; DNA editing; RNA editing; IN-VIVO; CPF1; SPECIFICITIES;
D O I
10.1186/s13059-023-02992-z
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
BackgroundThe CRISPR/Cas12a and CRISPR/Cas13d systems are widely used for fundamental research and hold great potential for future clinical applications. However, the short half-life of guide RNAs (gRNAs), particularly free gRNAs without Cas nuclease binding, limits their editing efficiency and durability.ResultsHere, we engineer circular free gRNAs (cgRNAs) to increase their stability, and thus availability for Cas12a and Cas13d processing and loading, to boost editing. cgRNAs increases the efficiency of Cas12a-based transcription activators and genomic DNA cleavage by approximately 2.1- to 40.2-fold for single gene editing and 1.7- to 2.1-fold for multiplexed gene editing than their linear counterparts, without compromising specificity, across multiple sites and cell lines. Similarly, the RNA interference efficiency of Cas13d is increased by around 1.8-fold. In in vivo mouse liver, cgRNAs are more potent in activating gene expression and cleaving genomic DNA.ConclusionsCgRNAs enable more efficient programmable DNA and RNA editing for Cas12a and Cas13d with broad applicability for fundamental research and gene therapy.
引用
收藏
页数:18
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