PhieDBEs: a DBD‐containing, PAM‐flexible, high‐efficiency dual base editor toolbox with wide targeting scope for use in plants

Author:

Zheng Zhiye1,Liu Taoli1,Chai Nan1,Zeng Dongchang12,Zhang Ruixiang1,Wu Yang1,Hang Jiaxuan1,Liu Yuxin1,Deng Qindi1,Tan Jiantao13,Liu Jialin1,Xie Xianrong1,Liu Yao‐Guang1ORCID,Zhu Qinlong1ORCID

Affiliation:

1. State Key Laboratory for Conservation and Utilization of Subtropical Agro‐Bioresources, Guangdong Laboratory for Lingnan Modern Agriculture, College of Agriculture, College of Life Sciences South China Agricultural University Guangzhou China

2. Key Laboratory of Ecology of Rare and Endangered Species and Environmental Protection (Guangxi Normal University) Ministry of Education, Guangxi Key Laboratory of Landscape Resources Conservation and Sustainable Utilization in Lijiang River Basin, Guangxi Normal University Guilin China

3. Rice Research Institute, Guangdong Academy of Agricultural Sciences, Key Laboratory of Genetics and Breeding of High‐Quality Rice in Southern China (Co‐construction by Ministry and Province) Ministry of Agriculture and Rural Affairs, Guangdong Key Laboratory of New Technology in Rice Breeding, Guangdong Rice Engineering Laboratory Guangzhou China

Abstract

SummaryDual base editors (DBEs) enable simultaneous A‐to‐G and C‐to‐T conversions, expanding mutation types. However, low editing efficiency and narrow targeting range limit the widespread use of DBEs in plants. The single‐strand DNA binding domain of RAD51 DBD can be fused to base editors to improve their editing efficiency. However, it remains unclear how the DBD affects dual base editing performance in plants. In this study, we generated a series of novel plant DBE‐SpGn tools consisting of nine constructs using the high‐activity cytidine deaminase evoFERNY, adenosine deaminase TadA8e and DBD in various fusion modes with the PAM‐flexible Streptococcus pyogenes Cas9 (SpCas9) nickase variant SpGn (with NG‐PAM). By analysing their editing performance on 48 targets in rice, we found that DBE‐SpGn constructs containing a single DBD and deaminases located at the N‐terminus of SpGn exhibited the highest editing efficiencies. Meanwhile, constructs with deaminases located at the C‐terminus and/or multiple DBDs failed to function normally and exhibited inhibited editing activity. We identified three particularly high‐efficiency dual base editors (C‐A‐SpGn, C‐A‐D‐SpGn and A‐C‐D‐SpGn), named PhieDBEs (Plant high‐efficiency dual base editors), capable of producing efficient dual base conversions within a narrow editing window (M5 ~ M9, M = A/C). The editing efficiency of C‐A‐D‐SpGn was as high as 95.2% at certain target sites, with frequencies of simultaneous C‐to‐T and A‐to‐G conversions as high as 81.0%. In summary, PhieDBEs (especially C‐A‐D‐SpGn) can produce diverse mutants and may prove useful in a wide variety of applications, including plant functional genomics, precise mutagenesis, directed evolution and crop genetic improvement, among others.

Funder

National Natural Science Foundation of China

National Key Research and Development Program of China

Publisher

Wiley

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