Author:
Wang Yanhong,Zhou Lifang,Tao Rui,Liu Nan,Long Jie,Qin Fengming,Tang Wenling,Yang Yang,Chen Qiang,Yao Shaohua
Abstract
AbstractWe present a base editing system, in which base editors are attached to different sites of sgRNA scaffold (sgBE). Each independent sgBE has its own specific editing pattern for a given target site. Among tested sgBEs, sgBE-SL4, in which deaminase is attached to the last stem-loop of sgRNA, yields the highest editing efficiency in the window several nucleotides next to the one edited by BE3. sgBE enables the simultaneous editing of adenine and cytosine. Finally, in order to facilitate in vivo base editing, we extend our sgBE system to an AAV-compatible Cas9, SaCas9 (Staphylococcus aureus), and observe robust base editing.
Funder
National Natural Science Foundation of China
National High-tech Research and Development Program
Publisher
Springer Science and Business Media LLC
Cited by
20 articles.
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