Docking sites inside Cas9 for adenine base editing diversification and RNA off-target elimination

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作者
Shuo Li
Bo Yuan
Jixin Cao
Jingqi Chen
Jinlong Chen
Jiayi Qiu
Xing-Ming Zhao
Xiaolin Wang
Zilong Qiu
Tian-Lin Cheng
机构
[1] Fudan University,Department of interventional Radiology, Zhongshan Hospital
[2] Chinese Academy of Sciences,Institute of Neuroscience, State Key Laboratory of Neuroscience, CAS Center for excellence in Brain Science and Intelligence Technology
[3] Fudan University,Institute of Science and Technology for Brain
[4] Fudan University,Inspired Intelligence, Key Laboratory of Computational Neuroscience and Brain
[5] Shanghai Institute of Medical Imaging,Inspired Intelligence, Ministry of Education
[6] Fudan University,Institute for Translational Brain Research, MOE Frontiers Center for Brain Science
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摘要
Base editing tools with diversified editing scopes and minimized RNA off-target activities are required for broad applications. Nevertheless, current Streptococcus pyogenes Cas9 (SpCas9)-based adenine base editors (ABEs) with minimized RNA off-target activities display constrained editing scopes with efficient editing activities at positions 4-8. Here, functional ABE variants with diversified editing scopes and reduced RNA off-target activities are identified using domain insertion profiling inside SpCas9 and with different combinations of TadA variants. Engineered ABE variants in this study display narrowed, expanded or shifted editing scopes with efficient editing activities across protospacer positions 2-16. And when combined with deaminase engineering, the RNA off-target activities of engineered ABE variants are further minimized. Thus, domain insertion profiling provides a framework to improve and expand ABE toolkits, and its combination with other strategies for ABE engineering deserves comprehensive explorations in the future.
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