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Protein language models-assisted optimization of a uracil-N-glycosylase variant enables programmable T-to-G and T-to-C base editing

Mol Cell . 2024-04; 
Yan He, Xibin Zhou, Chong Chang, Ge Chen, Weikuan Liu, Geng Li, Xiaoqi Fan, Mingsun Sun, Chensi Miao, Qianyue Huang, Yunqing Ma, Fajie Yuan, Xing Chang
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Synthetic sgRNA and crRNA Service Chemically modified sgRNAs were synthesized by Genscript, and mRNA of indicated editors was synthesized using an in vitro RNA transcription kit (mMESSAGE mMACHINE T7 Ultra Kit, Ambion). Get A Quote

摘要

Current base editors (BEs) use DNA deaminases, including cytidine deaminase in cytidine BE (CBE) or adenine deaminase in adenine BE (ABE), to facilitate transition nucleotide substitutions. Combining CBE or ABE with glycosylase enzymes can induce limited transversion mutations. Nonetheless, a critical demand remains for BEs capable of generating alternative mutation types, such as T>G corrections. In this study, we leveraged pre-trained protein language models to optimize a uracil-N-glycosylase (UNG) variant with altered specificity for thymines (eTDG). Notably, after two rounds of testing fewer than 50 top-ranking variants, more than 50% exhibited over 1.5-fold enhancement in enzymatic activities. When eTDG wa... More

关键词

C>G base editing; CRISPR; T-to-C base editing; T-to-G base editing; base excision repair; glycosylase-derived base editor; protein language models.