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Efficient and high-fidelity base editor with expanded PAM compatibility for cytidine dinucleotide

机译:高效且高保真基础编辑器,具有扩大的胞苷二核苷酸的PAM兼容性

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Cytidine base editor (CBE), which is composed of a cytidine deaminase fused to Cas9 nickase, has been widely used to induce C-to-T conversions in a wide range of organisms. However, the targeting scope of current CBEs is largely restricted to protospacer adjacent motif (PAM) sequences containing G, T, or A bases. In this study, we developed a new base editor termed “nNme2-CBE” with excellent PAM compatibility for cytidine dinucleotide, significantly expanding the genome-targeting scope of CBEs. Using nNme2-CBE, targeted editing efficiencies of 29.0%–55.0% and 17.3%–52.5% were generated in human cells and rabbit embryos, respectively. In contrast to conventional nSp-CBE, the nNme2-CBE is a natural high-fidelity base editing platform with minimal DNA off-targeting detected in vivo. Significantly increased efficiency in GC context and precision were determined by combining nNme2Cas9 with rationally engineered cytidine deaminases. In addition, the Founder rabbits with accurate single-base substitutions at Fgf5 gene loci were successfully generated by using the nNme2-CBE system. These novel nNme2-CBEs with expanded PAM compatibility and high fidelity will expand the base editing toolset for efficient gene modification and therapeutic applications.
机译:胞苷基础编辑器(CBE)由融合到Cas9酸碱酶的胞苷脱氨酶组成,已被广泛用于诱导各种生物中的C-T次转化。然而,目前CBE的靶向范围主要限于含有G,T或碱基的强化器相邻的基序(PAM)序列。在这项研究中,我们开发了一种新的碱基编辑,具有“NNME2-CBE”,具有优异的胞苷二核苷酸的PAM兼容性,显着扩展CBE的基因组靶向范围。使用NNME2-CBE,分别在人细胞和兔胚胎中产生29.0%-55.0%和17.3%-52.5%的目标编辑效率。与传统的NSP-CBE相反,NNME2-CBE是一种自然高保真基础编辑平台,在体内检测到最小的DNA脱靶。通过将NNME2CAS9与理性工程胞苷脱氨酶组合来确定GC上下文和精度的显着提高。此外,通过使用NNME2-CBE系统成功地生成了在FGF5基因基因座上精确单碱基取代的创始人兔。这些具有扩展PAM兼容性和高保真性的新型NNME2-CBE将扩展基本编辑工具集以获得有效的基因改性和治疗应用。

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