Deaminase base editing has emerged as a tool to install or correct point mutations in the genomes of living cells in a wide range of organisms. However, the genome-wide off-target effects introduced by base editors in the mammalian genome have been examined in only one study. Here, we have investigated the fidelity of cytosine base editor 4 (BE4) and adenine base editors (ABE) in mouse embryos using unbiased whole-genome sequencing of a family-based trio cohort. The same sgRNA was used for BE4 and ABE. We demonstrate that BE4-edited mice carry an excess of single-nucleotide variants and deletions compared to ABE-edited mice and controls. Therefore, an optimization of cytosine base editors is required to improve its fidelity. While the remarkable fidelity of ABE has implications for a wide range of applications, the occurrence of rare aberrant C-to-T conversions at specific target sites needs to be addressed. Hye Kyung Lee, Harold E. Smith et al. examined the fidelity of cytosine base editor 4 (BE4) and adenine base editors (ABEs) in mouse embryos using whole-genome sequencing of a family-based trio cohort. They show that BE4-edited mice carry more single-nucleotide variants and deletions than ABE-edited mice.
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机译:脱氨酶基础编辑作为在各种生物体中的活细胞基因组中安装或纠正点突变的工具。然而,在哺乳动物基因组中引入的基因组偏移偏移效应仅在一项研究中进行了检查。在这里,我们研究了使用基于家庭的三重组队列的无偏态的全基因组测序来研究胞嘧啶基础编辑器4(Be4)和腺嘌呤基础编辑器(ABE)的脂肪酸碱基编辑器(ABE)。同样的SGRNA用于BE4和ABE。与ABE编辑的小鼠和对照相比,我们证明Be4编辑的小鼠携带过量的单核苷酸变体和缺失。因此,需要优化胞嘧啶基础编辑器来改善其保真度。虽然ABE的显着保真度对广泛的应用具有影响,但需要解决特定目标站点的稀有异常C-T转化的发生。 Hye Kyung Lee,Harold E. Smith等。使用基于家族的三重组队列的全基因组测序检查小鼠胚胎中的胞嘧啶基础编辑器4(Be4)和腺嘌呤基础编辑器(Abes)的保真度。它们表明Be4编辑的小鼠比ABE编辑的小鼠携带更多单核苷酸变体和缺失。
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