The Key Laboratory of Industrial Biotechnology (Ministry of Education), School of Biotechnology, Jiangnan University, 1800 Lihu Avenue, Wuxi, 214122, China.
Science Center for Future Foods, Jiangnan University, Wuxi, 214122, China.
Adv Sci (Weinh). 2024 Jun;11(22):e2309767. doi: 10.1002/advs.202309767. Epub 2024 Apr 11.
Base editors (BEs) are widely used as revolutionary genome manipulation tools for cell evolution. To screen the targeted individuals, it is often necessary to expand the editing window to ensure highly diverse variant library. However, current BEs suffer from a limited editing window of 5-6 bases, corresponding to only 2-3 amino acids. Here, by engineering the CRISPR‒Cas12b, the study develops dCas12b-based CRISPRi system, which can efficiently repress gene expression by blocking the initiation and elongation of gene transcription. Further, based on dCas12b, a new-generation of BEs with an expanded editing window is established, covering the entire protospacer or more. The expanded editing window results from the smaller steric hindrance compared with other Cas proteins. The universality of the new BE is successfully validated in Bacillus subtilis and Escherichia coli. As a proof of concept, a spectinomycin-resistant E. coli strain (BL21) and a 6.49-fold increased protein secretion efficiency in E. coli JM109 are successfully obtained by using the new BE. The study, by tremendously expanding the editing window of BEs, increased the capacity of the variant library exponentially, greatly increasing the screening efficiency for microbial cell evolution.
碱基编辑器 (BEs) 被广泛用作细胞进化的革命性基因组操作工具。为了筛选目标个体,通常需要扩展编辑窗口以确保高度多样化的变体文库。然而,当前的 BEs 受到 5-6 个碱基的编辑窗口限制,对应于仅 2-3 个氨基酸。在这里,通过对 CRISPR-Cas12b 的工程改造,该研究开发了基于 dCas12b 的 CRISPRi 系统,该系统可以通过阻止基因转录的起始和延伸来有效抑制基因表达。此外,基于 dCas12b,建立了一种具有扩展编辑窗口的新一代 BE,可以覆盖整个原间隔或更多。与其他 Cas 蛋白相比,扩展的编辑窗口来自更小的空间位阻。该新型 BE 的通用性已在枯草芽孢杆菌和大肠杆菌中得到成功验证。作为概念验证,通过使用新型 BE,成功获得了壮观霉素抗性大肠杆菌菌株 (BL21) 和大肠杆菌 JM109 中蛋白质分泌效率提高了 6.49 倍。该研究通过极大地扩展 BE 的编辑窗口,使变体文库的容量呈指数级增长,极大地提高了微生物细胞进化的筛选效率。
Zotero 插件
