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基于转座酶 B 引导的工程 RNA 的超紧凑型腺嘌呤碱基编辑器。

Hypercompact adenine base editors based on transposase B guided by engineered RNA.

机构信息

GenKOre, Daejeon, Republic of Korea.

KRIBB School of Bioscience, Korea University of Science and Technology, Daejeon, Republic of Korea.

出版信息

Nat Chem Biol. 2022 Sep;18(9):1005-1013. doi: 10.1038/s41589-022-01077-5. Epub 2022 Aug 1.

Abstract

Transposon-associated transposase B (TnpB) is deemed an ancestral protein for type V, Cas12 family members, and the closest ancestor to UnCas12f1. Previously, we reported a set of engineered guide RNAs supporting high indel efficiency for Cas12f1 in human cells. Here we suggest a new technology whereby the engineered guide RNAs also manifest high-efficiency programmable endonuclease activity for TnpB. We have termed this technology TaRGET (TnpB-augment RNA-based Genome Editing Technology). Having this feature in mind, we established TnpB-based adenine base editors (ABEs). A Tad-Tad mutant (V106W, D108Q) dimer fused to the C terminus of dTnpB (D354A) showed the highest levels of A-to-G conversion. The limited targetable sites for TaRGET-ABE were expanded with engineered variants of TnpB or optimized deaminases. Delivery of TaRGET-ABE also ensured potent A-to-G conversion rates in mammalian genomes. Collectively, the TaRGET-ABE will contribute to improving precise genome-editing tools that can be delivered by adeno-associated viruses, thereby harnessing the development of clustered regularly interspaced short palindromic repeats (CRISPR)-based gene therapy.

摘要

转座子相关转座酶 B(TnpB)被认为是第五型、Cas12 家族成员的原始蛋白,也是 UnCas12f1 的最接近祖先。此前,我们报道了一组工程化的指导 RNA,可支持 Cas12f1 在人类细胞中实现高效的缺失效率。在这里,我们提出了一种新技术,即这些工程化的指导 RNA 也表现出对 TnpB 的高效可编程内切酶活性。我们将这项技术称为 TaRGET(TnpB 增强 RNA 为基础的基因组编辑技术)。考虑到这一特点,我们建立了基于 TnpB 的腺嘌呤碱基编辑器(ABE)。与 dTnpB(D354A)的 C 末端融合的 Tad-Tad 突变体(V106W,D108Q)二聚体显示出最高水平的 A 到 G 转换。通过工程化的 TnpB 变体或优化的脱氨酶,可扩展 TaRGET-ABE 的有限靶向靶标。TaRGET-ABE 的递送还确保了哺乳动物基因组中强大的 A 到 G 转换率。总的来说,TaRGET-ABE 将有助于改进可通过腺相关病毒递送的精确基因组编辑工具,从而利用基于成簇规律间隔短回文重复序列(CRISPR)的基因治疗的发展。

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