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基于 dCas9 的基因编辑技术实现长序列无切割基因组基因敲入

dCas9-based gene editing for cleavage-free genomic knock-in of long sequences.

机构信息

Department of Pathology, Stanford University School of Medicine, Stanford, CA, USA.

Department of Genetics, Stanford University School of Medicine, Stanford, CA, USA.

出版信息

Nat Cell Biol. 2022 Feb;24(2):268-278. doi: 10.1038/s41556-021-00836-1. Epub 2022 Feb 10.

Abstract

Gene editing is a powerful tool for genome and cell engineering. Exemplified by CRISPR-Cas, gene editing could cause DNA damage and trigger DNA repair processes that are often error-prone. Such unwanted mutations and safety concerns can be exacerbated when altering long sequences. Here we couple microbial single-strand annealing proteins (SSAPs) with catalytically inactive dCas9 for gene editing. This cleavage-free gene editor, dCas9-SSAP, promotes the knock-in of long sequences in mammalian cells. The dCas9-SSAP editor has low on-target errors and minimal off-target effects, showing higher accuracy than canonical Cas9 methods. It is effective for inserting kilobase-scale sequences, with an efficiency of up to approximately 20% and robust performance across donor designs and cell types, including human stem cells. We show that dCas9-SSAP is less sensitive to inhibition of DNA repair enzymes than Cas9 references. We further performed truncation and aptamer engineering to minimize its size to fit into a single adeno-associated-virus vector for future application. Together, this tool opens opportunities towards safer long-sequence genome engineering.

摘要

基因编辑是基因组和细胞工程的强大工具。以 CRISPR-Cas 为例,基因编辑会导致 DNA 损伤,并触发经常容易出错的 DNA 修复过程。在改变长序列时,这种不需要的突变和安全问题会更加严重。在这里,我们将微生物单链退火蛋白 (SSAP) 与无催化活性的 dCas9 结合起来用于基因编辑。这种无切割的基因编辑工具 dCas9-SSAP 可促进哺乳动物细胞中长序列的敲入。dCas9-SSAP 编辑器的靶标错误率较低,脱靶效应最小,比经典 Cas9 方法具有更高的准确性。它可以有效地插入千碱基规模的序列,效率高达约 20%,并且在供体设计和细胞类型方面具有稳健的性能,包括人类干细胞。我们表明,dCas9-SSAP 对 DNA 修复酶的抑制作用不如 Cas9 对照敏感。我们进一步进行了截断和适体工程改造,将其尺寸最小化,以适合单个腺相关病毒载体,用于未来的应用。总之,该工具为更安全的长序列基因组工程开辟了机会。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1000/8843813/de84e413229c/41556_2021_836_Fig1_HTML.jpg

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