Utilization of nicking properties of CRISPR-Cas12a effector for genome editing

Author:

Kim Chan Hyoung1,Lee Wi-jae2,Oh Yeounsun2,Lee Youngjeon3,Lee Hyomin K.4,Seong Jung Bae3,Lim Kyung-Seob3,Park Sang Je3,Huh Jae-Won3,Kim Young-Hyun3,Kim Kyoung Mi1,Hur Junho K.4,Lee Seung Hwan2

Affiliation:

1. Chungnam National University

2. Chung-Ang University

3. Korea Research Institute of Bioscience and Biotechnology (KRIBB)

4. Hanyang University

Abstract

Abstract The CRISPR-Cas nickase system for genome editing has attracted considerable attention owing to its safety, efficiency, and versatility. Although alternative effectors to Cas9 have the potential to expand the scope of genome editing, their application has not been optimized. Herein, we used an enhanced CRISPR-Cas12a nickase system to induce mutations by targeting genes in a human-derived cell line. The newly developed CRISPR-Cas12a nickase system effectively introduced mutations into target genes under a specific directionality and distance between nickases. In particular, the single-mode Cas12a nickase system can induce the target-specific mutations with less DNA double-strand breaks. By effectively inducing mutations in the Thymine-rich target genes in single- or dual-mode, Cas12a nickase addresses the limitations of Cas9 nickase and is expected to contribute to the development of future genome editing technologies.

Publisher

Research Square Platform LLC

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