Customized one-step preparation of sgRNA transcription templates via overlapping PCR Using short primers and its application in vitro and in vivo gene editing

Zheng Hu; Li Wang; Zhaoying Shi; Jing Jiang; Xiangning Li; Yonglong Chen; Kai Li; Dixian Luo

doi:10.1186/s13578-019-0350-7

Cell & Bioscience (Oct 2019)

Customized one-step preparation of sgRNA transcription templates via overlapping PCR Using short primers and its application in vitro and in vivo gene editing

Zheng Hu,
Li Wang,
Zhaoying Shi,
Jing Jiang,
Xiangning Li,
Yonglong Chen,
Kai Li,
Dixian Luo

Affiliations

Zheng Hu: The First People’s Hospital of Chenzhou, Affiliated to University of Southern Medical University
Li Wang: The First People’s Hospital of Chenzhou, Affiliated to University of Southern Medical University
Zhaoying Shi: Department of Biology, Guangdong Provincial Key Laboratory of Cell Microenvironment and Disease Research, Shenzhen Key Laboratory of Cell Microenvironment, Southern University of Science and Technology
Jing Jiang: National & Local Joint Engineering Laboratory for High-throughput Molecular Diagnosis Technology, Affiliated to The First People’s Hospital of Chenzhou, University of South China
Xiangning Li: National & Local Joint Engineering Laboratory for High-throughput Molecular Diagnosis Technology, Affiliated to The First People’s Hospital of Chenzhou, University of South China
Yonglong Chen: Department of Biology, Guangdong Provincial Key Laboratory of Cell Microenvironment and Disease Research, Shenzhen Key Laboratory of Cell Microenvironment, Southern University of Science and Technology
Kai Li: National & Local Joint Engineering Laboratory for High-throughput Molecular Diagnosis Technology, Affiliated to The First People’s Hospital of Chenzhou, University of South China
Dixian Luo: The First People’s Hospital of Chenzhou, Affiliated to University of Southern Medical University

DOI: https://doi.org/10.1186/s13578-019-0350-7
Journal volume & issue: Vol. 9, no. 1
pp. 1 – 7

Abstract

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Abstract Overlap extension polymerase chain reaction (PCR) is a powerful technology for DNA assembly. Based on this technology, we synthesized DNA templates, which were transcribed into sgRNA in vitro, and further detected their efficiency of purified sgRNAs with Cas9 nuclease. The sgRNAs synthesized by this approach can effectively cleave the DNA fragments of interest in vitro and in vivo. Compared with the conventional method for generating sgRNA, it does not require construction of recombinant plasmids and design of primers to amplify sgRNA core fragment. Only several short primers with overlapped sequences are needed to assemble a DNA fragment as the template of sgRNA. This modified and simplified method is highly applicable and less time-consuming.

Published in Cell & Bioscience

ISSN: 2045-3701 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Technology: Chemical technology: Biotechnology; Science: Biology (General); Science: Chemistry: Organic chemistry: Biochemistry
Website: https://cellandbioscience.biomedcentral.com/

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Abstract

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