CRISPR/Cas9 nuclease cleavage combined with Gibson assembly for seamless cloning

清脆的 Cas9 核酸酶 劈开 基因组编辑 质粒 生物 DNA 多克隆站点 限制性酶 计算生物学 遗传学 体外重组 分子克隆 分子生物学 基因 重组DNA 肽序列 表达式向量
作者
Jia-Wang Wang,Amy Wang,Kunyu Li,Bangmei Wang,Shunqian Jin,Michelle Reiser,Richard F. Lockey
出处
期刊:BioTechniques [Future Science Ltd]
卷期号:58 (4): 161-170 被引量:57
标识
DOI:10.2144/000114261
摘要

Restriction enzymes have two major limitations for cloning: they cannot cleave at any desired location in a DNA sequence and may not cleave uniquely within a DNA sequence. In contrast, the clustered regularly interspaced short palindromic repeat (CRISPR)–associated enzyme 9 (Cas9), when coupled with single guide RNAs (sgRNA), has been used in vivo to cleave the genomes of many species at a single site, enabling generation of mutated cell lines and animals. The Cas9/sgRNA complex recognizes a 17–20 base target site, which can be of any sequence as long as it is located 5′ of the protospacer adjacent motif (PAM; sequence 5′-NRG, where R = G or A). Thus, it can be programmed to cleave almost anywhere with a stringency higher than that of one cleavage in a sequence of human genome size. Here, the Cas9 enzyme and a specific sgRNA were used to linearize a 22 kb plasmid in vitro. A DNA fragment was then inserted into the linearized vector seamlessly through Gibson assembly. Our technique can be used to directly, and seamlessly, clone fragments into vectors of any size as well as to modify existing constructs where no other methods are available.

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