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Generation of mutant mice via the CRISPR/Cas9 system using FokI-dCas9

机译:使用FokI-dCas9通过CRISPR / Cas9系统生成突变小鼠

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Genome editing, which introduces mutations in genes of interest using artificial DNA nucleases such as the ZFN, TALEN, and CRISPR/Cas9 systems in living cells, is a useful tool for generating mutant animals. Although CRISPR/Cas9 provides advantages over the two other systems, such as an easier vector construction and high efficiency of genome editing, it raises concerns of off-target effects when single guide RNA (gRNA) is used. Recently, FokI-dCas9 (fCas9), a fusion protein comprised of the inactivated mutant form of Cas9 and the DNA nuclease domain of FokI, has been developed. It enables genome editing with reduced risks of off-target effects in mammalian cultured cell lines, as fCas9 requires gRNAs to bind opposite strands with an appropriate distance between them. Here, we demonstrated that fCas9 efficiently generates living mutant mice through microinjection of its mRNA and gRNAs into zygotes. A comparison of the relative efficiencies of genome editing using fCas9 and other modified Cas9s showed that these mutagenesis efficiencies are similar when the targets of two gRNAs are separated by an appropriate distance, suggesting that in addition to the ease of vector construction, fCas9 exhibit high efficiency in producing mutant mice and in reducing risks of off-target effects.
机译:基因组编辑是在活细胞中使用人工DNA核酸酶(例如ZFN,TALEN和CRISPR / Cas9系统)在目标基因中引入突变的工具,是生成突变动物的有用工具。尽管CRISPR / Cas9提供了相对于其他两个系统的优势,例如更容易的载体构建和高效的基因组编辑,但当使用单向导RNA(gRNA)时,它引起了脱靶效应的问题。近来,已经开发出FokI-dCas9(fCas9),其是由Cas9的失活突变体形式和FokI的DNA核酸酶结构域组成的融合蛋白。它使基因组编辑具有降低的哺乳动物培养细胞系脱靶效应的风险,因为fCas9要求gRNA结合相对链之间的距离合适。在这里,我们证明了fCas9通过将其mRNA和gRNA微注射入受精卵有效地产生了活体突变小鼠。使用fCas9和其他修饰的Cas9s编辑基因组的相对效率的比较显示,当两个gRNA的靶标隔开适当的距离时,这些诱变效率相似,这表明fCas9除了载体构建的简便性外,还显示出高效率在生产突变小鼠和减少脱靶效应的风险。

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