CRISPR-Cas9-Mediated Editing of the CYP82E4-Nicotine N-Demethylase (nnd) Gene in Tobacco Protoplasts

Ankita Shrestha, Ahamed Khan, N. Dey
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引用次数: 2

Abstract

The single RNA‐guided DNA recognition CRISPR-Cas9 method is a simple and powerful tool for targeted genome engineering. Here, we report the designing and testing of efficient caulimoviral promoter-derived binary vectors for performing genome editing employing the CRISPR-Cas9-gRNA system. For such targeted mutagenesis, we created binary transformation vectors to drive the expression of Cas9 by an efficient caulimoviral promoter, ‘M24’ isolated and characterized from the Mirabilis Mosaic Virus (MMV). The 20-nucleotide CRISPR guide (g)-RNAs were designed to induce targeted mutations in the CYP82E4-nicotine N-demethylase (nnd) gene of tobacco (Nicotiana tabacum). For editing the nnd gene, we employed a pair of gRNAs followed by the protospacer adjacent motif (PAM) targeting the first exon of the nnd-ORF. We evaluated the percent “indels” using tobacco protoplast cells where mutagenesis frequencies were recorded as 45% and 30% for the two targets respectively. A mutagenesis efficiency of 37% was obtained upon the simultaneous transfection of the two gRNAs in tobacco protoplasts. Successful demonstration of our caulimoviral-based CRISPR-Cas9-gRNA system bodes well for its near-term use as a potential and facile means to performing targeted genome editing in plants.
crispr - cas9介导的烟草原生质体cyp82e4 -尼古丁n -去甲基化酶(nnd)基因编辑
单RNA引导的DNA识别CRISPR-Cas9方法是一种简单而强大的靶向基因组工程工具。在这里,我们报道了利用CRISPR-Cas9-gRNA系统进行基因组编辑的有效的茎状病毒启动子衍生的二元载体的设计和测试。为了实现这种靶向诱变,我们创建了二元转化载体,通过从Mirabilis花叶病毒(MMV)中分离并鉴定的高效caulimoviral promoter ' M24 '来驱动Cas9的表达。设计20个核苷酸的CRISPR引导(g)- rna诱导烟草(Nicotiana tabacum) cyp82e4 -尼古丁n -去甲基化酶(nnd)基因的靶向突变。为了编辑nnd基因,我们使用了一对grna,然后是针对nnd- orf的第一个外显子的原间隔邻近基序(PAM)。我们评估了烟草原生质体细胞诱变率分别为45%和30%的“indels”百分比。在烟草原生质体中同时转染这两种grna的诱变效率为37%。我们基于茎状病毒的CRISPR-Cas9-gRNA系统的成功演示预示着它将在短期内作为一种潜在的、简便的方法在植物中进行靶向基因组编辑。
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