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An alternative strategy for targeted gene replacement in plants using a dual-sgRNA/Cas9 design

机译:使用双重-sgRNA / Cas9设计的植物靶向基因替代的替代策略

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Precision DNA/gene replacement is a promising genome-editing tool that is highly desirable for molecular engineering and breeding by design. Although the CRISPR/Cas9 system works well as a tool for gene knockout in plants, gene replacement has rarely been reported. Towards this end, we first designed a combinatory dual-sgRNA/Cas9 vector (construct #1) that successfully deleted miRNA gene regions (MIR169a and MIR827a). The deletions were confirmed by PCR and subsequent sequencing, yielding deletion efficiencies of 20% and 24% on MIR169a and MIR827a loci, respectively. We designed a second structure (construct #2) that contains sites homologous to Arabidopsis TERMINAL FLOWER 1 (TFL1) for homology-directed repair (HDR) with regions corresponding to the two sgRNAs on the modified construct #1. The two constructs were co-transformed into Arabidopsis plants to provide both targeted deletion and donor repair for targeted gene replacement by HDR. Four of 500 stably transformed T0 transgenic plants (0.8%) contained replaced fragments. The presence of the expected recombination sites was further confirmed by sequencing. Therefore, we successfully established a gene deletion/replacement system in stably transformed plants that can potentially be utilized to introduce genes of interest for targeted crop improvement.
机译:精确的DNA /基因替换是一种有前途的基因组编辑工具,对于分子工程和设计育种非常需要。尽管CRISPR / Cas9系统可以很好地用作基因敲除植物的工具,但很少有人报道过基因置换的情况。为此,我们首先设计了可成功删除miRNA基因区域(MIR169a和MIR827a)的组合双sgRNA / Cas9载体(结构1)。通过PCR和随后的测序证实了缺失,在MIR169a和MIR827a基因座上分别产生20%和24%的缺失效率。我们设计了第二个结构(第2个结构),该结构包含与拟南芥TERLOWAL FLOWER 1(TFL1)同源的位点,用于同源直接修复(HDR),其区域对应于修饰的第1个构建体上的两个sgRNA。将这两个构建体共转化到拟南芥植物中,以提供靶向缺失和供体修复,以通过HDR替代靶向基因。 500株稳定转化的T0转基因植物中有4株(占0.8%)含有置换片段。通过测序进一步证实了预期的重组位点的存在。因此,我们成功地在稳定转化的植物中建立了基因缺失/置换系统,该系统可潜在地用于引入目标基因以改善目标作物。

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