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Excision of Nucleopolyhedrovirus Form Transgenic Silkworm Using the CRISPR/Cas9 System

机译:使用CRISPR / Cas9系统切除核多角体病毒形成转基因蚕

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摘要

The CRISPR/Cas9-mediated genome engineering has been shown to efficiently suppress infection by disrupting genes of the pathogen. We recently constructed transgenic lines expressing CRISPR/Cas9 and the double sgRNA target Bombyx mori nucleopolyhedrovirus (BmNPV) immediate early-1 (ie-1) gene in the silkworm, respectively, and obtained four transgenic hybrid lines by G1 generation hybridization: Cas9(-)/sgRNA(-), Cas9(+)/sgRNA(-), Cas9(-)/sgRNA(+), and Cas9(+)/sgRNA(+). We demonstrated that the Cas9(+)/sgRNA(+) transgenic lines effectively edited the target site of the BmNPV genome, and large fragment deletion was observed after BmNPV infection. Further antiviral analysis of the Cas9(+)/sgRNA(+) transgenic lines shows that the median lethal dose (LD50) is 1,000-fold higher than the normal lines after inoculation with occlusion bodies. The analysis of economic characters and off-target efficiency of Cas9(+)/sgRNA(+) transgenic hybrid line showed no significant difference compared with the normal lines. Our findings indicate that CRISPR/Cas9-mediated genome engineering more effectively targets the BmNPV genomes and could be utilized as an insect antiviral treatment.
机译:CRISPR / Cas9介导的基因组工程已显示可通过破坏病原体的基因有效抑制感染。我们最近在蚕中构建了分别表达CRISPR / Cas9和双sgRNA靶标家蚕核多角体病毒(BmNPV)立即早期1(ie-1)基因的转基因品系,并通过G1代杂交获得了四个转基因杂交品系:Cas9(- )/ sgRNA(-),Cas9(+)/ sgRNA(-),Cas9(-)/ sgRNA(+)和Cas9(+)/ sgRNA(+)。我们证明,Cas9(+)/ sgRNA(+)转基因株系有效地编辑了BmNPV基因组的目标位点,并在BmNPV感染后观察到大片段缺失。对Cas9(+)/ sgRNA(+)转基因品系的进一步抗病毒分析表明,接种了封堵体后,中位致死剂量(LD50)比正常品系高1,000倍。与常规品系相比,Cas9(+)/ sgRNA(+)转基因杂交品系的经济特性和脱靶效率分析显示无显着差异。我们的发现表明,CRISPR / Cas9介导的基因组工程更有效地靶向BmNPV基因组,可以用作昆虫抗病毒治疗。

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