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Rapid Construction of Complex Plant RNA Virus Infectious cDNA Clones for Agroinfection Using a Yeast- E. coli-Agrobacterium Shuttle Vector

机译:使用酵母-大肠杆菌-土壤杆菌穿梭载体快速构建用于农杆菌感染的复杂植物RNA病毒感染性cDNA克隆

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The availability of infectious full-length clone is indispensable for reverse genetics studies of virus biology, pathology and construction of viral vectors. However, for RNA viruses with large genome sizes or those exhibiting inherent cloning difficulties, procedure to generate biologically active complementary DNA (cDNA) clones can be time-consuming or technically challenging. Here we have constructed a yeast- Escherichia coli - Agrobacterium shuttle vector that enables highly efficient homologous recombination in yeast for assembly of Agrobacterium compatible plant virus clones. Using this vector, we show that infectious cDNA clones of a plant negative-stranded RNA virus, sonchus yellow net rhabdovirus, can be rapidly assembled. In addition, one-step assembly of infectious clones of potato virus Y in yeast, either with or without intron, was readily achieved from as many as eight overlapping DNA fragments. More importantly, the recovered yeast plasmids can be transformed directly into Agrobacterium for inoculation, thereby obviating the E. coli cloning steps and associated toxicity issues. This method is rapid, highly efficient and cost-effective and should be readily applicable to a broad range of plant viruses.
机译:传染性全长克隆的可用性对于病毒生物学,病理学和病毒载体构建的反向遗传学研究必不可少。但是,对于具有大基因组大小的RNA病毒或表现出固有克隆困难的RNA病毒,生成具有生物活性的互补DNA(cDNA)克隆的过程可能很耗时或在技术上具有挑战性。在这里,我们构建了一种酵母-大肠杆菌-农杆菌穿梭载体,该载体能够在酵母中进行高效同源重组,以组装与农杆菌相容的植物病毒克隆。使用此载体,我们显示了植物负链RNA病毒,son黄色网状弹状病毒的感染性cDNA克隆可以快速组装。另外,从多达八个重叠的DNA片段中容易地实现了马铃薯病毒Y在酵母中的感染性克隆的一步组装,无论有无内含子。更重要的是,可以将回收的酵母质粒直接转化到土壤杆菌中进行接种,从而避免了大肠杆菌的克隆步骤和相关的毒性问题。该方法是快速,高效和具有成本效益的,并且应易于适用于多种植物病毒。

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