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首页> 外文期刊>Transgenic Research >Resistance to crown gall disease in transgenic grapevine rootstocks containing truncated virE2 of Agrobacterium
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Resistance to crown gall disease in transgenic grapevine rootstocks containing truncated virE2 of Agrobacterium

机译:含有农杆菌virE2截短的转基因葡萄砧木对冠gall病的抗性

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摘要

A truncated form of the Ti-plasmid virE2 gene from Agrobacterium tumefaciens strains C58 and A6, and A. vitis strain CG450 was transferred and expressed in somatic embryos of grapevine rootstocks 110 Richter (Vitis rupestris × V. berlandieri), 3309 Couderc (V. rupestris × V. riparia) and Teleki 5C (V. berlandieri × V. riparia) via Agrobacterium-mediated transformation to confer resistance to crown gall disease. Transformation was confirmed in 98% of the 322 lines by enzyme-linked immunosorbent assay for the neomycin phosphotransferase II protein and 97% of 295 lines by polymerase chain reaction for the truncated virE2 transgene. Southern blot analysis revealed the insertion of truncated virE2 at one to three loci in a subset of seven transgenic 110 Richter lines. In vitro resistance screening assays based on inoculations of shoot internode sections showed reduced tumorigenicity and very small galls in 23 of 154 transgenic lines. Non-transformed controls had a 100% tumorigenicity rate with very large galls. Disease resistance assay at the whole plant level in the greenhouse revealed seven transgenic lines (3 lines of 110 Richter, 2 lines of 3309 Couderc and 2 lines of Teleki 5C) were resistant to A. tumefaciens strain C58 and A. vitis strains TM4 and CG450 with a substantially reduced percentage of inoculation sites showing gall as compared to controls. No association was found between the level of resistance to crown gall disease and the source Agrobacterium strain of virE2. Taken together, our data showed that resistance to crown gall disease can be achieved by expressing a truncated form of virE2 in grapevines.
机译:截短形式的根癌农杆菌菌株C58和A6以及葡萄曲霉CG450的Ti质粒virE2基因被转移并在葡萄砧木110 Richter(Vitis rupestris×V.berlandieri),3309 Couderc(V.通过农杆菌介导的转化来获得rupestris×V. riparia)和Teleki 5C(V. berlandieri×V. riparia),以赋予对冠gall病的抗性。通过酶联免疫吸附法对新霉素磷酸转移酶II蛋白的322个品系中有98%进行了转化,对于virE2转基因截短的聚合酶链反应已确认了295个品系中97%。 Southern印迹分析表明,在七个转基因110 Richter品系的子集中,在1-3个基因座处插入了截短的virE2。基于接种节间节的接种的体外抗性筛选试验显示,在154个转基因品系中的23个中,致瘤性降低,胆汁非常小。未转化的对照具有100%的致癌率,胆汁非常大。在温室中整个植物水平上的抗病性分析显示,有七个转基因品系(3个110里希特品系,2个3309 Couderc品系和2个Teleki 5C品系)对根癌农杆菌C58和葡萄菌TM4和CG450有抗性与对照组相比,接种部位的百分数显着降低。在对冠gall病的抗性水平与源农杆菌菌株virE2之间没有关联。综上所述,我们的数据表明,通过在葡萄树中表达截短形式的virE2,可以实现对冠crown病的抗性。

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