Construction of high-efficiency transformation vector with multiple insect-resistant genes and expression in tobacco

被引:0
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作者
Shengliang Yuan
Yan Dong
Na Zhang
Yachao Ren
Minsheng Yang
Baojia Gao
机构
[1] Agricultural University of Hebei,Institute of Forest Biotechnology, Forestry College
[2] Hebei Key Laboratory for Tree Genetic Resources and Forest Protection,undefined
[3] Biological Control Center of Plant Diseases and Plant Pests of Hebei Province/National Engineering Research Center for Agriculture in Northern Mountainous Areas,undefined
来源
Acta Physiologiae Plantarum | 2017年 / 39卷
关键词
Co-expression of multiple genes; Plant transgenic vector; Bt proteins;
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学科分类号
摘要
A high-efficiency plant transgenic vector expressing multiple genes has been modified from expression vector pCAMBIA1302. Briefly, multiple cloning sites of a cloning vector pUCm-T were constructed into plant transgenic vector pCAMBIA1302 backbone using Bsp120 I and Spe I restriction digest site. Two Bt genes, cry1Ac and cry3A, were then constructed into the modified transgenic vector in different orders as p1870-35S::cry1Ac-Coy::cry3A and p1870-Coy::cry3A-35S::cry1Ac, respectively. Transgenic tobacco plants were generated using Agrobacterium-mediated transformation method. Polymerase chain reaction (PCR) results showed that both the exogenous genes were integrated into the genome of tobacco. Fluorescence qRT-PCR detected both transgenes and further ELISA assay validated the expressed Bt proteins. Transgenic lines showed enhanced resistance to larvae of Helicoverpa armigera Hubner in the further feeding assays. In conclusion, our modified transgenic vector was suitable for multiple gene expression and would greatly facilitate our future research.
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