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pCB-zeolin-GFP表达载体的构建及瞬时表达
引用本文:张玉,白史且,李聪,李达旭,邓永昌.pCB-zeolin-GFP表达载体的构建及瞬时表达[J].中国农学通报,2012,28(3):233-239.
作者姓名:张玉  白史且  李聪  李达旭  邓永昌
作者单位:1. 四川省草原科学研究院,成都犀浦,611731
2. 中国农业科学院北京畜牧兽医研究所,北京,100094
基金项目:国家十二五科技支撑计划“南方优质饲草高效生产加工利用关键技术研究与集成示范”(2011BAD17B03); 四川省十二五牧草育种攻关和国家牧草产业技术体系“阿坝综合实验站”(CARS-345)
摘    要:为利用荧光蛋白基因GFP检测外源基因在转基因植株中的表达和定位,构建含有GFP基因的植物表达载体pCB-zeolin-GFP。在目的基因的开放阅读框(ORF)两端设计引物,并引入酶切位点和保护碱基,用PCR方法从pDHA扩增得到zeolin基因的全长,克隆到中间载体pMD18-T,分别用NcoⅠ和BglⅡ2种限制性内切酶酶切重组质粒和经过改良的pCAMBIAI1302植物表达载体,经回收、连接、转化、鉴定后,利用基因枪转化法将重组载体转入洋葱表皮细胞,通过共聚焦显微镜检测绿色荧光蛋白在洋葱表皮细胞中的瞬时表达。构建了zeolin基因与绿色荧光蛋白(GFP)融合的植物表达载体pCB-zeolin-GFP,并在洋葱中得到了表达。构建的融合植物表达载体pCB-zeolin-GFP正确,该载体的成功构建为今后进行基因转移、基因功能研究及培育新品种奠定了基础。

关 键 词:商品林  商品林  投资  风险评价  
收稿时间:2011/5/12 0:00:00
修稿时间:2011/11/7 0:00:00

Construction of Plant Expression Vector pCAMBIAl302-zeolin-GFP and the Transient Expression
Zhang Yu , Bai Shiqie , Li Cong , Li Daxu , Deng Yongchang.Construction of Plant Expression Vector pCAMBIAl302-zeolin-GFP and the Transient Expression[J].Chinese Agricultural Science Bulletin,2012,28(3):233-239.
Authors:Zhang Yu  Bai Shiqie  Li Cong  Li Daxu  Deng Yongchang
Institution:1 Sichuan Grassland Science Academy , Xipu Chengdu 611731; 2 Institute of Animal Science, Chinese Academy of Agricultural Science , Beijing 100094)
Abstract:To utilize fluorescin gene GFP to detect the express and localization of exogenous gene, plant expression vector pCAMBIAl302-zeolin with a green fluorescent protein gene would be constructed. The total length sequence of zeolin gene in pDHA plasmid was amplified by PCR. The fragment was cloned into pMD18-T middle vector, and a new recombined vector named pMD18-T-zeolin was obtained. A new plant expression vector named pCB-GFP-zeolin was constructed after cutting two vector pMD18-zeolin and pCAMBIAI1302 with restriction enzymes, subsequently reclamation, ligation, transformation and identification. Then the recombined plant expression vector pCAMBIAl302-zeolin with a green fluorescent protein gene was transformed into epidemic cells of onion by gene gun method and was detected by confocal microscopy. The recombined plant expression vector pCAMBIAl302-zeolin with a green fluorescent protein gene had been constructed and the fusion gene was transient expressed. It was suggested that the recombined plant expression vector pCAMBIAl302-zeolin with a green fluorescent protein gene was successful. Construction of the plant expression vector might play an important role in genetic transformation, the gene functional identification and breeding of new varieties.
Keywords:green fluorescent protein (GFP)  zeolin gene  vector construction  transient expression
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