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作 者:董云洲[1]
机构地区:[1]中国农业科学院生物技术研究中心,北京100081
出 处:《Acta Botanica Sinica》1999年第2期146-149,共4页Acta Botanica Sinica(植物学报:英文版)
基 金:国家自然科学基金;农业部"95"重点基金
摘 要:构建了肌醇甲基转移酶(Imtl)基因的植物表达载体pDH5.通过农杆菌(Agrobacterium)介导,获得了转基因烟草(NicotianatabacumLev.SR1)植株,在附加1.2%-1.5%NaCl的生根培养基MSr(MSO+3g/L蔗糖+7g/L葡萄糖)上可生根。生化分析表明,不具有芒柄醇(D-ononitol)合成途径的烟草鲜叶片积累了100-654nmol/g的芒柄醇,新产生了一个代谢分支。Western杂交分析证明Imtl基因在烟草中的表达,从而为植物耐盐的基因工程育种提供了一条新途径。The plant expression vector with Imt1 (inositol O-methyltransferase) gene, pDH5, was constructed. The Imt1 gene was introduced to tobacco (Nicotiana tabocum cv. SR1) via Agrobacterium-mediatedtransformation. Thirty kanamycin-resistant shoots in MSS (MSO+1mg/L 6-BA+30g/L sucrose) selectivemedium was transferred to MSr (MSO+3g/L. sucrose+7g/L glucose) medium supplemented with 1. 2%~ 1. 5% NaCl for rooting. Eight plailtlets rooted among the thirty shoots. PCR and Southem blot assay indicatedthat foe Imt1 gene was integrated into tobaeeo genome in six plantlets. HPLC analysis showed that the produetof Imt1 gene, D-ononitol accumulated in tobacco fresh leaf cells in a scope of 100-654 nmol/g FW. Westernblot demonstrated the expression of Imt1 gene in tobacco cells.
分 类 号:S572.035.4[农业科学—烟草工业]
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