作物杂志,2016, 第3期: 3744 doi: 10.16035/j.issn.1001-7283.2016.03.008
杨浩,朱延明
Yang Hao,Zhu Yanming
摘要:
基于实验室前期野生大豆G07256碱胁迫转录组数据,结合生物信息学方法筛选得到响应碱胁迫的cation/H +逆向转运蛋白基因GsCHX19,克隆了GsCHX19基因全长CDS编码序列并将其构建到pCAMBIA330035Su植物超量表达载体中。以肇东紫花苜蓿为受体材料,通过农杆菌介导法将重组的植物表达载体转化其子叶节,用含0.5mg/L草铵膦的筛选培养基进行筛选,获得20株抗性植株。采用PCR方法检测抗性植株中bar基因的表达,获得16株PCR阳性植株。对获得的PCR阳性植株进行RT-PCR及real-time PCR检测,鉴定共获得11株RT- PCR阳性植株,且证明GsCHX19基因在各转基因植株中均有不同程度的表达。结果表明,GsCHX19基因成功转化苜蓿,并且得到表达,该转基因植株将为耐盐碱转基因苜蓿新品种的培育提供重要的试验材料。
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