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ThIPK2基因植物表达载体的构建

Construction of Plant Expression Vector Harboring ThIPK2
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摘要 为培育高度抗逆和无选择标记的转基因小麦,本研究从NCBI数据库中搜索到ThIPK2基因序列,依据该基因编码的氨基酸序列,参照小麦偏爱的密码子对该基因进行密码子优化,并将重复的和不必要的酶切位点去掉后进行人工合成。将改造后的ThIPK2基因插入到强启动子Ubiquitin和终止子AtSac66之间,然后将其插入到含有玉米Ac/Ds转座子背景骨架的植物表达载体中,获得了具有删除选择标记功能的、由玉米Ubiquitin启动子驱动ThIPK2基因的植物表达载体。经过限制性内切酶分析鉴定,该植物表达载体构建成功。 In order to get stress tolerant transgenic wheat plants without selective markers, the ThlPK2 gene sequence was got from the NCBI database, the gene codons were optimized based on wheat preference co- dons, the repeated and unnecessary restriction sites were removed, and the gene was synthesized. The synthe- sized ThlPK2 gene was constructed into vector with Ubiquitin promoter and AtSac66 terminator. The whole cassete was then ligated into a plant expression vector harboring Ac/Ds transposon, which could be further used for wheat transformation. Identified by restriction endonuclease, the expression vector was successfully constructed.
作者 张淑娟 宋国琦 高洁 王姣 李玉莲 黄承彦 樊庆琦 隋新霞 楚秀生 李根英
机构地区 山东省农业科学院作物研究所/农业部黄淮海北部小麦生物学与遗传育种重点实验室/小麦玉米国家工程实验室
出处 《山东农业科学》 2013年第5期18-23,共6页 Shandong Agricultural Sciences
基金 国家转基因重大专项(2013ZX08002004) 山东省农业良种工程项目 山东省产业技术体系项目资助
关键词 ThIPK2基因 密码子优化 表达载体构建 ThlPK2 gene Codon optimization Expression vector construction
分类号 Q786 [生物学—分子生物学]
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参考文献16

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