Cloning of CBF3 Gene from Arabidopsis thaliana and Construction of Plant Expression Vector 被引量：3

拟南芥CBF3基因克隆和植物表达载体的构建(英文)

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摘要 [Objective] The aim was to clone CBF3 gene from Arabidopsis thaliana and construct plant expression vector pCAMBIA1301-Rd29A-CBF3.[Method] CBF3 gene and stress-inducible promoter Rd29A were amplified from the genomic DNA of A.thaliana for the construction of plant expression vector.[Result] Sequencing results showed that the cloned CBF3 gene had 750 bp,and showed 100% identity with the sequence published on GenBank.The promoter Rd29A had 1 425 bp,and showed 100% identity with the sequence published on GenBank.[Conclusion] Based on the binary vector pCAMBIA1301,the plant expression vector pCAMBIA1301-Rd29A-CBF3 was constructed successfully,which could materially improve the salt resistance,drought-tolerance,cold resistance of plants. [目的]克隆拟南芥CBF3基因并构建植物表达载体pCAMBIA1301-Rd29A-CBF3。[方法]从模式植物拟南芥中克隆分离出转录因子CBF3与逆境诱导型启动子Rd29A的DNA序列,构建植物表达载体。[结果]克隆得到的CBF3与GenBank数据库所公布序列比对发现,同源性达到100%,全长为750bp;克隆克隆得到的Rd29A与GenBank数据库公布序列比对发现,同源性达到100%,全长为1425bp。[结论]以双元载体pCAMBIA1301为基础,植物表达载体pCAMBIA1301-Rd29A-CBF3被成功构建,对提高植物耐盐、耐旱和耐寒性有很大帮助。

作者张春平束良佐张启军吕川根蔡小宁

机构地区安徽农业大学南京晓庄学院江苏省农业科学院

出处《Agricultural Science & Technology》 CAS 2011年第5期670-673,共4页 农业科学与技术（英文版）

基金 Supported by Cultivation for New Varieties of Genetically Modified Organisms Technology Projects(2008ZX08001-004) Key Projects of Nanjing Xiaozhuang University(2007NXY01) Natural ScienceFoundation for Jiangsu Province Universities(08KJD180011)~~

关键词 CBF3 RD29A PROMOTER CLONE Plant expression vector CBF3 Rd29A 启动子克隆植物表达载体

分类号 Q943.2 [生物学—植物学]

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