南方农业学报Issue(3):345-351,7.DOI:10.3969/j.issn.2095-1191.2014.3.345
蝴蝶兰MADS-Box基因克隆及植物表达载体的构建
Cloning and vector construction of MADS-Box gene in Phalaenopsishybrid
摘要
Abstract
[Objective]Cloning as well as sense and antisense plant expression vector of MADS-Box gene in Phalaenopsis hybrid were conducted to provide references for researching its functions. [Method]The MADS-Box gene was cloned from scape of Phalaenopsis hybrid cv. Jiuhbao Red Rose using RT-PCR and RACE. Sense and antisense plant expression vector were also constructed. [Result]The cloned MADS-Box gene from scape was named DtpsMADS1(GenBank accession No. JQ065097). The full length cDNA of DtpsMADS1 was 960 bp, containing 37 bp of a 5'-untranslated region (5'-UTR),185 bp of 3'-UTR,and 738 bp of an opening reading frame (ORF). The gene encoded 245 predicted amino acids. The bioinfor-mation analysis results showed that the gene encoding protein was a basic hydrophilic protein and contained 62.45%ofα-heli-cal domains, 8.16%of extended strand and 29.39%of random coil. Sequence comparison and phylogenetic analysis revealed that DtpsMADS1 shared 99.0%homology with ORAP13 of Phalaenopsis amabilis, 83.0%and 82.0%homology with Dendrobi-um nobile and Cymbidium orchid, respectively. DtpsMADS1 belonged to A-class subfamily of MADS family. Sense and anti-sense plant expression vector pBI121-DtpsMADS1-S and pBI121-DtpsMADS1-A were constructed when DtpsMADS1 was connected to plant expression vector pBI121. [Conclusion]The DtpsMADS1 gene of Phalaenopsis hybrid was cloned suc-cessfully. The sense and antisense plant expression vector were constructed successfully and could be used for DtpsMADS1 genetic function identification and genetic improvement of Phalaenopsis hybrid.关键词
蝴蝶兰/MADS-Box基因/克隆表达/载体构建Key words
Phalaenopsis hybrid/gene cloning/MADS-Box/construction of vector分类
农业科技引用本文复制引用
袁秀云,蒋素华,王默霏,崔波..蝴蝶兰MADS-Box基因克隆及植物表达载体的构建[J].南方农业学报,2014,(3):345-351,7.基金项目
河南省科技攻关项目(092102110128);郑州市科技攻关项目(112PPTGY250-3);郑州师范学院科研项目 ()
