[Objective] The research aimed to construct the fusion protein expression vector of α-galactosidase-EGFP (enhanced green fluorescent protein) in cucumber controlled by CaMV35S promoter.[Method] CaMV35S promoter seq...
详细信息
[Objective] The research aimed to construct the fusion protein expression vector of α-galactosidase-EGFP (enhanced green fluorescent protein) in cucumber controlled by CaMV35S promoter.[Method] CaMV35S promoter sequence and the coding region of EGFP were amplified by polymerase chain reactions (PCR) with vector pCambia 1303 as the *** reverse transcript PCR technology,with total RNAs of cucumber as template,the coding region of acid α-galactosidase Ⅰ in cucumber was *** above three fragments were inserted into the multiple cloning sites of expression vector pCambia *** fusion expression vector of α-galactosidase-EGFP located at the C-terminal of the target genes was constructed.[Result] After enzyme digestion and sequencing,the fusion expression of α-galactosidase-EGFP in cucumber was constructed successfully.[Conclusion] The research laid the experimental basis for further study on the subcellular localization of α-galactosidase in cucumber.
暂无评论