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作 者:孙金霞[1,2] 刘艳环[2] 李海涛[2] 李庆超[2] 张广雷[1] 苗利光[2]
机构地区:[1]江苏科技大学,江苏镇江212018 [2]中国农业科学院特产研究所,吉林吉林132109
出 处:《特产研究》2010年第2期16-18,39,共4页Special Wild Economic Animal and Plant Research
基 金:中国农业科学院特产研究所基金项目
摘 要:根据GeneBank中提供的牛乳铁蛋白基因序列,设计并合成了重组LfcinB/LfampinB基因,并通过PGEM-Teasy载体扩增。酶切回收的LfcinB/LfampinB片段与中间载体pP6连接。pP6上的启动子、信号肽和调控序列与LfcinB/LfampinB共同切下,获得具有上游调控元件的PLfc/Lfa基因片段。将PLfc/Lfa与pME290表达载体连接,并转化绿脓杆菌。结果表明,本试验成功构建了重组pPLfc/Lfa表达载体。the Bovine lactoferrin gene deposited in GeneBank,LfcinB/LfampinB recombinant gene was designed and synthesized,and then amplified by PGEM-T easy plasmid.The purified LfcinB/LfampinB gene by restriction enzyme was linked to pP6 plasmid.Together with LfcinB/LfampinB gene,the promoter,signal peptide and regulator gene which were in pP6 plasmid were digested by restriction enzyme,PLfc/Lfa fragment which had upstream regulatory element was obtained.PLfc/Lfa was linked to pME290 expression plasmid and transformed into competent cells of.The results showed that recombinant expression plasmid pPLfc/Lfa was obtained.
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