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作 者:姜琼[1]
机构地区:[1]宜春学院化学与生物工程学院,江西宜春336000
出 处:《宜春学院学报》2011年第4期116-117,189,共3页Journal of Yichun University
基 金:江西省天然药物活性成分研究重点实验室开放基金项目
摘 要:目的:构建唾液抗菌肽P113基因多拷贝串联重组体,并将其克隆到表达载体pET-28a。方法:根据大肠杆菌偏爱的密码子设计并合成人唾液抗菌肽P113基因,采用PCR技术构建P113基因的自融合多拷贝串联重组体polyP113,BamHⅠ和HindⅢ双酶切表达载体pET-28a和polyP113基因,将两者连接后转化大肠杆菌DH5α,氨苄青霉素筛选阳性菌落,PCR、酶切、测序鉴定重组质粒。结果:所构建的含有十拷贝P113基因的重组体正确克隆到表达载体pET-28a上,无突变。结论:成功构建含十拷贝唾液抗菌肽P113基因表达框的大肠杆菌表达载体。Objective: To construct the tendem-repeated multiple copy recombinant for gene Salivary Antimicrobial Peptide P113 and then clone the gene to expression vector pET-28a.Methods: According to the optium codens of E.coli,we designed and synthesized the P113 gene PCR technique was used to construct the tendem-repeated multiple copy recombinant polP113,pET-28a and polyP113 were both digested by BamHⅠand HindⅢ,the digested pET-28a and polyP113 were linked and transformed to Ecoli DH5α,and the positive colonies were screened by ampicillin,and identified by PCR,digestion and sequencing.Result: The recombinant made up of ten copy P113 gene were correctly inserted into expression vector pET-28a without mutation.Conclusion: The expression vector of E.coli containing ten copies of Salivary Antimicrobial Peptide P113 was constructed successfully.
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