重叠延伸PCR法合成EV71 VP1-LTB融合基因及其原核表达

目的用重叠延伸PCR（overlap extension PCR）法获得人肠道病毒71型vp1与大肠埃希菌不耐热肠毒素B亚单位（ltb）的融合基因,构建EV71 VP1-LTB融合表达质粒并在原核系统表达。方法设计14对引物通过重叠延伸PCR技术合成vp1基因,以ETEC（44815）质粒DNA为模板,PCR扩增ltb基因,将vp1基因与ltb基因连接并测序,连接产物插入原核表达质粒pBEX,构建重组质粒pBEX-VP1-LTB,转化E.coliB1221（DE3）进行表达,SDS-PAGE及W estern blotting分析其表达。电转法将重组质粒转入双歧杆菌。结果合成的vp1基因全长891 bp,测序结果与预期相符,重组表达质粒pBEX-VP1-LTB经PCR及双酶切鉴定,表明构建正确;目的蛋白在E.coliBL21（DE3）中获得了表达,Western bloting分析结果表明该蛋白具有与EV71 VP1抗体的反应原性;电转法成功将重组质粒转入双歧杆菌。结论应用重叠延伸PCR技术成功构建了EV71 VP1-LTB融合表达质粒,并在E.coliBL21（DE3）中获得有生物学功能的VP1表达产物,重组质粒双歧杆菌转化及VP1-LTB融合蛋白的表达研究,为研制EV71分子内佐剂疫苗打下了基础。

Synthesis of human enterovirus 71 VP1 and E.coli Heat-Labile Enterotoxin Subunit B Fusion gene by Overlapping PCR and its prokaryotic expression

Objective To achieve synthesis of human enterovirus 71 vp1 gene(EV71 vp1) and construction of E.coli Heat-Labile Enterotoxin Subunit B(ltb) fusion gene by Overlapping PCR,and construct its prokaryotic expression vector and test the expression product in E.coli.Method Vp1 gene was synthesized with 14 pairs of primers and the ltb gene fragment of ETEC(44815) plasmid DNA was amplified by PCR.The two fragments were linked by Overlapping PCR;the product was identified by sequencing analysis and inserted into pro...