机构地区: 山东农业大学动物科技学院
出 处: 《西北农林科技大学学报(自然科学版)》 2007年第1期19-23,共5页
摘 要: 用PCR法扩增了牛疱疹病毒Ⅰ型B artha N u/67株gB基因,将其插入原核表达载体pBAD/TOPO中构建重组质粒pBAD-gB。将pBAD-gB质粒转化大肠杆菌TOP 10后进行了诱导表达,对表达产物进行了纯化和抗原性检测,并通过改变诱导剂L-A rab inose的浓度和诱导时间对诱导表达条件进行了优化。结果表明,重组质粒pBAD-gB构建成功,gB蛋白获得了高效表达,并以包涵体形式存在,纯化后gB蛋白的纯度达90%以上,gB蛋白抗原性良好,最佳诱导表达条件:L-A rab inose终浓度为0.2 g/L,诱导时间为5 h。 The gB gene fragment of bovine herpesvirus-1 Bartha Nu/67 strain was amplified by PCR and inserted into prokaryotie expressing vector pBAD/TOPO. The recombined plasmids were then trans- formed into E. coli TOP10 for expression. The expression was optimized with proper inducing conditions of 0. 2 g/L L-Arabinose and 5 hours induction. The SDS-PAGE assay showed that the recombined plasmids could be expressed in inclusion body at a high level when induced with L-Arabinose. The purity of fusion proteins which was purified by magnehis protein purification system was more than 90%. Western-blot showed the good antigenicity of the target proteins.