摘要
用提取的重组表达载体pET-E2转化BL21(DE3)感受态细胞,经IPTG绣导,再进行SDS-PAGE,可得到有一条约34 kDa的表达带,与理论推测的蛋白分子量一致,通过Western-blot鉴定,证明此带即为目的蛋白带。该产物有一个六聚组氨酸尾,主要以包涵体形式存在;计算机扫描分析考马斯亮兰染色后的蛋白胶显示:目的蛋白占整个菌体蛋白的36%以上,经Ni-柱纯化的E2蛋白纯度可达95%以上;以纯化的E2蛋白为抗原,用ELISA方法检测了20份抗HCV阴阳性血清,结果表明15份抗HCV阳性血清中检出5份E2抗体阳性血清,而5份抗HCV阴性血清中没有检测到E2抗体。
Rceomdinant plasmid pET-E2 was transformed into BL21 (DE3) competent cell, then induced the amplified culture with IPTG. There was a 34 kDa band in SDS-PAGE gel. The molecular weight of the expressed protein was comsistent to that of deduced E2 protein. Tested by western-blot, It showed that the product was HCV E2 protein. It contained a six-Histidine tag and aggregated into the inclusion body. Computer scan analysis showed the protein interested took the percentage more than 36 of the total bacterial proteins and the rate of purification was higher than 95% after purified by Ni-column. The activity of pruified E2 protein was tested by ELISA. The result showed that the 5/15 HCVpositive sera had anti-E2 antibody, and the other 5 negative HCV sera hadn't anti-E2 antibody.
出处
《中国病毒学》
CSCD
2003年第1期1-4,共4页
Virologica Sinica
关键词
HCV
E2
原核系统
基因表达
纯化
HCV E2
Prodaryotic system
Gene expression
Purification