摘要
用形成包涵体(OOC+)并能利用人工合成启动序列和多角体XIV启动子表达外源基因的转移载体质粒pSXIVVI+X3将多角体基因、乙型肝炎病毒表面抗原(HBSAg)基因和苜蓿丫纹夜蛾核型多角体病毒(AcNPV)的增强子hr5部分序列同时插入无包涵体的粉纹夜蛾核型多角体病毒TnNPV-SVI-G基因组中,得到两株高效表达HBsAg基因又形成包涵体的重组病毒TnNPV-shr35-OCC+和TnNPV-shr26-OCC+.对重组病毒的酶切鉴定、DNA斑点杂交和Southernblot分析证实,外源基因及其相应的启动子和增强子序列已正确插入病毒基因组中.插入顺序中,hr5增强子是插入HBsAg基因下游,多角体基因与HBsAg基因方向相反.125Ⅰ-固相放射免疫检测和Westernblot结果表明,HBsAg基因在昆虫离体细胞中得到高效表达并保留了抗原活性.TnNPV-shr26-OCC+和TnNPV-shr35-OCC+表达的HBsA吕蛋白与没有插入增强子序列的重组病毒TnNPV—HBs85-OCC+的比较,分别提高了40%和46%.
Two occluded (OCC+) recombinant Baculuviruses desingnated Tn NPV-shr 26-OCC+ and TnNPV-shr 35-OCC+ were sussesfully that contains the gene conding the hepapitis B virus suface antigen (HBsAg) gene of the dual control of synthetic and XIVpromoters and the AcNPV hr5 enhancer, that was used increasing HBsAg gene expression. The two correct recombinants were characterized by both DNA dot hybridization and southern blot analyses. Expression level of HBsAg gene in Spodoptera frugiperdacells infected with the two newty constructed recombinants was increased by 40% and 46% respectively, compared with that virus without additional the hr5 sequence. Western blot analysis indicated that the HBsAg proteins expressed by the baculovirus vector systems are antigenic properties indentical to HBsAg secreted by human cells and moleculur weights of about 18kD, 25kD and 35kD.
出处
《中山大学学报(自然科学版)》
CAS
CSCD
1996年第1期84-90,共7页
Acta Scientiarum Naturalium Universitatis Sunyatseni
基金
国家自然科学资金高技术探索性项目
高等学校博士点专项基金
