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在杂交病毒颗粒表面表达口蹄疫衣壳蛋白表位单体和二聚体形式的改良活传染性牛鼻气管炎病毒疫苗

Modified-live infectious bovine rhinotracheitis virus vaccine expressing monomer and dimer forms of foot-and-mouth disease capsid protein epitopes on surface of hybrid virus particles.

作者信息

Kit S, Kit M, DiMarchi R D, Little S P, Gale C

机构信息

Division of Biochemical Virology, Baylor College of Medicine, Houston, Texas.

出版信息

Arch Virol. 1991;120(1-2):1-17. doi: 10.1007/BF01310945.

DOI:10.1007/BF01310945
PMID:1718244
Abstract

Modified-live, attenuated infectious bovine rhinotracheitis (IBR) hybrid virus vaccines have been constructed by inserting in the major IBRV glycoprotein gIII gene chemically synthesized deoxyribonucleotide sequences encoding the bovine growth hormone signal sequence and monomeric or dimeric forms of the foot and mouth disease virus (FMDV) VP 1 epitope sequences. The foreign DNA sequences were inserted at the N-terminal end of the IBRV gIII coding sequence and were driven by the IBRV gIII promoter. The sequences encoding the first 38 and the first 21 amino acids of the IBRV gIII were deleted from the hybrid viruses containing inserts of the monomeric and dimeric FMDV epitope sequences, respectively, to avoid redundant signal sequences. Plaque immunoassay experiments with guinea pig and bovine anti-FMDV peptide antisera, and with anti-IBRV gIII monoclonal antibodies demonstrated that IBRV-FMDV fusion proteins were expressed in virus-infected MDBK cells. Immunoelectron microscopy analyses demonstrated that the IBRV-FMDV fusion proteins were expressed as repeated structures on the surface of virus particles. Experiments showed that the recombinant IBRV-FMDV viruses protected cattle from IBRV (Cooper) challenge and induced anti-FMDV peptide antibodies, thereby demonstrating that the FMDV epitopes were expressed in vivo.

摘要

通过在传染性牛鼻气管炎病毒(IBR)主要糖蛋白gIII基因中插入化学合成的脱氧核糖核苷酸序列来构建减毒活IBR杂交病毒疫苗,这些序列编码牛生长激素信号序列以及口蹄疫病毒(FMDV)VP1表位序列的单体或二聚体形式。外源DNA序列插入到IBR病毒gIII编码序列的N末端,并由IBR病毒gIII启动子驱动。在分别含有单体和二聚体FMDV表位序列插入片段的杂交病毒中,分别删除了编码IBR病毒gIII前38个和前21个氨基酸的序列,以避免信号序列冗余。用豚鼠和牛抗FMDV肽抗血清以及抗IBR病毒gIII单克隆抗体进行的空斑免疫测定实验表明,IBR病毒-FMDV融合蛋白在病毒感染的MDBK细胞中表达。免疫电子显微镜分析表明,IBR病毒-FMDV融合蛋白在病毒颗粒表面以重复结构形式表达。实验表明,重组IBR病毒-FMDV病毒可保护牛免受IBR病毒(库珀株)攻击,并诱导产生抗FMDV肽抗体,从而证明FMDV表位在体内表达。

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