流感病毒在Vero或MDCK细胞和胚鸡蛋中培养的生长和免疫原性

E A Govorkova, S Kodihalli, I V Alymova, B Fanget, R G Webster
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引用次数: 0

摘要

采用Vero细胞、MDCK细胞和胚化鸡蛋对乙型流感灭活疫苗诱导的流感病毒生长特性和免疫原性进行了评价。两种细胞系产生相当数量的总病毒和血凝素(HA)蛋白。序列分析表明,Vero-和mdck生长的病毒的HA具有遗传同一性,并维持来自人类的病毒的抗原特征。鸡蛋培养的流感B/Memphis/1/93变体与细胞培养的变体在氨基酸位置198 (Pro-Thr)上不同,并且失去了一个糖基化位点。神经氨酸酶(NA)活性水平在蛋培养病毒中最高,而以胎儿蛋白为底物的MDCK-和Vero细胞培养病毒的NA活性分别降低70%和90%。虽然每一种疫苗都能诱导高水平且相当水平的血清抗体,但哺乳动物细胞源性疫苗诱导的抗体更具交叉反应性,而蛋源性疫苗诱导的抗体对同源抗原更具特异性。ELISPOT分析表明,哺乳动物细胞培养疫苗诱导了针对细胞和鸡蛋培养抗原的高频率的IgG产生细胞,而鸡蛋培养疫苗诱导了高频率的IgG和igm产生细胞与同源抗原反应,低水平的IgG产生细胞与细胞培养的病毒抗原反应。综上所述,我们的结果表明,哺乳动物细胞是生产流感病毒疫苗的可行选择。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Growth and immunogenicity of influenza viruses cultivated in Vero or MDCK cells and in embryonated chicken eggs.

Vero cells, MDCK cells and embryonated chicken eggs (eggs) were used to evaluate influenza virus growth characteristics and immunogenicity induced by inactivated influenza B vaccines. Both cell lines produced comparable quantities of total viral and haemagglutinin (HA) proteins. Sequence analysis indicated genetic identity of the HA of Vero- and MDCK-grown virus counterparts with maintenance of antigenic characteristics of viruses derived from humans. The egg-grown influenza B/Memphis/1/93 variant differed from cell-grown counterparts at amino acid position 198 (Pro-Thr) and lost a glycosylation site. The level of neuraminidase (NA) activity was the highest in egg-grown virus, while MDCK- and Vero cell-grown viruses possessed 70% and 90% less NA activity respectively when fetuin was used as a substrate. Although each of the vaccines induced high and comparable levels of serum antibodies, mammalian cell-derived vaccines induced antibodies that were more cross reactive, and those antibodies induced by egg-derived vaccine were more specific to the homologous antigen. ELISPOT analysis indicated that the mammalian cell-grown vaccines induced high frequencies of IgG-producing cells directed against both cell- and egg-grown antigens, while egg-grown vaccine induced high frequencies of IgG and IgM-producing cells reacting with homologous antigen and low levels of IgG-producing cells reactive with cell-grown virus antigen. Taken together, our results suggest that mammalian cells are a viable option for the production of influenza virus vaccines.

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