Literature DB >> 10494958

Growth and immunogenicity of influenza viruses cultivated in Vero or MDCK cells and in embryonated chicken eggs.

E A Govorkova1, S Kodihalli, I V Alymova, B Fanget, R G Webster.   

Abstract

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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Year:  1999        PMID: 10494958

Source DB:  PubMed          Journal:  Dev Biol Stand        ISSN: 0301-5149


  25 in total

1.  Efficacy studies of influenza vaccines: effect of end points used and characteristics of vaccine failures.

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Review 2.  Cell culture-based influenza vaccines: A necessary and indispensable investment for the future.

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3.  Characterization of a porcine intestinal epithelial cell line for influenza virus production.

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4.  Measuring Influenza Neutralizing Antibody Responses to A(H3N2) Viruses in Human Sera by Microneutralization Assays Using MDCK-SIAT1 Cells.

Authors:  F Liaini Gross; Yaohui Bai; Stacie Jefferson; Crystal Holiday; Min Z Levine
Journal:  J Vis Exp       Date:  2017-11-22       Impact factor: 1.355

5.  Caveolin-1 influences human influenza A virus (H1N1) multiplication in cell culture.

Authors:  Lijing Sun; Gun-Viol Hemgård; Sony A Susanto; Manfred Wirth
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Review 6.  Designing vaccines for pandemic influenza.

Authors:  Taisuke Horimoto; Yoshihiro Kawaoka
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7.  Growth determinants for H5N1 influenza vaccine seed viruses in MDCK cells.

Authors:  Shin Murakami; Taisuke Horimoto; Le Quynh Mai; Chairul A Nidom; Hualan Chen; Yukiko Muramoto; Shinya Yamada; Ayaka Iwasa; Kiyoko Iwatsuki-Horimoto; Masayuki Shimojima; Akira Iwata; Yoshihiro Kawaoka
Journal:  J Virol       Date:  2008-09-03       Impact factor: 5.103

8.  Conversion of MDCK cell line to suspension culture by transfecting with human siat7e gene and its application for influenza virus production.

Authors:  Chia Chu; Vladimir Lugovtsev; Hana Golding; Michael Betenbaugh; Joseph Shiloach
Journal:  Proc Natl Acad Sci U S A       Date:  2009-08-17       Impact factor: 11.205

9.  MDCK-SIAT1 cells show improved isolation rates for recent human influenza viruses compared to conventional MDCK cells.

Authors:  Ding Yuan Oh; Ian G Barr; Jenny A Mosse; Karen L Laurie
Journal:  J Clin Microbiol       Date:  2008-05-14       Impact factor: 5.948

10.  MVA-based H5N1 vaccine affords cross-clade protection in mice against influenza A/H5N1 viruses at low doses and after single immunization.

Authors:  Joost H C M Kreijtz; Yasemin Suezer; Gerrie de Mutsert; Geert van Amerongen; Astrid Schwantes; Judith M A van den Brand; Ron A M Fouchier; Johannes Löwer; Albert D M E Osterhaus; Gerd Sutter; Guus F Rimmelzwaan
Journal:  PLoS One       Date:  2009-11-12       Impact factor: 3.240

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