4.5 Article Proceedings Paper

Enhancing enterovirus A71 vaccine production yield by microcarrier profusion bioreactor culture

期刊

VACCINE
卷 36, 期 22, 页码 3134-3139

出版社

ELSEVIER SCI LTD
DOI: 10.1016/j.vaccine.2017.02.042

关键词

Enterovirus A71; Inactivated whole virion vaccine; Serum-free bioreactor; Microcarrier culture; Perfusion technology

资金

  1. Ministry of Health and Welfare, Taiwan
  2. Ministry of Science and Technology, Taiwan [NSC 99A1-VCSP01-014]
  3. Taiwan CDC, Taiwan
  4. National Health Research Institutes, Taiwan [02A1-IVPP12-014]

向作者/读者索取更多资源

Hand, foot and mouth diseases (HFMD) are mainly caused by Enterovirus A71 (EV-A71) infections. Clinical trials in Asia conducted with formalin-inactivated EV-A71 vaccine candidates produced from serum-free Vero cell culture using either roller bottle or cell factory technology, are found to be safe and highly efficacious. To increase vaccine yields and reduce the production costs, the bioprocess improvement for EV-A71 vaccine manufacturing is currently being investigated. The parameters that could affect and enhance the production yields of EV-A71 virus growth in the microcarrier bioreactor were investigated. The medium replacement culture strategy included a multi-harvested semi-batch process and perfusion technology and was found to increase the production yields more than 7-14 folds. Based on the western blot and cryo-EM analyses of the EV-A71 virus particles produced from either the multi-harvested semi-batch (MHSBC) or perfusion cultures were found to be similar to those virus particles obtained from the single batch culture. Mouse immunogenicity studies indicate that the EV-A71 vaccine candidates produced from the perfusion culture have similar potency to those obtained from single batch bioprocess. The physical structures of the EV-A71 particles revealed by the cryo-EM analysis were found to be spherical capsid particles. These results provide feasible technical bioprocesses for increasing virus yields and the scale up of EV-A71 vaccine manufacturing using the bioreactor cell culture methods. (C) 2017 Elsevier Ltd. All rights reserved.

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