Separation and purification of highly infectious enterovirus A71 particles using a strong anion-exchange column

Sheng-Chieh Lien; Chia-Chun Lu; Yu-Sheng Shen; Ya-Ting Yang; Shang-Rung Wu; Chih-Yeu Fang; Yen-Hung Chow; Ching-Len Liao; Jen-Ron Chiang; Chia-Chyi Liu

doi:10.1016/j.chroma.2022.463427

Separation and purification of highly infectious enterovirus A71 particles using a strong anion-exchange column

J Chromatogr A. 2022 Sep 13:1680:463427. doi: 10.1016/j.chroma.2022.463427. Epub 2022 Aug 18.

Authors

Affiliations

¹ National Institute of Infectious Diseases and Vaccinology, National Health Research Institutes, Zhunan Town, Miaoli County, Taiwan.
² Institute of Oral Medicine, National Cheng Kung University College of Medicine and Hospital, Tainan, Taiwan.
³ National Institute of Infectious Diseases and Vaccinology, National Health Research Institutes, Zhunan Town, Miaoli County, Taiwan; Graduate Institute of Immunology, China Medical University, Taichung, Taiwan.
⁴ National Institute of Infectious Diseases and Vaccinology, National Health Research Institutes, Zhunan Town, Miaoli County, Taiwan; Centers for Disease Control, Taipei, Taiwan.
⁵ National Institute of Infectious Diseases and Vaccinology, National Health Research Institutes, Zhunan Town, Miaoli County, Taiwan. Electronic address: 010113@nhri.edu.tw.

PMID: 36029731
DOI: 10.1016/j.chroma.2022.463427

Abstract

Virions produced from cell culture is the primary source for production of formalin-inactivated whole virus vaccines for enteroviruses. EV-A71 particles produced from culture system comprise two major types, the immature/empty (E)-particle and the mature/full (F)-particle, which both exhibit low isoelectric point (pI) values but have distinct differences in infectivity and immunogenicity. Although EV-A71 particles can conventionally be separated into E-particle and F-particle using sucrose gradient ultracentrifugation, this procedure is cumbersome and difficult to put into practice for vaccine production. Methods based on ion-exchange chromatography have been exploited to improve the purification efficacy; however, none of them are capable of separating the E- and F-particles efficiently. In this study, we aimed to develop an approach to isolate and purify the highly immunogenic mature EV-A71 particles. By applying a step gradient elution procedure, we successfully isolated the viral structure protein VP0-cleaved particles of EV-A71 from a mixture of cultured viral solution using the Q-membrane anion-exchange chromatography. The elution started with 0.1x phosphate buffered saline (PBS) solution while increasing the percentage of 1x PBS containing 1M NaCl in sequential steps. By this procedure, the VP0-cleaved mature particles and VP0-uncleaved immature particles of EV-A71 could be separated into different fractions in Q-membrane with gradually increased NaCl concentration in elution buffer. The purified VP0-cleaved particles were shown to have characteristics equivalent to those of the highly infectious F-particles of EV-A71. The overall recovery rate for the mature EV-A71 particles by Q-membrane is 56% and its purity was shown to be equivalent to those isolated by the sucrose gradient ultracentrifugation. Our approach provides a simple and efficient purification method for recovering mature, highly infectious virus particles from the EV-A71 culture bulk.

Keywords: Anion-exchange column; Enterovirus A71; Liquid chromatography; Mature virions; Virus separation.

MeSH terms

Anions
Antigens, Viral
Enterovirus A, Human*
Enterovirus Infections* / prevention & control
Enterovirus*
Humans
Sodium Chloride
Sucrose

Substances

Anions
Antigens, Viral
Sodium Chloride
Sucrose