A Single-Step Method for Harvesting Influenza Viral Particles from MDCK Cell Culture Supernatant with High Yield and Effective Impurity Removal-Reference-Cited by-同舟云学术

A Single-Step Method for Harvesting Influenza Viral Particles from MDCK Cell Culture Supernatant with High Yield and Effective Impurity Removal

Published:2024-05-13 Issue:5 Volume:16 Page:768
ISSN:1999-4915
Container-title:Viruses
language:en
Short-container-title:Viruses

Author:

Liu Sixu¹,Li Jingqi¹²,Cheng Qingtian¹,Duan Kangyi¹,Wang Zhan³,Yan Shuang¹,Tian Shuaishuai¹,Wang Hairui¹⁴,Wu Shaobin¹⁵,Lei Xinkui¹⁵,Yang Yu³,Ma Ningning¹

Affiliation:

1. Wuya College of Innovation, Shenyang Pharmaceutical University, Shenyang 110016, China

2. GenScript (Shanghai) Biotech Co., Ltd., Shanghai 200131, China

3. School of Life Science and Biopharmaceutics, Shenyang Pharmaceutical University, Shenyang 110016, China

4. Qilu Pharmaceutical Co., Ltd., Jinan 250104, China

5. Beijing Zhifei Lvzhu Biopharmaceutical Co., Ltd., Beijing 100176, China

Abstract

Influenza vaccines, which are recommended by the World Health Organization (WHO), are the most effective preventive measure against influenza virus infection. Madin–Darby canine kidney (MDCK) cell culture is an emerging technology used to produce influenza vaccines. One challenge when purifying influenza vaccines using this cell culture system is to efficiently remove impurities, especially host cell double-stranded DNA (dsDNA) and host cell proteins (HCPs), for safety assurance. In this study, we optimized ion-exchange chromatography methods to harvest influenza viruses from an MDCK cell culture broth, the first step in influenza vaccine purification. Bind/elute was chosen as the mode of operation for simplicity. The anion-exchange Q chromatography method was able to efficiently remove dsDNA and HCPs, but the recovery rate for influenza viruses was low. However, the cation-exchange SP process was able to simultaneously achieve high dsDNA and HCP removal and high influenza virus recovery. For the SP process to work, the clarified cell culture broth needed to be diluted to reduce its ionic strength, and the optimal dilution rate was determined to be 1:2 with purified water. The SP process yielded a virus recovery rate exceeding 90%, as measured using a hemagglutination units (HAUs) assay, with removal efficiencies over 97% for HCPs and over 99% for dsDNA. Furthermore, the general applicability of the SP chromatography method was demonstrated with seven strains of influenza viruses recommended for seasonal influenza vaccine production, including H1N1, H3N2, B (Victoria), and B (Yamagata) strains, indicating that the SP process could be utilized as a platform process. The SP process developed in this study showed four advantages: (1) simple operation, (2) a high recovery rate for influenza viruses, (3) a high removal rate for major impurities, and (4) general applicability.

Publisher

MDPI AG

Link

https://www.mdpi.com/1999-4915/16/5/768/pdf

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