Harnessing metabolic plasticity in CHO cells for enhanced perfusion cultivation

Author:

Nöbel Matthias1ORCID,Barry Craig12ORCID,MacDonald Michael A.1,Baker Kym3,Shave Evan3,Mahler Stephen1ORCID,Munro Trent1ORCID,Martínez Verónica S.1ORCID,Nielsen Lars K.1245ORCID,Marcellin Esteban125ORCID

Affiliation:

1. Australian Institute for Bioengineering and Nanotechnology, ARC Training Centre for Biopharmaceutical Innovation The University of Queensland St. Lucia Australia

2. ARC Centre of Excellence in Synthetic Biology (COESB) The University of Queensland St. Lucia Australia

3. Thermo Fisher Scientific Woolloongabba Australia

4. The Novo Nordisk Foundation Centre for Biosustainability Technical University of Denmark Kongens Lyngby Denmark

5. Queensland Metabolomics and Proteomics (Q‐MAP) The University of Queensland St. Lucia Australia

Abstract

AbstractChinese Hamster Ovary (CHO) cells have rapidly become a cornerstone in biopharmaceutical production. Recently, a reinvigoration of perfusion culture mode in CHO cell cultivation has been observed. However, most cell lines currently in use have been engineered and adapted for fed‐batch culture methods, and may not perform optimally under perfusion conditions. To improve the cell's resilience and viability during perfusion culture, we cultured a triple knockout CHO cell line, deficient in three apoptosis related genes BAX, BAK, and BOK in a perfusion system. After 20 days of culture, the cells exhibited a halt in cell proliferation. Interestingly, following this phase of growth arrest, the cells entered a second growth phase. During this phase, the cell numbers nearly doubled, but cell specific productivity decreased. We performed a proteomics investigation, elucidating a distinct correlation between growth arrest and cell cycle arrest and showing an upregulation of the central carbon metabolism and oxidative phosphorylation. The upregulation was partially reverted during the second growth phase, likely caused by intragenerational adaptations to stresses encountered. A phase‐dependent response to oxidative stress was noted, indicating glutathione has only a secondary role during cell cycle arrest. Our data provides evidence of metabolic regulation under high cell density culturing conditions and demonstrates that cell growth arrest can be overcome. The acquired insights have the potential to not only enhance our understanding of cellular metabolism but also contribute to the development of superior cell lines for perfusion cultivation.

Funder

Novo Nordisk Fonden

Publisher

Wiley

Subject

Applied Microbiology and Biotechnology,Bioengineering,Biotechnology

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