Prediction of CHO cell line stability using expression of DNA repair genes

Author:

Cordova Lauren T.1,Dahodwala Hussain12,Cooley Rebecca3,Lee Kelvin H.12ORCID

Affiliation:

1. Department of Chemical and Biomolecular Engineering University of Delaware Newark Delaware USA

2. National Institute for Innovation in Manufacturing Biopharmaceuticals Newark Delaware USA

3. Pfizer, Inc, 875 Chesterfield Pkwy W Chesterfield Missouri USA

Abstract

AbstractChinese hamster ovary (CHO) cells are essential to biopharmaceutical manufacturing and production instability, the loss of productivity over time, is a long‐standing challenge in the industry. Accurate prediction of cell line stability could enable efficient screening to identify clones suitable for manufacturing saving significant time and costs. DNA repair genes may offer biomarkers to address this need. In this study, over 40 cell lines representing various host lineages from three companies/organizations were evaluated for expression of five DNA repair genes (Fam35a, Lig4, Palb2, Pari, and Xrcc6). Expression measured in cells with less than 30 population doubling levels (PDLs) was correlated to stability profiles at 60+ PDL. Principal component analysis identified markers which separate stable and unstable CHO‐DG44 cell lines. Notably, two genes, Lig4 and Xrcc6, showed higher expression in unstable CHO‐DG44 cell lines with copy number loss identified as the mechanism of production instability. Expression levels across all cell ages showed lower DNA repair gene expression was associated with increased cell age. Collectively, DNA repair genes provide critical insight into long‐term behavior of CHO cells and their expression levels have potential to predict cell line stability in certain cases.

Funder

National Science Foundation

National Institute of Standards and Technology

Publisher

Wiley

Subject

Molecular Medicine,Applied Microbiology and Biotechnology,General Medicine

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