4.7 Article

Exploring the molecular content of CHO exosomes during bioprocessing

Journal

APPLIED MICROBIOLOGY AND BIOTECHNOLOGY
Volume 105, Issue 9, Pages 3673-3689

Publisher

SPRINGER
DOI: 10.1007/s00253-021-11309-8

Keywords

Biotechnology; CHO; Exosomes; Proteomics; miRNA; piRNA

Funding

  1. Projekt DEAL
  2. European Regional Development Fund (EFRE) through project Cluster Industrial Biotechnology (CLIB) Kompetenzzentrum Biotechnologie (CKB) [34. EFRE-0300095/1703FI04]

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CHO cells derived from Chinese hamster ovaries are widely used in biopharmaceutical production, but research on exosomes in these cells is scarce. Exosomes are considered a universal mediator of intercellular communication and a proposed new drug delivery format in biopharmaceuticals. This study analyzed the proteome and RNA of exosomes from CHO-K1 cells, providing reference data for future research.
In biopharmaceutical production, Chinese hamster ovary (CHO) cells derived from Cricetulus griseus remain the most commonly used host cell for recombinant protein production, especially antibodies. Over the last decade, in-depth multi-omics characterization of these CHO cells provided data for extensive cell line engineering and corresponding increases in productivity. However, exosomes, extracellular vesicles containing proteins and nucleic acids, are barely researched at all in CHO cells. Exosomes have been proven to be a ubiquitous mediator of intercellular communication and are proposed as new biopharmaceutical format for drug delivery, indicator reflecting host cell condition and anti-apoptotic factor in spent media. Here we provide a brief overview of different separation techniques and subsequently perform a proteome and regulatory, non-coding RNA analysis of exosomes, derived from lab-scale bioreactor cultivations of a CHO-K1 cell line, to lay out reference data for further research in the field. Applying bottom-up orbitrap shotgun proteomics and next-generation small RNA sequencing, we detected 1395 proteins, 144 micro RNA (miRNA), and 914 PIWI-interacting RNA (piRNA) species differentially across the phases of a batch cultivation process. The exosomal proteome and RNA data are compared with other extracellular fractions and cell lysate, yielding several significantly exosome-enriched species.

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