Strategies for the production of isotopically labelled Fab fragments of therapeutic antibodies in Komagataella phaffii

Strategies for the production of isotopically labelled Fab fragments of therapeutic antibodies in Komagataella phaffii

The importance and fast growth of therapeutic monoclonal antibodies, both innovator and biosimilar products, have triggered the need for the development of characterization methods at high resolution such as nuclear magnetic resonance (NMR) spectroscopy. However, the full power of NMR spectroscopy c...

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Bibliographic Details
Published in:PloS one Vol. 18; no. 11; p. e0294406
Main Authors: Gagné, Donald, Sarker, Muzaddid, Gingras, Geneviève, Hodgson, Derek J, Frahm, Grant, Creskey, Marybeth, Lorbetskie, Barry, Bigelow, Stewart, Wang, Jun, Zhang, Xu, Johnston, Michael J. W, Lu, Huixin, Aubin, Yves
Format: Journal Article
Language:English
Published: Public Library of Science 29-11-2023
Subjects:
Analysis
Escherichia coli
Methods
Nuclear magnetic resonance spectroscopy
Yeast fungi
Canada
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Summary:The importance and fast growth of therapeutic monoclonal antibodies, both innovator and biosimilar products, have triggered the need for the development of characterization methods at high resolution such as nuclear magnetic resonance (NMR) spectroscopy. However, the full power of NMR spectroscopy cannot be unleashed without labelling the mAb of interest with NMR-active isotopes. Here, we present strategies using either Komagataella phaffii (Pichia pastoris) or Escherichia coli that can be widely applied for the production of the antigen-binding fragment (Fab) of therapeutic antibodies of immunoglobulin G1 kappa isotype. The E. coli approach consists of expressing Fab fragments as a single polypeptide chain with a cleavable linker between the heavy and light chain in inclusion bodies, while K. phaffii secretes a properly folded fragment in the culture media. After optimization, the protocol yielded 10-45 mg of single chain adalimumab-Fab, trastuzumab-Fab, rituximab-Fab, and NISTmAb-Fab per liter of culture. Comparison of the 2D-.sup.1 H-.sup.15 N-HSQC spectra of each Fab fragment, without their polyhistidine tag and linker, with the corresponding Fab from the innovator product showed that all four fragments have folded into the correct conformation. Production of .sup.2 H-.sup.13 C-.sup.15 N-adalimumab-scFab and .sup.2 H-.sup.13 C-.sup.15 N-trastuzumab-scFab (>98% enrichment for all three isotopes) yielded NMR samples where all amide deuterons have completely exchanged back to proton during the refolding procedure.
ISSN:1932-6203
1932-6203
DOI:10.1371/journal.pone.0294406