Literature DB >> 30442400

Heterogeneity assessment of antibody-derived therapeutics at the intact and middle-up level by low-flow sheathless capillary electrophoresis-mass spectrometry.

Rob Haselberg1, Thomas De Vijlder2, Raimond Heukers3, Martine J Smit3, Edwin P Romijn2, Govert W Somsen4, Elena Domínguez-Vega1.   

Abstract

Antibody-based pharmaceuticals often encompass a complex structural heterogeneity requiring enhanced analytical methods for reliable characterization of variants and degradation products. We have explored the capabilities of low-flow sheathless capillary electrophoresis-mass spectrometry (CE-MS) for the high-resolution and sensitive profiling of antibody therapeutics. Near-zero electroosmotic flow was achieved by employing a novel neutral capillary coating that also prevents protein adsorption. CE-MS analysis of intact model proteins using an acidic background electrolyte demonstrated satisfactory performance, with overall migration-time RSDs below 2.2% from three different capillaries tested. For system evaluation, three nanobody preparations, including mono- and bivalent forms, and three monoclonal antibodies (mAbs) were analyzed. Intact nanobodies were resolved from their degradation products, which could be assigned to deamidated, cleaved, and truncated forms at the C-terminal tag. Excellent resolution of isomeric deamidated products was obtained. The mAbs were analyzed intact and after digestion by the endoproteinase IdeS (middle-up approach). CE-MS of intact mAbs provided resolution of clipped species (e.g. light chain and light chain-heavy chain fragments) from the native protein. Moreover, glycoforms containing sialic acids were resolved from their non-sialylated counterparts. For IdeS-digested, F (ab)2 and Fc/2 portions where efficiently resolved for the three mAbs. Whereas the migration time of the Fc/2 fragments was fairly similar, the migration time of the F (ab)2 part was strongly varied among the mAbs. For all mAbs, separation of Fc/2 charge variants - including sialylated glycoforms and other post-translational modifications, such as loss of C-terminal lysine or asparagine deamidation - was achieved. This allowed a detailed and reliable assessment of the Fc/2 heterogeneity (18-33 proteoforms) of the three analyzed mAbs.
Copyright © 2018 The Authors. Published by Elsevier B.V. All rights reserved.

Entities:  

Keywords:  Intact protein analysis; Low-flow CE; Middle-up analysis; Monoclonal antibodies; Nanobodies; Sheathless CE-MS

Mesh:

Substances:

Year:  2018        PMID: 30442400     DOI: 10.1016/j.aca.2018.08.024

Source DB:  PubMed          Journal:  Anal Chim Acta        ISSN: 0003-2670            Impact factor:   6.558


  8 in total

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Review 2.  Recent trends of capillary electrophoresis-mass spectrometry in proteomics research.

Authors:  Fabio P Gomes; John R Yates
Journal:  Mass Spectrom Rev       Date:  2019-08-12       Impact factor: 10.946

Review 3.  Monitoring of immunoglobulin N- and O-glycosylation in health and disease.

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Journal:  Glycobiology       Date:  2020-03-20       Impact factor: 4.313

4.  Monitoring glycation levels of a bispecific monoclonal antibody at subunit level by ultrahigh-resolution MALDI FT-ICR mass spectrometry.

Authors:  Christoph Gstöttner; Dietmar Reusch; Markus Haberger; Irina Dragan; Peter Van Veelen; David P A Kilgour; Yury O Tsybin; Yuri E M van der Burgt; Manfred Wuhrer; Simone Nicolardi
Journal:  MAbs       Date:  2020 Jan-Dec       Impact factor: 5.857

5.  Investigation of monoclonal antibody dimers in a final formulated drug by separation techniques coupled to native mass spectrometry.

Authors:  G Rouby; N T Tran; Y Leblanc; M Taverna; N Bihoreau
Journal:  MAbs       Date:  2020 Jan-Dec       Impact factor: 5.857

Review 6.  Analytical Similarity Assessment of Biosimilars: Global Regulatory Landscape, Recent Studies and Major Advancements in Orthogonal Platforms.

Authors:  Neh Nupur; Srishti Joshi; Davy Gulliarme; Anurag S Rathore
Journal:  Front Bioeng Biotechnol       Date:  2022-02-09

7.  Affinity capillary electrophoresis - mass spectrometry permits direct binding assessment of IgG and FcγRIIa in a glycoform-resolved manner.

Authors:  Christoph Gstöttner; Alexander Knaupp; Gestur Vidarsson; Dietmar Reusch; Tilman Schlothauer; Manfred Wuhrer; Elena Domínguez-Vega
Journal:  Front Immunol       Date:  2022-09-08       Impact factor: 8.786

8.  MS-Based Allotype-Specific Analysis of Polyclonal IgG-Fc N-Glycosylation.

Authors:  Thomas Sénard; Andrea F G Gargano; David Falck; Steven W de Taeye; Theo Rispens; Gestur Vidarsson; Manfred Wuhrer; Govert W Somsen; Elena Domínguez-Vega
Journal:  Front Immunol       Date:  2020-08-21       Impact factor: 7.561

  8 in total

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