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

Rob Haselberg; Thomas De Vijlder; Raimond Heukers; Martine J Smit; Edwin P Romijn; Govert W Somsen; Elena Domínguez-Vega

doi:10.1016/j.aca.2018.08.024

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

Anal Chim Acta. 2018 Dec 31:1044:181-190. doi: 10.1016/j.aca.2018.08.024. Epub 2018 Aug 15.

Authors

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

Affiliations

¹ Division of BioAnalytical Chemistry, Department of Chemistry and Pharmaceutical Sciences, Vrije Universiteit Amsterdam, de Boelelaan 1085, 1081 HV, Amsterdam, The Netherlands.
² Pharmaceutical Development and Manufacturing Sciences, Janssen Research and Development, Turnhoutseweg 30, 2340, Beerse, Belgium.
³ Division of Medicinal Chemistry, Faculty of Sciences, Vrije Universiteit Amsterdam, de Boelelaan 1085, 1081 HV, Amsterdam, The Netherlands.
⁴ Division of BioAnalytical Chemistry, Department of Chemistry and Pharmaceutical Sciences, Vrije Universiteit Amsterdam, de Boelelaan 1085, 1081 HV, Amsterdam, The Netherlands. Electronic address: g.w.somsen@vu.nl.

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

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.

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

MeSH terms

Antibodies, Monoclonal / analysis*
Antibodies, Monoclonal / chemistry*
Antibodies, Monoclonal / pharmacology
Antibodies, Monoclonal / therapeutic use
Electrophoresis, Capillary / methods*
Immunoglobulin Fc Fragments / chemistry
Mass Spectrometry / methods*
Sialic Acids / chemistry

Substances

Antibodies, Monoclonal
Immunoglobulin Fc Fragments
Sialic Acids