Rapid identification of highly potent human anti-GPCR antagonist monoclonal antibodies

Martin J Scott; Amanda Jowett; Martin Orecchia; Peter Ertl; Larissa Ouro-Gnao; Julia Ticehurst; David Gower; John Yates; Katie Poulton; Carol Harris; Michael J Mullin; Kathrine J Smith; Alan P Lewis; Nick Barton; Michael L Washburn; Ruud de Wildt

doi:10.1080/19420862.2020.1755069

Rapid identification of highly potent human anti-GPCR antagonist monoclonal antibodies

MAbs. 2020 Jan-Dec;12(1):1755069. doi: 10.1080/19420862.2020.1755069.

Authors

Affiliations

¹ Department of Biopharm Discovery, Glaxo Smith Kline Research & Development, Hertfordshire, UK.
² Department of Protein & Cellular Sciences, Glaxo Smith Kline Research & Development, Hertfordshire, UK.
³ Department of Data & Computational Sciences, Glaxo Smith Kline Research & Development, Hertfordshire, UK.
⁴ Experimental Medicine Unit, Glaxo Smith Kline Research & Development, Collegeville, PA, USA.

Abstract

Complex cellular targets such as G protein-coupled receptors (GPCRs), ion channels, and other multi-transmembrane proteins represent a significant challenge for therapeutic antibody discovery, primarily because of poor stability of the target protein upon extraction from cell membranes. To assess whether a limited set of membrane-bound antigen formats could be exploited to identify functional antibodies directed against such targets, we selected a GPCR of therapeutic relevance (CCR1) and identified target binders using an in vitro yeast-based antibody discovery platform (Adimab^TM) to expedite hit identification. Initially, we compared two different biotinylated antigen formats overexpressing human CCR1 in a 'scouting' approach using a subset of the antibody library. Binders were isolated using streptavidin-coated beads, expressed as yeast supernatants, and screened using a high-throughput binding assay and flow cytometry on appropriate cell lines. The most suitable antigen was then selected to isolate target binders using the full library diversity. This approach identified a combined total of 183 mAbs with diverse heavy chain sequences. A subset of clones exhibited high potencies in primary cell chemotaxis assays, with IC₅₀ values in the low nM/high pM range. To assess the feasibility of any further affinity enhancement, full-length hCCR1 protein was purified, complementary-determining region diversified libraries were constructed from a high and lower affinity mAb, and improved binders were isolated by fluorescence-activated cell sorting selections. A significant affinity enhancement was observed for the lower affinity parental mAb, but not the high affinity mAb. These data exemplify a methodology to generate potent human mAbs for challenging targets rapidly using whole cells as antigen and define a route to the identification of affinity-matured variants if required.

Keywords: AdimabTM; Antibody discovery; G protein-coupled receptor; affinity maturation; complex membrane targets; live cell selections; mAb; monoclonal antibody; multi-transmembrane protein; yeast-based platform.

MeSH terms

Animals
Antibodies, Monoclonal / immunology*
Antibodies, Monoclonal / pharmacology
Antibody Affinity / immunology*
Antibody Specificity / immunology*
CHO Cells
Cricetinae
Cricetulus
HEK293 Cells
Humans
Peptide Library
Protein Binding / drug effects
Receptors, CCR1 / antagonists & inhibitors
Receptors, CCR1 / immunology*
Receptors, CCR1 / metabolism
Receptors, G-Protein-Coupled / antagonists & inhibitors
Receptors, G-Protein-Coupled / immunology*
Receptors, G-Protein-Coupled / metabolism
Recombinant Proteins / immunology
Recombinant Proteins / metabolism
Recombinant Proteins / pharmacology

Substances

Antibodies, Monoclonal
CCR1 protein, human
Peptide Library
Receptors, CCR1
Receptors, G-Protein-Coupled
Recombinant Proteins