Identification of Fc Gamma Receptor Glycoforms That Produce Differential Binding Kinetics for Rituximab

Jerrard M Hayes; Asa Frostell; Robert Karlsson; Steffen Müller; Silvia Míllan Martín; Martin Pauers; Franziska Reuss; Eoin F Cosgrave; Cecilia Anneren; Gavin P Davey; Pauline M Rudd

doi:10.1074/mcp.M117.066944

Identification of Fc Gamma Receptor Glycoforms That Produce Differential Binding Kinetics for Rituximab

Mol Cell Proteomics. 2017 Oct;16(10):1770-1788. doi: 10.1074/mcp.M117.066944. Epub 2017 Jun 2.

Authors

Affiliations

¹ From the ‡School of Biochemistry & Immunology, Trinity Biomedical Sciences Institute, Trinity College Dublin, Pearse St. Dublin 2, Ireland; jehayes@tcd.ie.
² §GE Healthcare, Björkgatan, SE-75184 Uppsala, Sweden.
³ ¶NIBRT-Glycoscience Group, NIBRT-The National Institute for Bioprocessing, Research and Training, Foster Avenue, Blackrock, County Dublin, Ireland.
⁴ ‖Boehringer Ingelheim Pharma, Biberach/Riss, Germany.
⁵ From the ‡School of Biochemistry & Immunology, Trinity Biomedical Sciences Institute, Trinity College Dublin, Pearse St. Dublin 2, Ireland.

Abstract

Fc gamma receptors (FcγR) bind the Fc region of antibodies and therefore play a prominent role in antibody-dependent cell-based immune responses such as ADCC, CDC and ADCP. The immune effector cell activity is directly linked to a productive molecular engagement of FcγRs where both the protein and glycan moiety of antibody and receptor can affect the interaction and in the present study we focus on the role of the FcγR glycans in this interaction. We provide a complete description of the glycan composition of Chinese hamster ovary (CHO) expressed human Fcγ receptors RI (CD64), RIIa_{Arg131/His131} (CD32a), RIIb (CD32b) and RIIIa_{Phe158/Val158} (CD16a) and analyze the role of the glycans in the binding mechanism with IgG. The interactions of the monoclonal antibody rituximab with each FcγR were characterized and we discuss the CHO-FcγRIIIa_{Phe158/Val158} and CHO-FcγRI interactions and compare them to the equivalent interactions with human (HEK293) and murine (NS0) produced receptors. Our results reveal clear differences in the binding profiles of rituximab, which we attribute in each case to the differences in host cell-dependent FcγR glycosylation. The glycan profiles of CHO expressed FcγRI and FcγRIIIa_{Phe158/Val158} were compared with the glycan profiles of the receptors expressed in NS0 and HEK293 cells and we show that the glycan type and abundance differs significantly between the receptors and that these glycan differences lead to the observed differences in the respective FcγR binding patterns with rituximab. Oligomannose structures are prevalent on FcγRI from each source and likely contribute to the high affinity rituximab interaction through a stabilization effect. On FcγRI and FcγRIIIa large and sialylated glycans have a negative impact on rituximab binding, likely through destabilization of the interaction. In conclusion, the data show that the IgG1-FcγR binding kinetics differ depending on the glycosylation of the FcγR and further support a stabilizing role of FcγR glycans in the antibody binding interaction.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
CHO Cells / metabolism
Cell Line
Cricetulus / immunology
Glycosylation
HEK293 Cells
Humans
Immunity, Cellular
Kinetics
Mice
Polysaccharides / immunology*
Polysaccharides / metabolism
Protein Binding
Receptors, IgG / immunology*
Receptors, IgG / metabolism
Rituximab / immunology*
Rituximab / metabolism

Substances

Polysaccharides
Receptors, IgG
Rituximab