Immunoglobulin G genetic variation can confound assessment of antibody levels via altered binding to detection reagents

Ruth A Purcell; L Carissa Aurelia; Robyn Esterbauer; Lilith F Allen; Katherine A Bond; Deborah A Williamson; Janine M Trevillyan; Jason A Trubiano; Jennifer J Juno; Adam K Wheatley; Miles P Davenport; Thi Ho Nguyen; Katherine Kedzierska; Stephen J Kent; Kevin John Selva; Amy W Chung

doi:10.1002/cti2.1494

Immunoglobulin G genetic variation can confound assessment of antibody levels via altered binding to detection reagents

Clin Transl Immunology. 2024 Feb 29;13(3):e1494. doi: 10.1002/cti2.1494. eCollection 2024.

Authors

Ruth A Purcell¹, L Carissa Aurelia¹, Robyn Esterbauer¹, Lilith F Allen¹, Katherine A Bond^{1

2}, Deborah A Williamson^{2

3

4}, Janine M Trevillyan^{4

5}, Jason A Trubiano^{5

6

7

8}, Jennifer J Juno¹, Adam K Wheatley¹, Miles P Davenport⁹, Thi Ho Nguyen¹, Katherine Kedzierska¹, Stephen J Kent^{1

10}, Kevin John Selva¹, Amy W Chung¹

Affiliations

¹ Department of Microbiology and Immunology The Peter Doherty Institute for Infection and Immunity, University of Melbourne Melbourne VIC Australia.
² Victorian Infectious Diseases Reference Laboratory (VIDRL) The Peter Doherty Institute for Infection and Immunity Melbourne VIC Australia.
³ Walter and Eliza Hall Institute of Medical Research Parkville VIC Australia.
⁴ Department of Infectious Diseases The Peter Doherty Institute for Infection and Immunity, University of Melbourne Melbourne VIC Australia.
⁵ Centre for Antibiotic Allergy and Research, Department of Infectious Diseases Austin Health Heidelberg VIC Australia.
⁶ Department of Medicine University of Melbourne Parkville VIC Australia.
⁷ Department of Infectious Diseases Peter MacCallum Cancer Centre Melbourne VIC Australia.
⁸ National Centre for Infections in Cancer Peter MacCallum Cancer Centre Melbourne VIC Australia.
⁹ Kirby Institute University of New South Wales Kensington NSW Australia.
¹⁰ Melbourne Sexual Health Centre and Department of Infectious Diseases, Alfred Health, Central Clinical School Monash University Melbourne VIC Australia.

Abstract

Objectives: Amino acid variations across more than 30 immunoglobulin (Ig) allotypes may introduce structural changes that influence recognition by anti-Ig detection reagents, consequently confounding interpretation of antibody responses, particularly in genetically diverse cohorts. Here, we assessed a panel of commercial monoclonal anti-IgG1 clones for capacity to universally recognise two dominant IgG1 haplotypes (G1m-1,3 and G1m1,17).

Methods: Four commercial monoclonal anti-human IgG1 clones were assessed via ELISAs and multiplex bead-based assays for their ability to bind G1m-1,3 and G1m1,17 IgG1 variants. Detection antibodies were validated against monoclonal IgG1 allotype standards and tested for capacity to recognise antigen-specific plasma IgG1 from G1m-1,3 and G1m1,17 homozygous and heterozygous SARS-CoV-2 BNT162b2 vaccinated (n = 28) and COVID-19 convalescent (n = 44) individuals. An Fc-specific pan-IgG detection antibody corroborated differences between hinge- and Fc-specific anti-IgG1 responses.

Results: Hinge-specific anti-IgG1 clone 4E3 preferentially bound G1m1,17 compared to G1m-1,3 IgG1. Consequently, SARS-CoV-2 Spike-specific IgG1 levels detected in G1m1,17/G1m1,17 BNT162b2 vaccinees appeared 9- to 17-fold higher than in G1m-1,3/G1m-1,3 vaccinees. Fc-specific IgG1 and pan-IgG detection antibodies equivalently bound G1m-1,3 and G1m1,17 IgG1 variants, and detected comparable Spike-specific IgG1 levels between haplotypes. IgG1 responses against other human coronaviruses and influenza were similarly poorly detected by 4E3 anti-IgG1 in G1m-1,3/G1m-1,3 subjects.

Conclusion: Anti-IgG1 clone 4E3 confounds assessment of antibody responses in clinical cohorts owing to bias towards detection of G1m1,17 IgG1 variants. Validation of anti-Ig clones should include evaluation of binding to relevant antibody variants, particularly as the role of immunogenetics upon humoral immunity is increasingly explored in diverse populations.

Keywords: IgG; allotype; anti‐immunoglobulin; polymorphisms; reproducibility; serology.