Vaccine-induced SARS-CoV-2 antibody response: the comparability of S1-specific binding assays depends on epitope and isotype discrimination

Silvia Schest; Claus Langer; Yuriko Stiegler; Bianca Karnuth; Jan Arends; Hugo Stiegler; Thomas Masetto; Christoph Peter; Matthias Grimmler

doi:10.3389/fimmu.2023.1257265

Vaccine-induced SARS-CoV-2 antibody response: the comparability of S1-specific binding assays depends on epitope and isotype discrimination

Front Immunol. 2023 Oct 26:14:1257265. doi: 10.3389/fimmu.2023.1257265. eCollection 2023.

Authors

Silvia Schest^{1

2}, Claus Langer¹, Yuriko Stiegler¹, Bianca Karnuth¹, Jan Arends¹, Hugo Stiegler¹, Thomas Masetto^{3

4}, Christoph Peter³, Matthias Grimmler^{4

5

6}

Affiliations

¹ Medizinisches Versorgungszentrum für Labormedizin und Mikrobiologie Ruhr GmbH, Essen, Germany.
² Health University of Applied Sciences Tyrol, Innsbruck, Austria.
³ Institute of Molecular Medicine I, Heinrich Heine University Düsseldorf, Düsseldorf, Germany.
⁴ DiaSys Diagnostic Systems GmbH, Holzheim, Germany.
⁵ Institute for Biomolecular Research, Hochschule Fresenius gGmbH, University of Applied Sciences, Idstein, Germany.
⁶ DiaServe Laboratories GmbH, Iffeldorf, Germany.

Abstract

Background: Quantification of the SARS-CoV-2-specific immune response by serological immunoassays is critical for the management of the COVID-19 pandemic. In particular, neutralizing antibody titers to the viral spike (S) protein have been proposed as a correlate of protection (CoP). The WHO established the First International Standard (WHO IS) for anti-SARS-CoV-2 immunoglobulin (Ig) (NIBSC 20/136) to harmonize binding assays with the same antigen specificity by assigning the same unitage in binding antibody units (BAU)/ml.

Method: In this study, we analyzed the S1-specific antibody response in a cohort of healthcare workers in Germany (n = 76) during a three-dose vaccination course over 8.5 months. Subjects received either heterologous or homologous prime-boost vaccination with ChAdOx1 nCoV-19 (AstraZeneca) and BNT162b2 (Pfizer-BioNTech) or three doses of BNT162b2. Antibodies were quantified using three anti-S1 binding assays (ELISA, ECLIA, and PETIA) harmonized to the WHO IS. Serum levels of neutralizing antibodies were determined using a surrogate virus neutralization test (sVNT). Binding assays were compared using Spearman's rank correlation and Passing-Bablok regression.

Findings: All assays showed good correlation and similar antibody kinetics correlating with neutralizing potential. However, the assays show large proportional differences in BAU/ml. ECLIA and PETIA, which detect total antibodies against the receptor- binding domain (RBD) within the S1 subunit, interact similarly with the convalescent plasma-derived WHO IS but differently with vaccine serum, indicating a high sensitivity to the IgG/IgM/IgA ratio.

Conclusion: All three binding assays allow monitoring of the antibody response in COVID-19-vaccinated individuals. However, the assay-specific differences hinder the definition of a common protective threshold in BAU/ml. Our results highlight the need for the thoughtful use of conversion factors and consideration of method-specific differences. To improve the management of future pandemics and harmonize total antibody assays, we should strive for reference material with a well-characterized Ig isotype composition.

Keywords: COVID-19 vaccines; SARS-CoV-2 antibody; WHO standard; correlate of protection; humoral immune response; neutralizing antibodies; serological testing; spike protein.

MeSH terms

Antibodies, Viral
BNT162 Vaccine
COVID-19 Serotherapy
COVID-19*
ChAdOx1 nCoV-19
Epitopes
Humans
Immunoglobulin Isotypes
Pandemics
SARS-CoV-2
Vaccines*

Substances

BNT162 Vaccine
Epitopes
ChAdOx1 nCoV-19
Immunoglobulin Isotypes
Antibodies, Viral
Vaccines

Grants and funding

The author(s) declare that no financial support was received for the research, authorship, and/or publication of this article.