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Affinity tag coating enables reliable detection of antigen-specific B cells in ImmunoSpot assays
Sebastian Koppert; Carla Wolf; Noemi Becza; Giuseppe A Sautto; Fridolin Franke; Stefanie Kurten; Paul V Lehmann; Ted M Ross; Greg A Kirchenbaum.
Afiliação
  • Sebastian Koppert; Institute of Anatomy and Cell Biology, Friedrich-Alexander University Erlangen-Nurnberg
  • Carla Wolf; Institute of Anatomy and Cell Biology, Friedrich-Alexander University Erlangen-Nurnberg
  • Noemi Becza; Research & Development Department, Cellular Technology Limited
  • Giuseppe A Sautto; Center for Vaccines and Immunology, University of Georgia
  • Fridolin Franke; Research & Development Department, Cellular Technology Limited
  • Stefanie Kurten; Institute of Anatomy and Cell Biology, Friedrich-Alexander University Erlangen-Nurnberg
  • Paul V Lehmann; Research & Development Department, Cellular Technology Limited
  • Ted M Ross; University System of Georgia
  • Greg A Kirchenbaum; Research & Development Department, Cellular Technology Limited
Preprint em En | PREPRINT-MEDRXIV | ID: ppmedrxiv-21258073
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ABSTRACT
Assessment of humoral immunity to SARS-CoV-2 and other infectious agents is typically restricted to detecting antigen-specific antibody in the serum. Rarely does immune monitoring entail assessment of the memory B cell compartment itself, although it is these cells that engage in secondary antibody responses capable of mediating immune protection when pre-existing antibodies fail to prevent re-infection. There are few techniques that are capable of detecting rare antigen-specific B cells while also providing information regarding their precursory frequency, class/subclass usage and functional affinity. In theory, the ELISPOT/FluoroSpot (collectively ImmunoSpot) assay platform is ideally-suited for antigen-specific B cell assessments since it provides this information at single-cell resolution for individual antibody-secreting cells (ASC). Here, we tested the hypothesis that antigen coating efficiency could be universally improved across a diverse set of viral antigens if the standard direct (non-specific, low affinity) antigen absorption to the membrane was substituted by high affinity capture. Specifically, we report an enhancement in assay sensitivity and a reduction in required protein concentrations through the capture of recombinant proteins via their encoded hexahistidine (6XHis) affinity tag. Affinity tag antigen coating enabled detection of SARS-CoV-2 Spike receptor binding domain (RBD)-reactive ASC, and also significantly improved assay performance using additional control antigens. Collectively, establishment of a universal antigen coating approach streamlines characterization of the memory B cell compartment after SARS-CoV-2 infection or COVID-19 vaccinations, and facilitates high-throughput immune monitoring efforts of large donor cohorts in general.
Licença
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Texto completo: 1 Coleções: 09-preprints Base de dados: PREPRINT-MEDRXIV Tipo de estudo: Cohort_studies / Diagnostic_studies / Observational_studies / Prognostic_studies Idioma: En Ano de publicação: 2021 Tipo de documento: Preprint
Texto completo: 1 Coleções: 09-preprints Base de dados: PREPRINT-MEDRXIV Tipo de estudo: Cohort_studies / Diagnostic_studies / Observational_studies / Prognostic_studies Idioma: En Ano de publicação: 2021 Tipo de documento: Preprint