Development of a novel flow cytometry method for detecting pneumococcal-specific B cells

Irene Tzovara; Ioanna Papadatou; Marianna Tzanoudaki; Vasiliki Spoulou

doi:10.1002/cyto.a.24654

Development of a novel flow cytometry method for detecting pneumococcal-specific B cells

Cytometry A. 2022 Jul;101(7):588-596. doi: 10.1002/cyto.a.24654. Epub 2022 May 24.

Authors

Irene Tzovara¹, Ioanna Papadatou¹, Marianna Tzanoudaki², Vasiliki Spoulou¹

Affiliations

¹ Department of Infectious Diseases - Immunobiology and Vaccinology Research Lab, "Aghia Sophia" Children's Hospital, 1st Department of Pediatrics - National and Kapodistrian University of Athens, Athens, Greece.
² Department of Immunology and Histocompatibility, Specific Reference Centre for Primary Immunodeficiencies-Paediatric Immunology, "Aghia Sophia" Children's Hospital, Athens, Greece.

PMID: 35527678
DOI: 10.1002/cyto.a.24654

Abstract

Antigen-specific B cell identification by flow cytometry is crucial for investigating their immunophenotype, subset distribution, and kinetics post-infection or immunization. Methods using biotinylated polysaccharide antigens have been described, but there is still room for improvement regarding sensitivity and applicability. The aim of this study was the development and validation of a multimer bead-based method for detecting pneumococcal polysaccharide serotypes (PS)-specific B cells following pneumococcal immunization. PS was chemically biotinylated and mounted on anti-biotin beads, and labeled with phycoerythrin (PE)-conjugated anti-biotin antibody to form a PS-multimer used for cell staining. Labeled beads were washed to remove excess fluorochrome and diminish non-specific labeling and background noise. Optimal ratios of PS-bead conjugate to PE and PS-multimer to cells were determined with titration assays. Comparison between the PS-multimer and a PS-PE monomer revealed enhanced detection of PS-specific cells and considerable signal amplification, attributed to the multimeric form of the detection probe and increased availability of antigen epitopes. To validate the specificity of the method, a competition assay using unbound PS was performed. Following pre-incubation with increasing PS concentrations, detection of PS-specific B cells with the PS-multimer was inhibited in a stepwise manner. Pre-incubation with excess PS completely blocked the fluorescent signal. This novel bead-based flow cytometry approach is a sensitive method demonstrating high specificity. It generated enhanced signals, provided clear-cut results, and was easily applicable, not requiring B cell pre-enrichment. It could be modified to adapt other antigens of interest, especially polysaccharides and proteins that could be used to probe antigen-specific B cell responses. The study of such responses may elucidate the underlying mechanisms involved in the establishment of long-term protection, provide evidence-based rationale for improving currently available vaccines and vaccination strategies, and pave the way for future vaccine development.

Keywords: 13-valent pneumococcal vaccine; antigen-specific; antigen-specific B cells; antigen-specific multimer; flow cytometry; memory B cells; pneumococcal vaccines; pneumococcal-specific B cells.

Publication types

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

MeSH terms

Antibodies, Bacterial*
B-Lymphocytes
Flow Cytometry
Pneumococcal Vaccines* / metabolism
Streptococcus pneumoniae

Substances

Antibodies, Bacterial
Pneumococcal Vaccines