AI Article Synopsis

  • The study explores the use of Activation Induced Marker (AIM) assays to measure antigen-specific T-cell responses while preserving information about pre-activation cell populations by utilizing specific lineage markers.
  • Researchers sorted three distinct CD4 T-cell populations (memory non-Tregs, CD39 Tregs, and another Treg type) and labeled them with fluorescent dyes to track their responses during AIM assays triggered by CMV and HSV antigens.
  • Findings indicate that while CD39 Tregs are prominent in AIM responses, they do not significantly contribute to the overall T-cell proliferative response, allowing for a better understanding of how different T-cell subsets participate in immune memory.

Article Abstract

Activation induced marker (AIM) assays are being used increasingly to measure antigen-specific T-cell responses, but this activation can alter cell lineage defining phenotypic markers. We aimed to extend the utility of AIM assays to enable pre-activation defined cell populations to be tracked and quantified within T-cell memory responses. We sorted three ex vivo CD4 T-cell populations prior to any activation using well defined ex vivo lineage surface marker combinations. These populations were memory non-Tregs, CD39 Tregs and CD39 Tregs, although any three memory CD4 T-cell populations able to be isolated by cell surface markers could potentially be tracked. These cells were labeled with three distinct fluorescent cell proliferation dyes (CFSE, CellTrace Violet and Cell Proliferation Dye eF670) and then all autologous PBMCs were reconstituted maintaining ex vivo cell ratios and CD25/OX40 AIM assays performed with CMV and HSV antigens. This approach enabled tracking of pre-defined cell populations within antigen stimulated responses using both activation marker and cell proliferation readouts. We confirmed that although CD39 Tregs comprise a substantial proportion of AIM assay responses, they do not make substantial contributions to the proliferative response. This extends the utility of AIM assays to enable parallel analysis of the relative contribution of several CD4 memory T-cell subsets to recall responses.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10952787PMC
http://dx.doi.org/10.1111/imcb.12606DOI Listing

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