MHC class II tetramers identify peptide-specific human CD4+ T cells proliferating in response to influenza A antigen
Erik J. Novak, … , Gerald T. Nepom, William W. Kwok
Erik J. Novak, … , Gerald T. Nepom, William W. Kwok
Published December 15, 1999
Citation Information: J Clin Invest. 1999;104(12):R63-R67. https://doi.org/10.1172/JCI8476.
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MHC class II tetramers identify peptide-specific human CD4+ T cells proliferating in response to influenza A antigen

Abstract

Antigen-specific T helper cells present in peripheral blood at very low frequencies are capable of rapid clonal expansion during antigenic challenge. The exquisite specificity of this response provides for activation and expansion of a very select cohort of T cells, a feature we have used to directly identify and quantify human epitope-specific T helper cells from peripheral blood. Soluble tetramerized class II MHC molecules, loaded with an immunodominant peptide from hemagglutinin (HA) and labeled with fluorescent dyes, were constructed and used to directly identify antigen-specific T cells from influenza-immune individuals. After 7 days of proliferation in response to stimulation by HA peptide or whole influenza vaccine, cells staining positive with the HA tetramer had undergone between 6 and 9 divisions and were CD3+, CD4+, CD25+, and CD8–, characteristic of activated T helper cells responding to antigen. The HA epitope-specific component of the complex response to whole influenza vaccine represented a major subset of proliferating T helper cells. Soluble class II tetramers allow a direct approach for the analysis of immunodominant antigenic specificities. The identification of antigen-specific T helper cells in the peripheral blood provides a means for tracking the immune response against infectious agents and in autoimmune disease.

Authors

Erik J. Novak, Andrew W. Liu, Gerald T. Nepom, William W. Kwok

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Figure 3

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Phenotypic characterization of HA307–319 tetramer-specific cells. Nylon ...
Phenotypic characterization of HA307–319 tetramer-specific cells. Nylon wool–purified T cells were labeled with CFSE before culture with autologous adherent cells and antigen. On day 7, cells were stained with PE-labeled tetramer and then stained with combinations of fluorochrome-labeled anti-CD3, -CD4, -CD8, and -CD25 antibodies before flow-cytometry analysis. All panels are gated on tetramer-positive cells. Upper panels show CD8 versus CD4 staining in cells stimulated with (a) HA307–319 peptide, and (b) whole influenza vaccine, whereas lower panels show CD25 versus CD3 staining in cells stimulated with (c) HA307–319 peptide, and (d) whole influenza vaccine. Boundaries for positive and negative populations were determined by controls. Percentages shown in the margins of each panel represent the percent of total cells present in each quadrant. The panels depict results from a representative individual experiment.