CD3 downregulation identifies high-avidity, multipotent SARS-CoV-2 vaccine– and recall antigen–specific Th cells with distinct metabolism
Arne Sattler, Stefanie Gamradt, Vanessa Proß, Linda Marie Laura Thole, An He, Eva Vanessa Schrezenmeier, Katharina Jechow, Stefan M. Gold, Sören Lukassen, Christian Conrad, Katja Kotsch
Arne Sattler, Stefanie Gamradt, Vanessa Proß, Linda Marie Laura Thole, An He, Eva Vanessa Schrezenmeier, Katharina Jechow, Stefan M. Gold, Sören Lukassen, Christian Conrad, Katja Kotsch
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Research Article Immunology Vaccines

CD3 downregulation identifies high-avidity, multipotent SARS-CoV-2 vaccine– and recall antigen–specific Th cells with distinct metabolism

Abstract

Functional avidity is supposed to critically shape the quality of immune responses, thereby influencing host protection against infectious agents including SARS-CoV-2. Here we show that after human SARS-CoV-2 vaccination, a large portion of high-avidity spike-specific CD4+ T cells lost CD3 expression after in vitro activation. The CD3– subset was enriched for cytokine-positive cells, including elevated per-cell expression levels, and showed increased polyfunctionality. Assessment of key metabolic pathways by flow cytometry revealed that superior functionality was accompanied by a shift toward fatty acid synthesis at the expense of their oxidation, whereas glucose transport and glycolysis were similarly regulated in SARS-CoV-2–specific CD3– and CD3+ subsets. As opposed to their CD3+ counterparts, frequencies of vaccine-specific CD3– T cells positively correlated with both the size of the naive CD4+ T cell pool and vaccine-specific IgG levels. Moreover, their frequencies negatively correlated with advancing age and were impaired in patients under immunosuppressive therapy. Typical recall antigen–reactive T cells showed a comparable segregation into functionally and metabolically distinct CD3+ and CD3– subsets but were quantitatively maintained upon aging, likely due to earlier recruitment in life. In summary, our data identify CD3– T helper cells as correlates of high-quality immune responses that are impaired in at-risk populations.

Authors

Arne Sattler, Stefanie Gamradt, Vanessa Proß, Linda Marie Laura Thole, An He, Eva Vanessa Schrezenmeier, Katharina Jechow, Stefan M. Gold, Sören Lukassen, Christian Conrad, Katja Kotsch

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Figure 6

Functional and metabolic assessment of CEF-specific CD3CD4+ and CD3+CD4+ Th cell subsets.

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Functional and metabolic assessment of CEF-specific CD3–CD4+ and CD3+CD4...
PBMCs were stimulated or not with CEF peptide mix for 16 hours. Specific CD4+ Th cells were identified as before and further assessed intracellularly for cytokine production. (A) Frequencies (left, n = 42) and expression levels (right, n = 42) of IFN-γ+ T cell subsets specific for CEF. (B) Frequencies of TNF-α– (left), IL-2– (middle), or IL-4– (right) expressing CEF-specific T cells and (C) those of IFN-γ–, TNF-α–, and IL-2– coexpressing polyfunctional T cells. n = 41 for all analyses. Statistical analysis with paired, 2-tailed t test (A, left, B, middle) or paired, 2-tailed Wilcoxon test (remaining graphs). (D) Expression levels (according to MFI) of the indicated key metabolic proteins were analyzed in CEF-specific (CD154+CD137+) CD3+CD4+ versus CD3CD4+ T cells versus nonspecific CD154CD137CD3+CD4+ bulk control T cells within the same sample. n = 7 (upper panels) and 9 (lower panels); statistical analyses were performed using paired 1-way ANOVA (ACAC, CPT1a, IDH2, G6PD, LDH, ATP5a) or Friedman test (GLUT1, HK2). Where applicable, graphs show means ± SD.