Figure 1
PDCs and CD11c+ DCs both induce extensive HCMV-dependent proliferation but different cytokine profiles in CD4+ memory T cells. PDCs or CD11c+ DCs were cocultured with autologous CFSE-labeled purified CD4+ T cells in the presence of HCMV (MOI of 5) or mock, as indicated. On day 6.5, accumulated proliferation was measured by flow cytometry as the percentage of CFSElow cells, gated on CD3+CD123− (PDC cultures) or CD3+CD11c− (CD11c+ DC cultures) cells. A representative experiment is shown in panel A. Proliferation was HCMV-dependent in cells from HCMV seropositive individuals (A-B) and was lower in cocultures with PDCs than with CD11c+ DCs (B; n = 7, *P < .001 relative to mock, **P < .05 relative to CD11c+ DC cultures). Only minor responses were observed in seronegative individuals (B; n = 3). Supernatants from the cocultures described in panels A and B were harvested following stimulation with HCMV on day 6.5 (C), or at 12, 24, and 48 hours (D). Cytokines were measured with CBA. (C) The IL-10 levels were 8.8 ± 2.2-fold higher in cultures with PDCs than with CD11c+ DCs, whereas the amounts of IFN-γ were 5.7 ± 1.6-fold higher in the cocultures containing CD11c+ DCs as opposed to PDCs (n = 12, *P < .05). (D) IL-10 was detected at 24 hours in the PDC cocultures, whereas IFN-γ was detected at 12 hours in the CD11c+ DC cocultures. One representative experiment of 2 is shown. (E) Cytokine production was measured by flow cytometry at the single-cell level in CD3+ T cells from DC–T-cell cocultures 24 hours subsequent to HCMV stimulation. One representative experiment of 3 is shown. Means and SEM are indicated in panels B and C.

PDCs and CD11c+ DCs both induce extensive HCMV-dependent proliferation but different cytokine profiles in CD4+ memory T cells. PDCs or CD11c+ DCs were cocultured with autologous CFSE-labeled purified CD4+ T cells in the presence of HCMV (MOI of 5) or mock, as indicated. On day 6.5, accumulated proliferation was measured by flow cytometry as the percentage of CFSElow cells, gated on CD3+CD123 (PDC cultures) or CD3+CD11c (CD11c+ DC cultures) cells. A representative experiment is shown in panel A. Proliferation was HCMV-dependent in cells from HCMV seropositive individuals (A-B) and was lower in cocultures with PDCs than with CD11c+ DCs (B; n = 7, *P < .001 relative to mock, **P < .05 relative to CD11c+ DC cultures). Only minor responses were observed in seronegative individuals (B; n = 3). Supernatants from the cocultures described in panels A and B were harvested following stimulation with HCMV on day 6.5 (C), or at 12, 24, and 48 hours (D). Cytokines were measured with CBA. (C) The IL-10 levels were 8.8 ± 2.2-fold higher in cultures with PDCs than with CD11c+ DCs, whereas the amounts of IFN-γ were 5.7 ± 1.6-fold higher in the cocultures containing CD11c+ DCs as opposed to PDCs (n = 12, *P < .05). (D) IL-10 was detected at 24 hours in the PDC cocultures, whereas IFN-γ was detected at 12 hours in the CD11c+ DC cocultures. One representative experiment of 2 is shown. (E) Cytokine production was measured by flow cytometry at the single-cell level in CD3+ T cells from DC–T-cell cocultures 24 hours subsequent to HCMV stimulation. One representative experiment of 3 is shown. Means and SEM are indicated in panels B and C.

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