Nonredundant antigen presentation by CD1c+ DCs infected with HIV and influenza virus. Nonredundant antigen presentation by CD1c+ DCs infected with HIV.

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Nonredundant antigen presentation by CD1c+ DCs infected with HIV and influenza virus. Nonredundant antigen presentation by CD1c+ DCs infected with HIV and influenza virus. (A) Stimulation of a CD8+ T cell line by infected DCs. Combined intracellular expression of macrophage inflammatory protein–1β, tumor necrosis factor–α (TNF-α), IFN-γ, and interleukin-2 by an SL9-specific CD8+ T cell line exposed to blood DCs infected for 48 hours by HIV-1SL9(BaL) Vpx (MOI = 0.8) alone or in the presence of viral inhibitors AZT and NVP (n = 3 donors combined from three independent experiments). (B) IFN-γ concentration in culture supernatants of M1- and NS1-specific CD8+ T cell lines exposed for 18 hours to DCs that were treated with or without chloroquine for 30 min and then pulsed with FluA(PR8) (MOI = 2) for 1 hour (n = 3 donors combined from three experiments). (C) Down-regulation of HLA-ABC in HIV-infected DCs. HLA-ABC expression in Gag+ and Gag– CD1c+ DCs 48 hours after infection with HIV-2(JK) nef+ (MOI = 1) or HIV-1(AD8) nef+ Vpx (MOI = 0.8) (n = 3). (D) GFP expression and viability in CD1c+ DCs at 4, 12, and 24 hours after infection with GFP-encoding influenza virus. (E) GFP expression and viability as in (D) (n = 4; three or four different donors combined from three independent experiments). (F) Down-regulation of HLA-ABC and CD86 in influenza virus-infected DCs. GFP, HLA-ABC, and CD86 expression in DAPI (4′,6-diamidino-2-phenylindole)–negative CD1c+ DCs analyzed before and 12 hours after infection with GFP-encoding influenza virus. (G) HLA-ABC expression as in (F) (n = 4; four different donors combined from three independent experiments). (H) CD86 expression as in (F) (n = 4; four different donors combined from three independent experiments). (I) T cell stimulation by infected versus bystander CD1c+ DCs. GFP expression in bulk CD1c+, sorted GFP+CD1c+, and GFP-CD1c+ DCs 24 hours after infection with GFP-encoding influenza virus (top). Carboxyfluorescein diacetate succinimidyl ester (CFSE) levels and FluM1-tetramer binding on CD8+ T cells after 7-day cocultures at 1:30 and 1:100 DC/T ratio (bottom). (J) Summary of the percentage of FluM1-tetramer binding CFSElow CD8+ T cells at 7 days after coculture as in (I) (n = 2; two different donors combined from two independent experiments). MFI, mean fluorescence intensity. *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001. Aymeric Silvin et al. Sci. Immunol. 2017;2:eaai8071 Copyright © 2017 The Authors, some rights reserved; exclusive licensee American Association for the Advancement of Science. No claim to original U.S. Government Works