T cells presenting viral antigens or autoantigens induce cytotoxic T cell anergy
Nathalie E. Blachère, Dana E. Orange, Emily C. Gantman, Bianca D. Santomasso, Graeme C. Couture, Teresa Ramirez-Montagut, John Fak, Kevin J. O’Donovan, Zhong Ru, Salina Parveen, Mayu O. Frank, Michael J. Moore, Robert B. Darnell
Nathalie E. Blachère, Dana E. Orange, Emily C. Gantman, Bianca D. Santomasso, Graeme C. Couture, Teresa Ramirez-Montagut, John Fak, Kevin J. O’Donovan, Zhong Ru, Salina Parveen, Mayu O. Frank, Michael J. Moore, Robert B. Darnell
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Research Article Immunology Oncology

T cells presenting viral antigens or autoantigens induce cytotoxic T cell anergy

Abstract

In the course of modeling the naturally occurring tumor immunity seen in patients with paraneoplastic cerebellar degeneration (PCD), we discovered an unexpectedly high threshold for breaking CD8+ cytotoxic T cell (CTL) tolerance to the PCD autoantigen, CDR2. While CDR2 expression was previously found to be strictly restricted to immune-privileged cells (cerebellum, testes, and tumors), unexpectedly we have found that T cells also express CDR2. This expression underlies inhibition of CTL activation; CTLs that respond to epithelial cells expressing CDR2 fail to respond to T cells expressing CDR2. This was a general phenomenon, as T cells presenting influenza (flu) antigen also fail to activate otherwise potent flu-specific CTLs either in vitro or in vivo. Moreover, transfer of flu peptide–pulsed T cells into flu-infected mice inhibits endogenous flu-specific CTLs. Our finding that T cells serve as a site of immune privilege, inhibiting effector CTL function, uncovers an autorepressive loop with general biologic and clinical relevance.

Authors

Nathalie E. Blachère, Dana E. Orange, Emily C. Gantman, Bianca D. Santomasso, Graeme C. Couture, Teresa Ramirez-Montagut, John Fak, Kevin J. O’Donovan, Zhong Ru, Salina Parveen, Mayu O. Frank, Michael J. Moore, Robert B. Darnell

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Figure 2

CDR2 expression in WT mice limits the generation of humoral and cellular immune responses to CDR2.

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CDR2 expression in WT mice limits the generation of humoral and cellular...
(A) Western blots of serum from Cdr2-KO or WT mice immunized with β-gal or CDR2 and tested for the presence of IgG 21 days later. Left panel: CDR2 resolved by SDS-PAGE. Right panel: β-Gal resolved by SDS-PAGE. One experiment is shown and is representative of 2 experiments. (B) CD4+ T cell proliferation as measured by 3H-thymidine incorporation from unimmunized or CDR2-immunized Cdr2-KO mice stimulated with candidate CDR2 peptide–pulsed Cdr2-KO splenocytes. Each triangle represents CD4+ T cells from 2 mice pooled and plated in triplicate wells and is representative of 3 experiments. (C) IFN-γ ELISPOT assay of CD4+ T cells from Cdr2-KO (n = 2) or WT hosts (n = 2) immunized with both AdV-β-gal and AdV-CDR2 and cultured with Cdr2-KO splenocytes pulsed with various peptides. Each triangle is the mean of triplicate wells of CD4+ T cells from 1 mouse and is representative of 3 experiments. (D) IFN-γ ELISPOT assay of CD8+ T cells from Cdr2-KO or WT hosts immunized with AdV-Trk or AdV-CDR2. Each triangle represents CD8+ T cells from 2 mice pooled and plated in triplicate wells and is representative of 3 experiments. *P < 0.05, ***P < 0.001; ns, statistically not significant as calculated using unpaired Student’s t test. AdV, adenovirus; Cpm, counts per minute; SFC, spot-forming cells; OVA, ovalbumin peptide.