MHC-derived allopeptide activates TCR-biased CD8+ Tregs and suppresses organ rejection
Elodie Picarda, … , Ignacio Anegon, Carole Guillonneau
Elodie Picarda, … , Ignacio Anegon, Carole Guillonneau
Published May 1, 2014
Citation Information: J Clin Invest. 2014;124(6):2497-2512. https://doi.org/10.1172/JCI71533.
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Research Article Immunology

MHC-derived allopeptide activates TCR-biased CD8+ Tregs and suppresses organ rejection

Abstract

In a rat heart allograft model, preventing T cell costimulation with CD40Ig leads to indefinite allograft survival, which is mediated by the induction of CD8+CD45RClo regulatory T cells (CD8+CD40Ig Tregs) interacting with plasmacytoid dendritic cells (pDCs). The role of TCR-MHC-peptide interaction in regulating Treg activity remains a topic of debate. Here, we identified a donor MHC class II–derived peptide (Du51) that is recognized by TCR-biased CD8+CD40Ig Tregs and activating CD8+CD40Ig Tregs in both its phenotype and suppression of antidonor alloreactive T cell responses. We generated a labeled tetramer (MHC-I RT1.Aa/Du51) to localize and quantify Du51-specific T cells within rat cardiac allografts and spleen. RT1.Aa/Du51-specific CD8+CD40Ig Tregs were the most suppressive subset of the total Treg population, were essential for in vivo tolerance induction, and expressed a biased, restricted Vβ11-TCR repertoire in the spleen and the graft. Finally, we demonstrated that treatment of transplant recipients with the Du51 peptide resulted in indefinite prolongation of allograft survival. These results show that CD8+CD40Ig Tregs recognize a dominant donor antigen, resulting in TCR repertoire alterations in the graft and periphery. Furthermore, this allopeptide has strong therapeutic activity and highlights the importance of TCR-peptide-MHC interaction for Treg generation and function.

Authors

Elodie Picarda, Séverine Bézie, Vanessa Venturi, Klara Echasserieau, Emmanuel Mérieau, Aurélie Delhumeau, Karine Renaudin, Sophie Brouard, Karine Bernardeau, Ignacio Anegon, Carole Guillonneau

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Figure 2

Analysis of CD8+CD45RClo Treg activation in response to donor-derived peptide stimulation.

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Analysis of CD8+CD45RClo Treg activation in response to donor-derived pe...
(A) CD8+ Tregs were cocultured for 6 days with syngeneic CpG-matured pDCs in the presence of peptides. For each experiment, the percentage of CD25+ Tregs after 6 days of coculture with pDCs alone was given a value of 1. The mean value of 1 is equal to 32.85 ± 1.98%. Results are expressed as the ratio ± SEM between the percentage of CD25+ cells after peptide stimulation and the percentage of CD25+ cells in the control condition without peptide. *P < 0.05, **P < 0.01, and ***P < 0.001 versus control condition (value 1.0). n = 4–18 for each peptide. (B) Analysis of Treg activation in response to Du51 shorter peptide derivatives. On the left, 18 Du51 derivatives are detailed and classified by aa sequence length, from 9 aa to 15 aa. The box highlights mismatched aa between the donor and recipient. On the right, Treg activation in response to Du51 derivatives was analyzed by CD25 expression. CD8+ Tregs were cocultured for 6 days with syngeneic CpG-matured pDCs in the presence of each peptide. Bars represent the ratio between the percentage of CD25+ cells after peptide stimulation and the percentage of CD25+ cells in the control condition without peptide. *P < 0.05, **P < 0.01, and ***P < 0.001 versus Du51 condition. n = 3–14 for each peptide.