Regulatory functions of CD8+CD28 T cells in an autoimmune disease model
Nader Najafian, Tanuja Chitnis, Alan D. Salama, Bing Zhu, Christina Benou, Xueli Yuan, Michael R. Clarkson, Mohamed H. Sayegh, Samia J. Khoury
Nader Najafian, Tanuja Chitnis, Alan D. Salama, Bing Zhu, Christina Benou, Xueli Yuan, Michael R. Clarkson, Mohamed H. Sayegh, Samia J. Khoury
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Article Autoimmunity

Regulatory functions of CD8+CD28 T cells in an autoimmune disease model

Abstract

CD8+ T cell depletion renders CD28-deficient mice susceptible to experimental autoimmune encephalomyelitis (EAE). In addition, CD8–/–CD28–/– double-knockout mice are susceptible to EAE. These findings suggest a role for CD8+ T cells in the resistance of CD28-deficient mice to disease. Adoptive transfer of CD8+CD28– T cells into CD8–/– mice results in significant suppression of disease, while CD8+CD28+ T cells demonstrate no similar effect on the clinical course of EAE in the same recipients. In vitro, CD8+CD28– but not CD8+CD28+ T cells suppress IFN-γ production of myelin oligodendrocyte glycoprotein–specific CD4+ T cells. This suppression requires cell-to-cell contact and is dependent on the presence of APCs. APCs cocultured with CD8+CD28– T cells become less efficient in inducing a T cell–dependent immune response. Such interaction prevents upregulation of costimulatory molecules by APCs, hence decreasing the delivery of these signals to CD4+ T cells. These are the first data establishing that regulatory CD8+CD28– T cells occur in normal mice and play a critical role in disease resistance in CD28–/– animals.

Authors

Nader Najafian, Tanuja Chitnis, Alan D. Salama, Bing Zhu, Christina Benou, Xueli Yuan, Michael R. Clarkson, Mohamed H. Sayegh, Samia J. Khoury

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Figure 8

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CD8+CD28– T cells induce suppression by modification of APCs. (a) APCs i...
CD8+CD28 T cells induce suppression by modification of APCs. (a) APCs incubated with CD8+CD28 T cells and Con A for at least 24 hours have significantly decreased capacity to stimulate BALB/c splenocytes (white bar) than APCs exposed to Con A and CD8+CD28+ T cells (black bar). (b) Mean decrease in percentage of APCs expressing CD40, B7-1, and B7-2 (y axis). CD11c+ cells conditioned by preculture with CD8+CD28 T cells for 24 hours in the presence of Con A were stained for expression of CD40, B7-1, and B7-2, and the percentage of positive cells was compared with CD11c+ cells precultured with CD8+CD28+ T cells. (c) Antigen-presenting capacity of APCs cocultured with CD8+CD28 T cells and MOG (white bar) as compared with that of APCs cocultured with CD8+CD28+ T cells and MOG for 24 hours (black bar). As expected, 100% purified primed CD4+ T cells are unable to respond to MOG in the absence of APCs (gray bar).