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T-cell activation and receptor downmodulation precede deletion induced by mucosally administered antigen
Jacqueline M. Benson, … , Thomas Forsthuber, Caroline C. Whitacre
Jacqueline M. Benson, … , Thomas Forsthuber, Caroline C. Whitacre
Published October 15, 2000
Citation Information: J Clin Invest. 2000;106(8):1031-1038. https://doi.org/10.1172/JCI10738.
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Article

T-cell activation and receptor downmodulation precede deletion induced by mucosally administered antigen

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Abstract

The fate of antigen-specific T cells was characterized in myelin basic protein (MBP) T-cell receptor (TCR) transgenic (Tg) mice after oral administration of MBP. Peripheral Th cells are immediately activated in vivo, as indicated by upregulation of CD69 and increased cytokine responses (Th1 and Th2). Concurrently, surface TCR expression diminishes and internal TCR levels increase. When challenged for experimental autoimmune encephalomyelitis during TCR downmodulation, Tg mice are protected from disease. To characterize Th cells at later times after antigen feeding, it was necessary to prevent thymic release of naive Tg cells. Therefore, adult Tg mice were thymectomized before treatment. TCR expression returns in thymectomized Tg mice 3 days after MBP feeding and then ultimately declines in conjunction with MBP-specific proliferation and cytokine responses (Th1-type and Th2-type). The decline correlates with an increase in apoptosis. Collectively, these results demonstrate that a high dose of fed antigen induces early T-cell activation and TCR downmodulation, followed by an intermediate stage of anergy and subsequent deletion.

Authors

Jacqueline M. Benson, Kim A. Campbell, Zhen Guan, Ingrid E. Gienapp, Scott S. Stuckman, Thomas Forsthuber, Caroline C. Whitacre

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Figure 5

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The number of Vβ8+/CD4+ Tg T cells declines after MBP feeding. Euthymic ...
The number of Vβ8+/CD4+ Tg T cells declines after MBP feeding. Euthymic and thymectomized MBP TCR Tg mice were fed 100 mg MBP and sacrificed 1, 3, 7, 10, and 14 days after feeding. Cells were analyzed by flow cytometry for the Tg Vβ8 TCR on CD4+ cells. Each bar is the mean percentage of Vβ8+/CD4+ cells ± SEM (n = 3–5). AValues are statistically different from corresponding control-fed mice at P ≤ 0.05.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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