TCR stimulation with modified anti-CD3 mAb expands CD8+ T cell population and induces CD8+CD25+ Tregs
Brygida Bisikirska, … , Jeffrey A. Bluestone, Kevan C. Herold
Brygida Bisikirska, … , Jeffrey A. Bluestone, Kevan C. Herold
Published October 3, 2005
Citation Information: J Clin Invest. 2005;115(10):2904-2913. https://doi.org/10.1172/JCI23961.
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Research Article Immunology

TCR stimulation with modified anti-CD3 mAb expands CD8+ T cell population and induces CD8+CD25+ Tregs

Abstract

Modified anti-CD3 mAbs are emerging as a possible means of inducing immunologic tolerance in settings including transplantation and autoimmunity such as in type 1 diabetes. In a trial of a modified anti-CD3 mAb [hOKT3γ1(Ala-Ala)] in patients with type 1 diabetes, we identified clinical responders by an increase in the number of peripheral blood CD8+ cells following treatment with the mAb. Here we show that the anti-CD3 mAb caused activation of CD8+ T cells that was similar in vitro and in vivo and induced regulatory CD8+CD25+ T cells. These cells inhibited the responses of CD4+ cells to the mAb itself and to antigen. The regulatory CD8+CD25+ cells were CTLA4+ and Foxp3+ and required contact for inhibition. Foxp3 was also induced on CD8+ T cells in patients during mAb treatment, which suggests a potential mechanism of the anti-CD3 mAb immune modulatory effects involving induction of a subset of regulatory CD8+ T cells.

Authors

Brygida Bisikirska, John Colgan, Jeremy Luban, Jeffrey A. Bluestone, Kevan C. Herold

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The CD8+CD25+ cells induced with hOKT3γ1(Ala-Ala) suppress CD4 cell resp...
The CD8+CD25+ cells induced with hOKT3γ1(Ala-Ala) suppress CD4 cell response to SEB and IFN-γ secretion. (A) CD8+CD25+ or CD8+CD25 cells sorted from PBMCs stimulated for 6 days with hOKT3γ1(Ala-Ala) or CD8+ cells from fresh PBMCs were irradiated and cocultured for 3 days with fresh PBMCs depleted of CD8 in the presence of SEB. Proliferative response was assessed by [3H]thymidine uptake. (B) The levels of IFN-γ in the supernatants from the same cultures were measured by Luminex system using Th1/Th2 multiplex microspheres. Representative results of 2 independent experiments are shown. (C) Sorted CD8+CD25+ (bottom panel) or untreated CD8 cells (upper panel) were cocultured for 6 days with CFSE-labeled, CD8-depleted PBMCs at 1:2 ratio in the presence of SEB. SEB-specific clonal expansion was analyzed by flow cytometry. The expansion of Vβ3-positive CD4 (M1) lymphocytes was reduced from 46.1% to 15.5% of Vβ3+ T cells. Similar results were obtained in 2 additional studies.