Alloantigen-specific regulatory T cells generated with a chimeric antigen receptor
Katherine G. MacDonald, … , Raewyn Broady, Megan K. Levings
Katherine G. MacDonald, … , Raewyn Broady, Megan K. Levings
Published March 21, 2016
Citation Information: J Clin Invest. 2016;126(4):1413-1424. https://doi.org/10.1172/JCI82771.
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Technical Advance Immunology

Alloantigen-specific regulatory T cells generated with a chimeric antigen receptor

Abstract

Adoptive immunotherapy with regulatory T cells (Tregs) is a promising treatment for allograft rejection and graft-versus-host disease (GVHD). Emerging data indicate that, compared with polyclonal Tregs, disease-relevant antigen-specific Tregs may have numerous advantages, such as a need for fewer cells and reduced risk of nonspecific immune suppression. Current methods to generate alloantigen-specific Tregs rely on expansion with allogeneic antigen-presenting cells, which requires access to donor and recipient cells and multiple MHC mismatches. The successful use of chimeric antigen receptors (CARs) for the generation of antigen-specific effector T cells suggests that a similar approach could be used to generate alloantigen-specific Tregs. Here, we have described the creation of an HLA-A2–specific CAR (A2-CAR) and its application in the generation of alloantigen-specific human Tregs. In vitro, A2-CAR–expressing Tregs maintained their expected phenotype and suppressive function before, during, and after A2-CAR–mediated stimulation. In mouse models, human A2-CAR–expressing Tregs were superior to Tregs expressing an irrelevant CAR at preventing xenogeneic GVHD caused by HLA-A2+ T cells. Together, our results demonstrate that use of CAR technology to generate potent, functional, and stable alloantigen-specific human Tregs markedly enhances their therapeutic potential in transplantation and sets the stage for using this approach for making antigen-specific Tregs for therapy of multiple diseases.

Authors

Katherine G. MacDonald, Romy E. Hoeppli, Qing Huang, Jana Gillies, Dan S. Luciani, Paul C. Orban, Raewyn Broady, Megan K. Levings

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Figure 3

A2-CAR–mediated stimulation activates Tregs.

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A2-CAR–mediated stimulation activates Tregs. (A) Signaling downstream of...
(A) Signaling downstream of TCR or CAR stimulation was assessed in A2-CAR Tregs and Tconvs loaded with αCD3 (TCR) or αMyc (CAR) mAbs, which were then crosslinked by addition of αIgG. Cells were fixed at 0, 5, 10, and 20 minutes and stained for phosphorylated ZAP70 (n = 4). (BD) A2-CAR Tregs or Tconvs were stimulated with K562.64 cells loaded with αCD3/28 mAbs (TCR stim) or expressing HLA-A2 (CAR stim) (n = 4). After 1 day, T cells were assayed for expression of (B) CD69 and CD154, (C) CTLA-4, and (D) membrane-bound TGF-β (LAP) and GARP. Gates were set based on unstimulated controls. (E) After 48 hours, cytokine production upon A2-CAR stimulation was measured by cytometric bead array (n = 2). Averaged data represent mean ± SEM. Significance determined by 2-way ANOVA. *P < 0.05; **P < 0.01; ***P < 0.001.