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Stability of the Regulatory T Cell Lineage in Vivo

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Science  24 Sep 2010:
Vol. 329, Issue 5999, pp. 1667-1671
DOI: 10.1126/science.1191996

Abstract

Tissue maintenance and homeostasis can be achieved through the replacement of dying cells by differentiating precursors or self-renewal of terminally differentiated cells or relies heavily on cellular longevity in poorly regenerating tissues. Regulatory T cells (Treg cells) represent an actively dividing cell population with critical function in suppression of lethal immune-mediated inflammation. The plasticity of Treg cells has been actively debated because it could factor importantly in protective immunity or autoimmunity. By using inducible labeling and tracking of Treg cell fate in vivo, or transfers of highly purified Treg cells, we have demonstrated notable stability of this cell population under physiologic and inflammatory conditions. Our results suggest that self-renewal of mature Treg cells serves as a major mechanism of maintenance of the Treg cell lineage in adult mice.

Continuous replacement of differentiated cells within some tissues, such as the gut epithelium, is achieved by their de novo generation from a pool of precursor cells (1), whereas other tissues with reduced regenerative and proliferative capacity, such as the central nervous system, largely rely on cellular longevity for maintenance. Replication and self-renewal of differentiated cells, as shown for pancreatic β-cells, represents another potential mechanism underlying tissue maintenance (2). The latter strategy raises the issue of stability versus plasticity of a differentiated state, which is of particular importance for the proliferating cells of the immune system. Regulatory T cells (Treg cells), defined by expression of the transcription factor Foxp3, represent a dedicated suppressor cell type whose maintenance is required throughout life to restrain fatal autoimmunity (37). The instability of the Treg cell fate—their ability to further differentiate into diverse effector T cell (Teff cell) types—remains controversial. Many Treg cells express T cell receptors (TCRs) with heightened affinity for self-peptide major histocompatibility complexes (MHCs) (811), and ablation of a conditional Foxp3 allele in mature Treg cells results in generation of “former” Treg cells that are capable of causing inflammatory tissue lesions (12). Thus, the stability of Foxp3 expression under basal and inflammatory conditions is an important determinant of immune homeostasis and of immediate relevance to the question of whether Treg cells represent a distinct, stable cell lineage or a transient meta-stable activation state. Genetic fate mapping provides means to evaluate both lineage stability and informs mechanisms of tissue maintenance in vivo.

We used this approach to evaluate Treg cell lineage stability under basal and inflammatory conditions and generated knock-in mice harboring a cassette containing an internal ribosome entry site (IRES) followed by DNA sequence encoding a “triple” fusion protein of the enhanced green fluorescent protein (eGFP) with Cre recombinase and mutated human estrogen receptor ligand-binding domain (ERT2) inserted into the 3′ untranslated region (UTR) of the Foxp3 gene (13). The Foxp3eGFP-Cre-ERT2 mice were bred to mice that expressed a Cre recombination reporter allele of the ubiquitously expressed ROSA26 locus containing a loxP site–flanked STOP cassette followed by a DNA sequence encoding yellow fluorescent protein (YFP) (R26Y) (fig. S1). In the Foxp3eGFP-Cre-ERT2 × R26Y mice, the GFP-CreERT2 fusion protein is sequestered in the cytosol, and therefore YFP is not expressed; but treatment with tamoxifen allows for nuclear translocation of the fusion protein, excision of the floxed STOP cassette, and constitutive and heritable expression of YFP in a cohort of cells that expressed Foxp3 at the time of tamoxifen administration. In contrast to continuous labeling, inducible labeling of Foxp3-expressing cells with YFP avoids the constant incorporation into the labeled population of cells that transiently up-regulate Foxp3 and affords assessment of bona fide Treg cell maintenance.

Foxp3eGFP-Cre-ERT2 × R26Y mice had normal numbers of CD4 and CD8 double- and single-positive thymocytes and CD4+ and CD8+ T cells in the secondary lymphoid organs (fig. S2). Foxp3 and the associated eGFP reporter were expressed in a manner indistinguishable from expression of the Foxp3 protein in control wild-type mice, and eGFP expression was limited to Foxp3+ cells (figs. S2 and S3A). YFP was not detected in eGFP+ cells in the absence of tamoxifen and was restricted to Foxp3+ cells upon tamoxifen administration (fig. S3, B and C). Treatment with tamoxifen resulted in three main populations of CD4+ T cells: eGFPYFP–Foxp3 “non-Treg” cells, eGFP+YFP unlabeled Foxp3+ Treg cells, and tagged eGFP+YFP+ Foxp3+ cells (fig. S4). We also observed a minor population of eGFPYFP+ cells (<5% of YFP+ cells), which may represent cells that were transiently expressing Foxp3 at the time of tamoxifen exposure. Both YFP-tagged and -untagged eGFP+ Treg cells expressed identical amounts of Foxp3 and all other Treg cell phenotypic and activation markers tested thus far (figs. S4 and S5).

To evaluate long-term stability of Foxp3+ Treg cells under basal conditions, Foxp3eGFP-Cre-ERT2 × R26Y mice were treated with tamoxifen and analyzed 5 to 8 months later for Foxp3 expression in YFP+CD4+ T cells. The overwhelming majority of YFP+CD4+ T cells remained eGFP-positive in the lymph nodes, spleen, Peyer’s patches, skin, and lung up to 5 months after tamoxifen treatment (Fig. 1, A and B). This result was confirmed by means of intracellular staining for Foxp3 of fluorescence-activated cell sorter (FACS)–purified YFP+ cells (fig. S6). Furthermore, expression of Treg cell–associated molecules was comparable between YFP+ and YFP+GFP+ cells (Fig. 1C and fig. S6), and production of proinflammatory cytokines was comparably low in both subsets (Fig. 1D). The minor population of eGFPYFP+ cells observed 14 days after labeling failed to expand and in fact further decreased over time (Fig. 1, C and D). Thus, we did not observe a noticeable “conversion” of Treg cells and their progeny into follicular T helper (TFH) or effector T cells or their dedifferentiation into naïve T cells under physiologic conditions.

Fig. 1

Inducible labeling of Foxp3+ cells reveals stability of Treg cell subset under physiologic conditions. (A) Representative flow-cytometric analyses demonstrate stability of Foxp3 expression at 14 days and 5 months after tamoxifen-induced labeling. YFP+, YFPGFP+, and YFPGFP subsets of CD4+ T cells and proportion of GFP+ cells among YFP-tagged cells are shown. Numbers represent percentages of cells within the indicated gates. (B) Percentages of YFP+ cells expressing GFP in the indicated organs analyzed as in (A) at 5 months after tamoxifen administration (bottom). Each symbol represents an individual mouse. (C) Flow cytometric analysis of CD25 expression in CD4+ cell subsets at 5 months after initial tamoxifen treatment. Expression of CD25 within the indicated subset is shown for individual mice. (D) Splenocytes from Foxp3eGFP-Cre-ERT2 × R26Y mice were isolated 5 months after tamoxifen administration and stimulated with phorbol 12-myristate 13-acetate and ionomycin in vitro, and production of IFNγ and IL-2 was assessed by means of flow cytometry. Expression of IFNγ and IL-2 in YFP+Foxp3+, YFPFoxp3+, and YFPFoxp3subsets is shown. (E) Proportion of YFP-labeled cells among Foxp3+ cells in the periphery of thymectomized and nonthymectomized Foxp3eGFP-Cre-ERT2 × R26Y mice at 14 days and 5 months after tamoxifen treatment. Atx, adult thymectomy. Data are representative of three independent experiments (n ≥ 3 mice per group). Mice were 6 to 8 weeks of age at the time of labeling.

Surprisingly, in euthymic mice the proportion of YFP+ Treg cells among all Foxp3+ cells at 5 to 8 months after labeling was comparable with that observed at 14 days despite continuous, albeit declining with age, output of thymus-derived Treg cells (Fig. 1E). Furthermore, thymectomy failed to influence the proportion of YFP+ Treg cells among Foxp3+ cells at these later time points (Fig. 1E), suggesting that the peripheral Treg cell pool, which is characterized by a high proportion of cycling cells (fig. S7), is not only highly stable in adult mice but is largely self-sustained with a relatively minor contribution by newly generated thymic emigrants.

We next asked whether Foxp3 can be lost upon growth factor deprivation as a validation of our Treg cell–fate tracking approach. Foxp3 induction and Treg cell homeostasis are dependent upon interleukin-2 (IL-2) receptor signaling (1419), and antibody-mediated blockade of IL-2 or IL-2R causes contraction of the Treg cell population (16). Thus, we sought to explore whether IL-2 deprivation of mature Treg cells is associated with death or loss of Foxp3 expression and concomitant acquisition of immune effector cytokine production. Tamoxifen-treated Foxp3eGFP-Cre-ERT2 × R26Y mice were treated with IL-2–neutralizing antibody. IL-2 deprivation resulted in a ~30% decrease in total Foxp3+ Treg cell numbers and a modest decrease in Foxp3 protein amounts at the single-cell level (Fig. 2, A to C). Moreover, a small subset of YFP+ cells was completely devoid of Foxp3. We did not, however, observe derepression of proinflammatory cytokines [interferon-γ (IFNγ), IL-17, IL-2, and tumor necrosis factor–α (TNFα)] by YFP+, YFPGFP+ Treg cells with decreased Foxp3 levels, or eGFPYFP+ cells which had lost Foxp3 expression (fig. S8). These results demonstrate that upon IL-2 deprivation, the bulk of Treg cells maintained Foxp3 expression albeit at a moderately decreased level, yet sufficient to prevent acquisition of an effector cell phenotype. Nevertheless, it is possible that IL-2 deprivation under conditions of overwhelming infection might result in a loss of Foxp3 in some Treg cells (20).

Fig. 2

IL-2 deprivation results in a small but detectable decrease in Foxp3 expression. (A to C) Tamoxifen-treated Foxp3eGFP-Cre-ERT2 × R26Y mice were injected with IL-2–blocking antibody or control immunoglobulin G (IgG), and Foxp3 expression in FACS-sorted YFP+ cells was assessed 9 days later. (A) Intracellular Foxp3 staining of splenic YFP+ cells. Numbers represent percentages of cells in the indicated gate. (B) Percentages of YFP+ cells expressing Foxp3. Each symbol represents an individual mouse. (C) Relative expression of Foxp3 in YFP+ cells from spleens of mice treated with IL-2–blocking antibody. Data are representative of three independent experiments (n ≥ 2 mice per group). Mice were 6 to 8 weeks of age at the time of antibody administration. (D to F) Treg cells maintain stable expression of Foxp3 under lymphopenic conditions. Lymphopenia was induced in tamoxifen-treated Foxp3eGFP-Cre-ERT2 × R26Y mice upon irradiation (6 Gy), and mice were analyzed 14 days later. (D) Representative flow-cytometric analysis of Foxp3 expression among cells isolated from spleens of control and irradiated mice 14 days after irradiation. Numbers represent percentages of cells in the indicated gate. (E) Percentages of GFP+ cells among YFP+ cells in spleens 14 days after irradiation. Each symbol represents an individual mouse. (F) Representative flow-cytometric analysis of Foxp3 and Ki67 expression by YFP+ splenocytes on day 14 after irradiation. Similar data were obtained from cells isolated from lymph nodes of irradiated mice. Data are representative of ≥2 independent experiments, each with ≥2 mice per group. Mice were 8 to 12 weeks of age at the time of irradiation.

Lymphopenia may also facilitate loss of Foxp3 expression in expanding Treg cells. Despite use of purified Treg cells in previously published transfer studies, the possibility of outgrowth of a small number of contaminating non-Treg cells and stress associated with cell transfer remain potential caveats in interpretation of these results. To circumvent these issues, we used sublethal irradiation to evaluate stability of Foxp3 expression under lymphopenic conditions. Tamoxifen-treated Foxp3eGFP-Cre-ERT2 × R26Y mice were irradiated (6 Gy), and the proportion of eGFP+ and Foxp3+ cells among YFP+CD4+ T cells was evaluated 14 days after irradiation. Despite a marked increase in numbers of dividing Treg cells reflected in heightened expression of Ki67 in YFP+ and YFPTreg cells, GFP and Foxp3 expression was preserved in YFP+ cells (Fig. 2, D to F). We considered that perturbation of the 3′UTR in Foxp3eGFP-Cre-ERT2 × R26Y mice may have resulted in increased Foxp3 mRNA or protein stability. However, Foxp3 mRNA decay in the presence of actinomycin D in Treg cells from Foxp3eGFP-Cre-ERT2 × R26Y mice was more pronounced than that in Treg cells from the previously described Foxp3GFP mice, in which GFP sequence was inserted into the 5′ end of the Foxp3 coding sequence, leaving the 3′UTR intact (fig. S9) (4). To compare the stability of Foxp3 protein expression in Treg cells from Foxp3eGFP-Cre-ERT2 × R26Y mice with that in Foxp3GFP mice in vivo, CD4+GFP+ cells were doubly purified by means of FACS from each mouse strain and cotransferred with Ly5.1+CD4+ T cells into TCRβδ-deficient mice. Three weeks after transfer, the majority (~90%) of CD4+Ly5.2+ cells maintained GFP and Foxp3 protein expression, and their percentages among cells transferred from both mouse strains were similar (fig. S10), further supporting the stability of the Treg cell lineage and indicating that the modification of the 3′UTR in Foxp3eGFP-Cre-ERT2 × R26Y mice cannot account for this observation.

Previous studies suggested that during infection, exposure of Treg cells to pro-inflammatory cytokines results in a loss of Foxp3 expression and Treg cell conversion into effector T cells and was interpreted as a means to facilitate appropriate immune responsiveness (21). To examine the fate of Foxp3+ Treg cells during infection, Foxp3eGFP-Cre-ERT2 × R26Y mice were treated with tamoxifen, infected with a sublethal dose of Listeria monocytogenes, and analyzed for Treg cell stability at the peak of the immune response. After infection, we observed considerable up-regulation of the T helper 1 transcription factor T-bet and CXCR3 in Foxp3, Foxp3+, and YFP+ CD4+ cells (Fig. 3, A and B, and fig. S11) and IFNγ production by effector CD4+ T cells in response to listeriolysin O (LLO) peptide (Fig. 3C and fig. S11). Nevertheless, essentially all YFP+ Treg cells maintained expression of Foxp3 (Fig. 3D), including those with increased T-bet expression. Foxp3 stability was also observed in T-bet+Foxp3+ cells generated upon induction of a strong IFNγ-dominated Th1 inflammatory response upon antibody-mediated cross-linking of CD40 (fig. S12) (22). Cross-linking of CD40 after tamoxifen-induced labeling resulted in a marked up-regulation of T-bet and CXCR3 in Foxp3+ and Foxp3 cells (fig. S12). YFP-tagged cells demonstrated increased expression of CXCR3 and T-bet but at best marginally increased IFNγ and IL-2 production (fig. S12). Furthermore, Treg cells maintained expression of Foxp3 at 14 days and up to 5 months after CD40 cross-linking (fig. S12). Thus, Treg cells maintain heritable Foxp3 expression even after up-regulation of the Th1 transcription factor T-bet in the course of Th1-dependent antibacterial infection and CD40 cross-linking driven Th1 inflammatory response. T-bet and CXCR3 induction in Treg cells was recently shown to facilitate their ability to restrain Th1 inflammation (22).

Fig. 3

Th1-type inflammation does not induce loss of Foxp3. Tamoxifen-treated Foxp3eGFP-Cre-ERT2 × R26Y mice were infected intravenously with 5 × 103 colony-forming units (CFU) of Listeria monocytogenes and analyzed 9 days later. (A) Flow-cytometric analysis demonstrates up-regulation of T-bet and CXCR3 by splenic YFP+CD4+ cells in infected mice. (B) Percent of T-bet positive cells among Foxp3 and YFP+ splenocytes as determined in (A). Each symbol represents an individual mouse. (C) Antigen-specific production of IFNγ in splenocytes restimulated with LLO190-201 peptide. CD4+ T cell gate is shown; numbers represent percentages of cells in corresponding quadrants. (D) Foxp3 expression in sorted (top) YFPGFP+ or (bottom) YFP+ cells from L. monocytogenes infected or control mice 9 days after infection. Data are representative of three independent experiments with ≥2 mice per group each. Mice were 6 to 8 weeks of age at the time of infection.

Lastly, to evaluate the stability of Foxp3+ cells in an autoimmune inflammatory setting, highly purified pancreatic-islet-antigen–specific GFP+ Treg cells from NOD.Foxp3gfp.BDC2.5 TCR-transgenic mice (23) were transferred into prediabetic, lymphoreplete NOD.Thy1.1 recipients at 12 weeks of age, a time point at which pancreatic infiltration is well established. Four weeks later, donor cells were enriched in the inflamed pancreas but retained expression of Foxp3 and, in contrast to recipient effector cells, expressed no detectable IL-17 or IFNγ (Fig. 4, A to C). In parallel experiments, Treg cell stability was evaluated in the K/BxN TCR-transgenic model, in which reactivity to a ubiquitous self-antigen leads IL-17– and gut microbiota–dependent generation of arthritogenic auto-antibodies (24). Highly purified GFP+ Treg cells from K/BxN.Foxp3gfp mice were transferred into 20-day-old K/BxN recipients—at the initiation of the very robust inflammatory process—and again remained almost exclusively Foxp3+ and failed to produce IL-17 in lymphoid organs or the lamina propria (Fig. 4, D to F). Thus, Treg cells maintained stable Foxp3 expression and showed no evidence of effector cytokine production under conditions of autoimmune inflammation.

Fig. 4

Foxp3 expression is stable in Treg cells during autoimmune inflammation. (A to C) Highly purified GFP+ cells from BDC2.5.Foxp3eGFP mice were transferred into 12-week-old prediabetic NOD.Thy1.1 recipients, and the spleen, pancreatic lymph nodes (PLN), or pancreatic infiltrates were analyzed 4 weeks later. (A) Representative Foxp3 staining of Thy1.2+CD4+ donor cells. (B) Tabulation of individual mice in three independent experiments. (C) Intracellular IFNγ and IL-17 staining of host and donor CD4+ cells (numbers represent percentage of cells in the gate ± SD; n = 3 to 6 mice per group). (D to F) Highly purified CD4+GFP+ cells from 20-day-old K/BxN.Foxp3gfp mice were transferred into age-matched K/BxN.CD45.2 mice. (D) Spleen, joint-draining lymph node, and small intestine lamina propria (LP) were collected from arthritic 35-day-old recipients and CD45.1+CD4+ donor cells analyzed for Foxp3-GFP expression. (E) Tabulation of individual mice in two independent experiments. (F) Expression of IL-17a by host and donor CD4+ cells from the lamina propria (numbers represent percentage of cells in the gate ± SD; n = 3 mice per group). Data are representative of two independent experiments.

In contrast to our findings, a recent study reported a marked loss of Foxp3 expression in YFP-tagged Foxp3+ Treg cells in R26Y × Foxp3-Cre BAC transgenic mice and acquisition of effector function by YFP+Foxp3 T cells (25). Likewise, upon transfer into lymphopenic recipients Foxp3+ Treg cells were found to lose Foxp3 expression and differentiate into TFH cells in the Peyer’s patches (26). Seemingly unstable Foxp3 expression observed in these and other studies (21) can be due to cellular stress, the presence of few contaminating Foxp3 cells or cells which underwent transient Foxp3 up-regulation, or recently generated Foxp3+ cells on their way to stable Foxp3 expression yet still able to expand and differentiate into effector T cells in lymphopenic or nonlymphopenic settings. Consistent with the latter notion, loss of Foxp3 expression by a minor population of YFP+ cells was observed during induction of Foxp3 in peripheral YFPGFPCD4+ T cells under lymphopenic conditions. In contrast, YFP+GFP+ Treg cells maintained Foxp3 expression in these experiments (fig. S13). Furthermore, transient expression of Foxp3 during retinoic acid receptor (RAR)–related orphan receptor–γ (RORγ)–dependent differentiation of Th17 cells was visualized through activation of the R26Y allele by Cre recombinase constitutively expressed under control of the endogenous Foxp3 locus (27). Additionally, differences in regulation of expression of Foxp3 bacterial artificial chromosome (BAC) transgene and the endogenous Foxp3 locus encoding Cre can also affect the discrepant outcomes of YFP-tagging of Treg cells in the corresponding experimental models.

We demonstrated that the Treg cell lineage is remarkably stable under physiologic conditions and after a variety of challenges. Stable Foxp3 expression in committed Treg cells is probably facilitated by a positive autoregulatory loop (28). Our results also suggest that continuous self-renewal of the established Treg cell population combined with heritable maintenance of Foxp3 expression serves as a major mechanism of maintenance of this lineage in adult mice.

Supporting Online Material

www.sciencemag.org/cgi/content/full/329/5999/1667/DC1

Materials and Methods

Figs. S1 to S13

References and Notes

  1. Materials and methods are available as supporting material on Science Online.
  2. We thank K. Forbush, T. Chu, L. Karpik, A. Bravo, J. Herlihy, P. Zarin, G. Gerard, A. Ortiz-Lopes, and K. Hattori for assistance with mouse colony management; F. Costantini for R26Y mice; V. Kuchroo for Foxp3-IRES-GFP mice; P. Chambon for Cre-ERT2 plasmid; E. Pamer, C. Shi, and E. Leiner for L. monocytogenes and assistance with experiments; and P. Fink and K. Simmons for cells from Rag2pGFP mice and helpful discussion. R.E.N. was supported by NIH Medical Scientist Training Program grant GM07739. A.Y.R. is an investigator with the Howard Hughes Medical Institute, and this work was also supported by grant AI51530 from the NIH to C.B. and D.M.
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