The kinetics of CD4+Foxp3+ T cell accumulation during a human cutaneous antigen-specific memory response in vivo (original) (raw)
Human CD4+CD25hiFoxp3+ Tregs proliferate in vivo. To confirm and extend our previous findings that CD4+CD25+ Tregs are highly proliferative in vivo in humans (8), we analyzed the expression in these cells of Ki67, a nuclear protein expressed by proliferating cells in all phases of the active cell cycle (23). Gating strategy for nTregs was based on high expression of CD25, low expression of CD127, and high expression of Foxp3 (Supplemental Figure 1; supplemental material available online with this article; doi:10.1172/JCI35834DS1). We found that in freshly isolated PBMC populations, in all individuals tested, significantly higher proportions of CD4+CD25+CD127loFoxp3+ T cells expressed Ki67 than CD4+CD25int and CD4+CD25– T cell populations (mean ± SEM, 22.8% ± 2.2% compared with 5% ± 0.3% and 2.6% ± 0.2%, respectively; Figure 1, A and B). This supports previous data showing that human nTregs are highly proliferative in vivo (8). The cycling Foxp3+ Tregs displayed a predominantly CD45RO+ memory phenotype (mean ± SEM, 97% ± 1.2%, n = 10; data not shown). In addition, we followed 3 healthy donors over a period of 3–4 months and observed that the high proliferative activity of nTregs was maintained over time in the absence of any evidence of overt immune activation in vivo (Figure 1C). This raised 2 possibilities that are not mutually exclusive: either thymus-derived nTregs proliferate extensively in the periphery to maintain constant numbers, or proliferating memory T cells are converted to nTregs in the periphery (17). To probe the latter possibility, we first established a human experimental system that enabled us to examine the development, accumulation, and proliferation of CD4+Foxp3+ T cells during a secondary immune response to antigens in vivo.
Human CD4+CD25hi Tregs turn over rapidly in vivo. Freshly isolated PBMCs from healthy individuals were stained for CD4/CD25/CD127/Foxp3 and Ki67 following the standard protocol. Tregs were identified as CD25hi, Foxp3+, and CD127lo (for details, see Supplemental Figure 1). (A) Expression of Ki67 on CD4+CD25hi, CD4+CD25int, and CD4+CD25– cells from a representative sample. Numbers denote the percentage of cells expressing Ki67 relative to the control gate set with an irrelevant antibody. FSC, forward scatter. (B) Cumulative data showing the percentage of Ki67+ cells in each subset. Each symbol represents a different individual (n = 10 per group), and the mean percentage is shown as a horizontal line. Significance was determined by paired t test. (C) Graphs show expression of Ki67 in Treg and non-Treg populations examined over the course of 4 months in 3 individuals.
The induction of a memory T cell response in humans in vivo. The MT was induced by the intradermal injection of tuberculin purified protein derivative (PPD) in healthy individuals who had been previously vaccinated against tuberculosis with BCG (Figure 2A). The clinical manifestation of this response is measured by the induction of erythema, induration, and palpability of the lesion (Figure 2A), which peaked at 3 days after PPD injection, as described previously (21, 22). Punch biopsies and skin suction blisters were induced at various time points following the injection of PPD (Figure 2A), permitting the examination of the underlying cellular response. In contrast to clinical response, the infiltrating T cells reached maximal levels 7 days after PPD injection (Figure 2B, dashed line, left axis). CD4+ T cells were the predominant cell type identified in the MT, and 95% of these cells (taken from the lesion) had a CD45RA– (CD45RO+) CCR7lo phenotype, compared with 50% of CD4+ T cells taken from the same subject’s blood (Supplemental Figure 2, A–C). Furthermore, the T cells that accumulated in the skin were highly differentiated, as indicated by low expression of CD45RB (data not shown). Other leukocytes found in the suction blister–derived populations included CD68+ macrophages, CD1a+ Langerhans cells, and CD11c+ and DC-SIGN+ dendritic cells, which have been characterized in this model previously (ref. 21 and data not shown).
The MT is a well-characterized model of a memory immune response. Samples were collected between 0 and 19 days after PPD injection. (A) Skin biopsies were collected for immunohistochemistry (top panel), and cutaneous lymphocytes were isolated from skin suction blisters that were induced over the sites of PPD injection at different time points (lower panel). (B) PPD-specific memory T cells accumulate during the course of MT. PBMCs and blister cells were stimulated with PPD for 15 hours in the presence of Brefeldin A and stained for intracellular expression of IFN-γ (right y axis, solid lines). The number of CD3+ T cells within dermal perivascular infiltrates was determined by indirect immunoperoxidase staining of 5-μm tissue sections. The 5 largest perivascular infiltrates were counted and data presented per unit area (UA). The mean ± SEM of 5 individuals per time point is shown (dashed line, left y axis). (C) Blister cells recovered from day 7 blisters were stimulated with PPD or with irrelevant antigen (HSV, CMV, tetanus) or left unstimulated and stained for intracellular expression of IFN-γ. Representative dot plots (n = 3 samples per antigen) are shown. Numbers denote the percentage of cells expressing IFN-γ. (D) IFN-γ production from day 7 blisters raised over MT response or the site of the control (saline) injection. Numbers denote the percentage of cells expressing IFN-γ. PBMCs and blister cells (PPD and control) from the same donor were stimulated with PPD overnight as described in Methods.
We next evaluated the antigen specificity of the skin-infiltrating CD4+ T cells after intradermal challenge. CD4+ T cells harvested from skin suction blisters were assessed for their ability to synthesize IFN-γ after restimulation with PPD in vitro. The proportion of IFN-γ+ antigen-specific CD4+ T cells increased significantly after PPD injection (Figure 2B; Kruskal-Wallis test, P < 0.0001). The proportion of antigen-specific CD4+ T cells detected after antigen challenge on day 14 was considerably higher than that predicted from previous studies that only investigated early time points after injection (0.5%–2.0%) (24). Minimal IFN-γ was synthesized when PPD was not added to the blister cells or when the cells were stimulated with irrelevant antigens such as herpes simplex virus (HSV; Figure 2C), tetanus toxoid, or CMV (data not shown). In contrast, up to 30% of the CD4+ T cells from the skin expressed IFN-γ after PPD restimulation in vitro (Figure 2C). There was no increase in antigen-specific CD4+ T cells in the blood after cutaneous PPD challenge, and the numbers of these cells remained relatively constant at 0.5% of the CD4+ T cell pool at all time points (Figure 2, B and D). In addition, we showed that only 2% of CD4+ T cells that were harvested from a saline control injection at a separate site in the same individual secreted IFN-γ after PPD stimulation (compared with 23% of CD4+ T cells that were isolated from the site of PPD injection) (Figure 2D). There was variability in the size (volume) of blisters from different individuals that was probably related to the physical characteristics of the skin in different subjects. This made the assessment of the absolute numbers of antigen-specific cells unreliable for exact quantitation (range, 500–70,000 IFN-γ+CD4+ cells per blister). Therefore, the absolute numbers of PPD-specific cells in the skin is better estimated by equating together the number of CD4+ T cells in skin sections and the percentage of PPD-specific cells from suction blisters, which was considerably more consistent (Figure 2B). CD8+ antigen-specific T cells in the blisters did not increase during the course of the response and were present at less than 1% at all time-points (data not shown). The MT, therefore, enables the investigation of the kinetics of CD4+ memory T cell accumulation during a secondary immune response in vivo (22).
Accumulation of CD4+Foxp3+ T cells during a secondary response to antigen in vivo. We next investigated whether proliferation of T cells in situ contributed to the accumulation of antigen-specific CD4+ T cells after PPD injection. Tissue biopsies obtained from the site of antigen injection at different times were co-stained with Ki67 and CD4 (Figure 3A). The 5 largest perivascular infiltrates per section were photographed and counted, and data were expressed as mean absolute cell number per frame. Very few proliferating cells were observed in normal skin (day 0), and the perivascular infiltrates were very small or absent. Similar proportions of proliferating CD4+ T cells were identified by flow cytometry of blister (but not PBMC) populations taken at the same time points (Figure 3C and data not shown). At day 7, the time of maximal CD4+ T cell accumulation, the number of CD4+ T cells expressing Ki67 was significantly increased (Figure 3D) and more than 20% of the CD4+ T cells were in cycle (Figure 3, A and E). This indicated that the increase in PPD-specific CD4+ T cells in the skin after antigenic challenge occurred in part through their extensive local proliferation (Figure 2B).
Antigen-specific memory CD4+ T cell proliferation at the site of the MT. (A) Double immunofluorescence staining of representative biopsies from days 0, 3, 7, and 14 following MT induction. Green indicates Ki67; red indicates CD4. Original magnification, ×400. (B) Double immunofluorescence staining of representative biopsies (days 0, 3, 7, and 14; n = 5 per time point) shows CD4+ (green) and Foxp3+ (red) cells in a perivascular lymphocytic infiltrate (original magnification, ×400). The 5 largest perivascular infiltrates present in the upper and middle dermis were selected for analysis. Cell numbers were expressed as the mean absolute number of cells counted within the frame. (C) The proportion of Ki67+CD4+ cells was also determined by flow cytometry using blister cells (n = 3–5 per time point). Representative dot plots for day 7 PPD blister cells and PBMCs are shown. Numbers denote the percentage of cells expressing Ki67 relative to control gate set with an irrelevant antibody. (D) Number of total CD4+ cells (filled squares) and number of Ki67+CD4+ cells (open squares) in perivascular infiltrates following PPD injection. (E) Percentage of CD4+ cells expressing Ki67 found per perivascular infiltrate in each donor. Each circle represents an average of 5 perivascular infiltrates counted for each individual (n = 5–7 per time point; horizontal lines indicate the mean). (F) Number of total CD4+ cells (filled squares) and CD4+Foxp3+ cells (open squares) in perivascular infiltrates following PPD injection. (G) Percentage of CD4+ cells expressing Foxp3 per perivascular infiltrate counted. Each symbol represents an average of 5 perivascular infiltrates counted for each individual (n = 5–7 per time point). Data are mean ± SEM.
We have previously shown a high level of proliferation in circulating CD4+CD25hi Tregs (8). We examined tissue biopsies taken during MT for the expression of CD4 and Foxp3 and enumerated double-positive cells in the perivascular infiltrates. Figure 3B shows the expression of CD4 and Foxp3 in representative cellular infiltrates at days 0 (control skin), 3, 7, and 14 following PPD injection. Cumulative data from 5 individuals per time point are presented in Figure 3F, showing a significant increase in the number of CD4+Foxp3+ T cells on day 7 (P = 0.04, 1-way ANOVA). This increase in the percentage of CD4+Foxp3+ cells coincided with the increase in total CD4+ T cell numbers and also with peak cellular proliferation (P = 0.01, 1-way ANOVA). However, when the corresponding increase in CD4+ T cell numbers was taken into account and the data were expressed as the proportion of CD4+ T cells expressing Foxp3, this value remained fairly constant during the response (between 8%–15% of CD4+ cells; Figure 3G). The percentage of CD4+Foxp3+ cells on day 0 could not be accurately assessed due to the very low CD4 numbers, although Foxp3+ Tregs could be observed in some samples of normal skin (Figure 3B and ref. 25). We concluded that both memory and Foxp3+ (putative regulatory) T cells accumulate at the same rate after antigenic stimulation in vivo.
Induction of Foxp3 expression in activated CD4+ T cells in vitro. Previous studies have found that human CD4+CD25– effector T cells can upregulate Foxp3 transiently, following activation (26–28). It was possible, therefore, that the Foxp3-expressing CD4+ T cells that were found in the skin after antigen challenge were activated memory T cell populations that were induced to express this marker temporarily. To clarify this we first investigated the relationship between Foxp3 expression and proliferation in CD4+CD25–Foxp3– T cells after activation in vitro (Figure 4A). These cells were isolated from peripheral blood, labeled with CFSE, and then activated with anti-CD3/CD28 coated beads. The expression of CD25, Foxp3, and Ki67 was determined on days 0, 3, 5, and 7. By day 3, approximately 80% of cells were CD25+ and 35% of CD4+ cells expressed Foxp3. All Foxp3+ cells were Ki67+, and approximately 80% of the activated CD4+ T cell population had lost the CFSE label (Figure 4). Most cells lost Foxp3 expression (but remained CD25+ and Ki67+) by day 7, indicating that the induction of Foxp3 expression in CD4+ T cells after activation was transient (Figure 4A).
Induction of Foxp3 expression in human CD4+CD25– T cells by stimulation. (A) CD4+CD25– (responder) T cells were isolated from PBMCs using MACS and labeled with CFSE. Cells were stimulated with magnetic beads coated with antibodies to CD3 and CD28 for 7 days. Samples were removed at regular intervals and stained for the expression of CD25, Foxp3, and Ki67. Numbers in dot plots indicate the percentage of cells in each quadrant. Dilution of the CFSE signal indicates proliferation of the cells. Percentages refer to cells that have not divided. Data shown are representative of 3 independent experiments. (B) Cells were removed from CD3/CD28-stimulated cultures on day 4 and restimulated with PMA and ionomycin before staining for Foxp3, IL-2, and IFN-γ. Histograms show cytokine production by Foxp3– and Foxp3+ cells and are representative of 3 independent experiments. Numbers indicate the percentage of cells expressing IL-2 or IFN-γ.
To assess whether CD4+Foxp3+ cells that develop as a result of activation exhibit functional characteristics of Tregs, we examined their capacity to synthesize effector cytokines following restimulation, since Tregs do not synthesize IL-2 or IFN-γ (29–32). CD3/CD28-activated CD4 cells were removed from culture on day 4 and restimulated with PMA and ionomycin for 4 hours, followed by staining with Foxp3, IL-2, and IFN-γ (Figure 4B). There was no difference in cytokine production between Foxp3+ and Foxp3– cells, indicating that the induction of Foxp3 transiently in T cells is not accompanied by the acquisition of functional characteristics of Tregs, in agreement with previous reports (27, 33, 34).
Foxp3+ T cells at the site of MT proliferate in parallel to effector T cells and have a Treg phenotype. To determine whether the Foxp3+ cells found in the skin represented a Treg population or activated CD4+ T cells that expressed Foxp3 transiently, we double-stained the MT skin sections for Ki67 and Foxp3 expression (Figure 5A). In contrast to the CD4+ T cells that were activated in vitro, where all Foxp3+ cells are also Ki67+, in the skin only a proportion of CD4+Foxp3+ cells expressed Ki67 (14%–33% at all times following PPD injection; mean, 23.2%). The kinetics of Ki67 expression in Foxp3+ (putative Tregs) and CD4+Foxp3– (effector cells) are very similar (Figure 5B). To characterize the Foxp3+ T cells in the skin more extensively, we induced skin suction blisters at the site of the MT response on day 7 following PPD injection. This time point was chosen because it coincided with the peak CD4+ T cell infiltration and proliferation. Cells isolated from the blisters were stained for the co-expression of Foxp3 with CD25, CD127, CD39, and CD27, as all these markers have been shown to identify nTregs (19, 35–38) (Figure 5C). The percentage of Foxp3+ cells in day 7 blisters was very similar to that observed in histology (range, 7.1% to 22.2%; mean, 14.5% ± 2.0%; n = 6). The majority of Foxp3-expressing CD4+ T cells were CD25+ (78.5% ± 7.5%, n = 3) and expressed low levels of CD127 (mean ± SEM, 10% ± 2.7%, n = 5). Furthermore, these cells were uniformly CD27+, a hallmark of Tregs at sites of immune activation in vivo (19). Finally, the Foxp3-expressing T cells in skin also express CD39, another marker for nTregs (mean, 83.6% ± 4.0%) (37, 38). In contrast, the CD4+Foxp3– T cells that were found in the same samples were largely CD25– and CD39– but had high expression of CD127.
Foxp3+ T cells have a Treg phenotype and proliferate at the site of an immune response. (A) Double immunofluorescence staining of Ki67 (green) and Foxp3 (red) in a representative day 7 skin section (original magnification, ×400). Arrows indicate cells staining positive for both Ki67 and Foxp3 (yellow). (B) Graph shows the percentage of CD4+ (white bars) and CD4+Foxp3+ (black bars) cells expressing Ki67. Data are mean ± SD; n = 5 per time point. (C) Blister cells were isolated on day 7 following MT induction and stained for Foxp3, CD127, CD25, CD27, and CD39. Representative staining (n = 6) is shown. Dot plot indicates the gating strategy, and histograms show the expression of surface molecules on CD4+Foxp3+ and CD4+Foxp3– subsets. MFI and percentage of positive cells are indicated. CLA, cutaneous lymphocyte antigen. (D) Blister cells were isolated on day 7 following MT induction, stimulated with PPD for 15 hours in the presence of brefeldin A, and stained for intracellular expression of cytokines and Foxp3. The percentage of Foxp3+ and Foxp3– cells secreting cytokines is indicated. Dot plots are representative of 4–6 independent experiments.
Technical limitations, namely very small numbers of leukocytes collected from blisters, precluded purification of the putative Treg population from the skin. For day 7 blisters in 30 subjects that were investigated, a mean of 295,000 cells were obtained (range 40 to 900,000 leukocytes, of which 5%–50% were CD4+ T cells). Therefore, the estimated mean number of CD4+CD25+CD127lo cells that were present and that we were unable to isolate with current technology was about 2,000–25,000. However, unlike effector cells, nTregs do not secrete IL-2 and IFN-γ after recent stimulation in vitro (29–32). We therefore investigated the capacity of Foxp3+ and Foxp3– CD4+ T cells that were isolated from suction blisters to produce effector cytokines following restimulation with antigen in vitro. Cells isolated from day 7 blisters were stimulated with PPD for 16 hours and stained for CD4, Foxp3, and IFN-γ or IL-2. Following restimulation, significantly greater numbers of CD4+Foxp3– cells synthesized IFN-γ compared with the CD4+Foxp3+ T cell population (IFN-γ: P = 0.015, Wilcoxon paired test; n = 6). Similar data were obtained for IL-2 in 4 separate donors (Figure 5D; P = 0.06). Thus, although we were not able to assess suppressive function directly, we found that the CD4+Foxp3+ cells in the skin after antigenic challenge are not recently activated effector CD4+ T cells and are clearly distinct, phenotypically and functionally, from the CD4+Foxp3– population.
Finally, to determine whether the cycling Foxp3+ cells (Ki67+) also exhibit a Treg phenotype, we compared the expression of CD127 on Foxp3+Ki67+ and Foxp3+Ki67– T cells (Figure 6). Both cycling and non-cycling Foxp3-expressing populations expressed low levels of CD127, indicating that they were Tregs (mean ± SEM, 8% ± 2.3% and 10.5% ± 3.2%, respectively; n = 6). In contrast, CD127 was highly expressed in both in Foxp3–Ki67+ and Foxp3–Ki67– populations (mean ± SEM, 55.7% ± 7% and 80.1% ± 2%, respectively; n = 6). Therefore, we determined that Foxp3+ cells that accumulate during the course of MT have multiple phenotypic and functional characteristics of naturally occurring Tregs, and a significant proportion of these proliferate in parallel with the corresponding effector T cells.
Proliferating Foxp3+ T cells in the skin express low levels of CD127. Blister cells were isolated on day 7 following MT induction and stained for CD4, Foxp3, CD127, and Ki67. Representative staining (n = 6) is shown. (A) Dot plot indicates gating strategy. The percentage of cells in each quadrant is indicated. Histograms show the expression of CD127 on CD4+Foxp3+ and CD4+Foxp3– subsets divided by Ki67 expression. Numbers indicate the percentage of cells expressing CD127. (B) Cumulative data comparing Foxp3+Ki67+ and Foxp3+Ki67– subsets. P values were calculated using a paired t test. Data are mean ± SEM.
The generation of Tregs from skin-derived memory T cell populations. Foxp3+ Tregs observed during MT could originate from natural CD4+CD25+ Tregs, which either are resident in the skin or migrate into the skin after immune challenge. Both of these possibilities are supported by observations that some Foxp3+ cells reside in normal human skin (Figure 3B and ref. 25) and that circulating Tregs in humans preferentially express the skin-homing molecules CCR4, CLA (ref. 39 and Supplemental Figure 3), and CCR8 (40). An additional possibility is that some Tregs are derived from memory CD4+ T cells that are activated in the skin after antigenic activation.
To test the possibility that memory CD4+ T cells isolated from the skin can be converted into CD4+CD25hi Tregs in vitro, we first isolated PPD-specific CD4+ T cells from the skin 21 days after antigen injection, when maximal antigen-specific CD4+ T cells are present (21). Freshly isolated PPD-specific CD4+ T cells from the skin were not anergic and were not suppressive (data not shown). To obtain sufficient cell numbers for the functional assays, the skin-derived memory T cells were expanded by 3 rounds of stimulation with PPD and autologous irradiated PBMCs in vitro (Figure 7A), after which more than 90% were specific for PPD as determined by IFN-γ production in response to PPD restimulation (Figure 7B). We then investigated whether the expanded PPD-specific CD4 cells could be induced to express Treg markers and acquire suppressive activity_._ After expansion, PPD-specific CD4+ T cells were still responsive to PPD stimulation (Figure 7, A and B) and did not exhibit suppressive activity (Figure 7D). Previous studies showed that cloned CD4+ T cells could be induced to become regulatory if they were first rendered anergic (41, 42). We therefore anergized these cells by incubating them with immobilized anti-CD3 antibody and found that dose-dependent anergy was induced and that these cells were refractory to subsequent stimulation with PPD and irradiated antigen-presenting cells (Figure 7C and Supplemental Figure 4). In addition, anergized PPD-specific CD4+ T cells suppressed the ability of non-anergized PPD-specific T cell populations to proliferate in response to PPD presented by irradiated autologous antigen-presenting cells (Figure 7D and Supplemental Figure 4). Finally, we showed that, while Foxp3 was expressed at very low levels in both freshly isolated (blister cells ex vivo) and in vitro expanded, non-anergized PPD-stimulated CD4+ T cells derived from the skin (Figure 7E), after anergy induction, there was up to a 100-fold increase in the levels of Foxp3 detected (Figure 7E). In addition, anergized PPD-specific cells show other hallmarks of naturally occurring, CD4+CD25hi Tregs, including elevated levels of CD25, GITR, and CTLA-4 and low levels CD127 compared with their non-anergized counterparts (data not shown). In separate experiments, an increase in Foxp3 expression following anergy induction was confirmed at the protein level (Supplemental Figure 5). These data indicate that the induction of anergy in activated memory CD4+ T cells isolated from the site of a secondary immune response in vitro can lead to the generation of a Treg population that has all the identical phenotypic and functional characteristics of naturally occurring CD4+CD25hi Tregs in vivo.
Anergy induction leads to the development of a suppressive phenotype. (A) Cells recovered from a suction blister induced over a MT site 21 days following the induction were stimulated in vitro with PPD every 14 days (indicated by arrows). Peripheral blood CD4+ T cells from the same donor were cultured in parallel. (B) Dot plot shows IFN-γ production by the cell line in response to PPD stimulation. The percentage of cells expressing IFN-γ is indicated. (C) PPD-specific CD4+ T cell line was stimulated with immobilized anti-CD3 mAb. The cells were then washed and stimulated with PPD and antigen-presenting cells for 3 days, and proliferation was measured by [3H]-thymidine incorporation. The mean of triplicate wells ± SEM is shown (representative of 3 separate experiments). PPD-specific CD4+ T cells that were not anergized were used as control. (D) Anergized PPD-specific cells described in C were mixed with an equal number of autologous non-anergized PPD-specific cells and stimulated with PPD and autologous antigen-presenting cells. Proliferation was measured on day 3 and is expressed as mean ± SEM. Responders, non-anergized PPD cell lines cultured alone; control, responders with non-anergized PPD-specific cells. Results are representative of 2 separate experiments. (E) Foxp3 expression was measured by real-time quantitative RT-PCR using 18s rRNA as an internal control. Relative quantity values are plotted in a log-scale bar chart using the triplicate values to estimate SD. Cells recovered from the blister are indicated as “blister cells ex vivo.” Blister cells expanded in vitro prior to anergy induction were used as a control.