GARP: a key receptor controlling FOXP3 in human regulatory T cells

Fig. S1 Alignment of human GARP with the structure of the ectodomain of human TLR3. (A) Comparison of the ectodomain of TLR3 (pdb-id: 2A0Z) and GARP, conserved sequences are indicated by blue boxes, strictly conserved residues are highlighted white-on-red, and similar residues indicated by red characters. Secondary structure elements of the TLR3 structure are indicated by arrows (β strand), coils (helices) and TT (turns). (B) Ribbon diagram of a hypothetical GARP dimmer model, based on the dimerization proposed for TLR3. The prominent loops at 296–308 and 421–432 of GARP (▾) could have similar functions for dimerization as proposed for TLR3. Putative glycolysation sites are indicated with space-filling representations.

Fig. S2 GARP induced transcriptional control. (A) Analysis of LGMN, UBD, IL1R2, and GARP mRNA by semi-quantitative RT-PCR in T_h cells transduced with GARP, FOXP3, LGMN, LGALS3, and GFP as described in Figs 1–4. cDNA was tested in threefold dilutions starting with 1:3 using RPS9 as housekeeping control. (B) Western blot analysis of LGMN protein expression in the same cells as in (A).

Fig. S3 GARP induces genes of the extended T_reg-signature. (A) Semi-quantitative RT-PCR analysis of IL7R, CPE, RYR-1 and HPGD in Th cells as in Figs 1–4 under resting conditions (no stim.) and 3 days after stimulation with anti-CD3 and 100 U/ml IL-2 as described in Fig. S1. (B) Quantitative real-time RT-PCR analysis of GARP and FOXP3 in T_h cells as in (A) tested under resting conditions and 3 days after stimulation as in (A). Relative mRNA expression of T_hGFP cells was arbitrarily set as 1.

Fig. S4 Characterization of the T_reg cell line used in this study and for siRNA experiments. (A) This alloantigen-reactive T_reg cells line (T_regTHU) used, has been established and characterized in detail recently [15]. These cells constitutively express known T_reg-markers, FOXP3, LGALS3, and CD25 are shown as selected examples. For comparison T cells derived from sorted CD4^+CD25⁻ T_h cells were stimulated with the same allogeneic EBV B cells and IL-2 in the presence of vehicle or 10 ng/ml TGF-β₁. Analysis was done at day 7 after stimulation. (B) The same cells as in (A) were stimulated with anti-CD3/-CD28 DynalBeads (Invitrogen) and IL-2 for 6 hrs in the presence of 10 μg/ml brefeldin and tested for intracellular IL-2 and FOXP3 expression. Allo-antigen specific T_h cells served as control. (C) Lentiviral transduction efficacy of the T_reg cells as in (A) is similar as compared to T_h cells. (D) The hallmark feature of T_reg cells, anergy and suppressor function, are preserved over a period of six months of in vitro expansion of the same T_reg cells as in (A) and Figs 1–5.

Fig. S5 GARP is not up-regulated in TGF-β₁-induced T_reg cells. (A) Sorted CD4^+CD25⁻ T_h cells were stimulated with anti-CD3/-CD28/IL-2 without (T_h), in the presence of solvent (T_h^vehicle), and 10 ng/ml human TGF-β₁ (T_h^TGF-β1) as in Fig. S4. Expression of GARP and FOXP3 mRNA was assessed at day 6 by real-time RT-PCR as in Fig. 1. (B) TGF-β₁-induced T_reg cells as in (A) were tested for proliferation and suppressor function (upper panel) and proliferation with exogenous IL-2 (lower panel); bkg. ∇ background proliferation, stim. ∇ T-cell proliferation induced by irradiated allogeneic EBV B cells. Proliferation was assessed at day 3 by measuring incorporation of H³-thymidin (cpm).

Fig. S6 Anergy and suppressor function in alloantigen-specific T_h cells transduced with GARP following cryopreservation. (A) T_reg cells (T_reg cell lines MPO and HG [15]) and T_h cells as in Figs 1–4 were stimulated for proliferation using irradiated EBV B cells in the absence (stim.) or presence of IL-2 (stim.+IL-2) 1 week after thawing cryopreserved cells; bkg. ∇ background proliferation. Proliferation was assessed at day 3 by measuring incorporation of H³-thymidin (cpm). T_reg and T_h cells as in (A) were tested for suppressor function of alloantigen-stimulated parental T_h cells at a ratio of 1:1. Percent inhibition of T_h cell proliferation by the addition of retrovirally engineered T_h cells is indicated, setting addition of wilt-type T_h cells (T_h/T_h) as 100%. Proliferation was assessed at day 3.

Fig. S7 Effects of S6A-mutant LGALS3 on gene expression. (A) T_h cells transduced with either wild-type (T_hLGALS3) or mutant (T_hLGALS3^S6A) were analysed for FOXP3 and CD25 expression at day 3 following stimulation with anti-CD3 and 100 U/ml IL-2 compared to T_hGFP cells. (B) Quantitative real-time RT-PCR analysis of GARP, LGALS3, LGMN and KLF-2 expression of the same cells as in (A). T_h cells were tested under resting conditions and 3 days after stimulation with anti-CD3 and 100 U/ml IL-2. Relative mRNA expression of T_hGFP cells was arbitrarily set as 1.

Table S1 Differential gene expression of resting and activated CD4^+CD25^hi T_reg versus CD4^+CD25⁻ T_h cells analysed ex vivo as detected by array analysis

Table S2 Differential gene expression T_reg cells, T_hGARP and T_hFOXP3 compared to T_hGFP cells

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