Fig 1: Tregs suppress T595_S597 phosphorylation of DEF6 in responder Tcons. (A) The peptide sequences of DEF6 containing the conserved phosphosites in respective organisms are shown. Ser (S) and Thr (T) with detected phosphorylation in =2/3 donors are highlighted in red. Phosphosites of interest (T595 and S597) are additionally highlighted in big letters. (B) log2 of average ratio of T595_S597 phosphorylated DEF6 peptide in the given comparisons. (C) Representative FTMS spectrum of the indicated DEF6 phosphopeptide (phospho-T595_S597). Precursor areas of the three indicated samples are depicted. Shown is the spectrum from Donor 3 (from one out of three technical replicate mass spectrometry runs) representative of three donors, with following properties: quantified Ion: z = +3, Mono m/z = 744.31616 Da, and MH+ = 2,230.93393 Da. Filled circles are isotope pattern peaks used in calculating the quantification values for the different quantification channels, as opposed to unfilled circles. The bar chart (right) shows quantification of the respective spectrum.
Fig 2: Proposed model of activation- and suppression-induced changes in the Tcon phosphoproteome. The scheme depicts the general upregulation of phosphorylation (P) upon TCR stimulation, which is largely counteracted by Tregs. Treg-suppressed cells partially resemble the unstimulated state and also present some additional changes not occurring upon activation. Tregs inhibit DEF6 phosphorylation at T595 and S597 sites, which is proposed to occur upon TCR activation and to confer interaction with the IP3R and downstream NFAT signaling and cytokine expression. Lower right panel modified from Ref. (8).
Fig 3: T595 and S597 phosphosites in DEF6 protein contribute to IP3R interaction and T cell activation. Plasmids encoding for DEF6-WT, DEF6 T595_S597 phospho-mutant (DEF6-2A), and DEF6 T595_S597 phospho-mimic (DEF6-2E) were generated. (A) HEK293 cells were cotransfected with indicated myc-tagged DEF6 constructs along with FLAG-tagged IP3R. Whole cell lysates (WCLs) were subjected to immunoprecipitation (IP) with anti-myc antibody (left), and aliquots of WCLs were kept untreated (right). Western blot antibodies are indicated. A representative experiment of 2 is shown. (B–E) Primary human Tcons were transiently transfected with plasmids encoding the indicated DEF6 protein or empty vector [EV; green fluorescent protein (GFP) in place of DEF6] for 8 h. Where indicated, cells were subsequently stimulated (Stim) with anti-CD3/anti-CD28 antibodies and processed as follows: (B) transfection efficiency based on GFP expression in EV-transfected cells was determined by flow cytometry. It was pre-gated on live lymphocytes based on fsc/ssc. Overlaid histogram of GFP expression in untransfected and EV-transfected Tcons is representative of five donors in two independent experiments. (C) Cells were stimulated for 5 min and analyzed by Western blot with antibodies against indicated targets (left). The ratio of levels of dephosphorylated NFAT1 and phosphorylated NFAT1 was calculated after quantification of the bands. Expression levels of myc-tagged DEF6 or total DEF6 and GAPDH served as transfection and loading controls, respectively. Blot is representative of five donors. Right: NFAT1 ratios were normalized to the corresponding NFAT1 ratio in unstimulated Tcons of the same donor which was set to 1. Individual NFAT1 ratios from n = 5 donors (represented by individual symbol per donor) from 2 independent experiments along with the mean values (line) are shown. IL2 (D) and IFNG (E) mRNA in transfected Tcons after 3 h of stimulation or without stimulation (Unstim), normalized to RPL13A mRNA. Results are presented as fold change compared to unstimulated Tcons of the same donor, which was set to 1. Left: mean ± SD of technical triplicates from quantitative RT-PCR is shown for one donor, representative of five donors from two independent experiments. Right: individual values of log2 fold change of mRNA levels of the respective cytokines from five donors (represented by individual symbol) are shown along with mean values (lines). P values (C–E) were determined by paired, two-sided Student’s t-test (*P < 0.05).
Supplier Page from Abcam for Anti-DEF6 antibody [EPR7492]