Tregs in human secondary lymphoid are in a late activation stage and are polyclonally activated. (A) CpG methylation in the Treg cell-specific demethylation region of the FOXP3 gene in FACS-sorted, human SPL-derived CD4posCD25hpos Tregs and CD4posCD25neg Tconvs. Methylation status of the indicated CpG positions is indicated by circles: ○, hyperdemethylated (<95% methylation) or ●, methylated (>95% methylation). Complete demethylation was indicated by >95% conversion of C to T in the sequenced product; sites of complete methylation were indicated when >95% of the sequence peak heights indicated C (N = 3 male donors, a representative example is shown). (B) Mononuclear cells were obtained from healthy human PB and SPL samples and analyzed for expression of Helios and FoxP3 on CD4pos cells by flow cytometry (N = 3 for each tissue, representative examples are shown). (C) Flow cytometry of Ki67 expression in human PB, BM, liLNs, inLNs, and SPL Tregs (left panel) and in CD4posCD25posCD69pos liLN, inLN, and SPL Tregs (right panel; N = 5 for each tissue). Data were analyzed using a random-effect logistic regression model and no significant differences were found. (D) Flow cytometry of TCR-Vβ expression of CD69neg and CD69pos Tregs in liLN, inLN, and SPL samples. Representative examples are shown (N = 2-6 for each tissue). (E) TCR gene rearrangement patterns of CD25posCD69pos and CD25posCD69neg sorted T cells from PB and SPL, showing polyclonal TRB gene rearrangement patterns, both the complete VDJ-rearranged TRB genes (tubes A and B) and the incomplete DJ-rearranged TRB genes (tube C). A polyclonal sample is shown as control. A representative example is shown (N = 2); duplicates revealed similar patterns (not shown).