Figure 1
Figure 1. Characterization of CD25highCD27posCD45RAnegCD4pos Tregs. (A) Flow cytometry of peripheral CD25high and CD25neg cells within the PBMC CD4posCD27posCD45RAneg gate (n = 6). Percentages of cells positive for the indicated marker (top) are given. (B) Flow cytometry of sorted CD25highCD27posCD45RAnegCD4pos (CD25highCD27pos) Tregs and CD25negCD27posCD45RAnegCD4pos (CD25negCD27pos) Teffs. CD4 cells were isolated by magnetic bead–based negative selection. The enriched cells were labeled with anti-CD25, anti-CD27, and anti-CD45RA mAb and next, CD25highCD27posCD45RAneg and CD25negCD27posCD45RAneg cell populations were isolated by high-purity flow cytometric cell sorting. Density plots show surface staining of CD127 (x-axis) and intracellular staining of Foxp3 (y-axis). (C) Real-time quantitative reverse-transcriptase (RT)–PCR of the mRNA expression of Tbet, GATA3, RORγt, FOXP3, and TGFβ in freshly sorted CD25highCD27pos Tregs and CD25negCD27pos Teffs. The RT-PCR data shown were normalized to human HPRT1 levels, and expression in nonstimulated conditions of CD25negCD27pos cells was set as 1.0, and fold reduction or increase in gene expression was calculated. Cells obtained from 3 to 5 different donors were used. Mean and SD from different experiments are shown. * indicates statistically significant differences. (D) 3H-thymidine incorporation–based suppression assay of sorted CD25highCD27pos Tregs and CD25negCD27pos Teffs. Sorted cells were titrated (x-axis) into cultures with CD4pos responder T cells (25 × 103) and subsequently stimulated with anti-CD3 plus anti-CD28 mAb–coated beads. Proliferation (y-axis) was measured at day 3 after the start of the culture. A representative experiment is shown. Mean and SD of triplicate measurements are shown. Data are from n = 6 different healthy volunteers (A), or show representative experiments of 2 (C,D) or 3 (D) separate experiments performed with cells obtained from different cell donors.

Characterization of CD25highCD27posCD45RAnegCD4pos Tregs. (A) Flow cytometry of peripheral CD25high and CD25neg cells within the PBMC CD4posCD27posCD45RAneg gate (n = 6). Percentages of cells positive for the indicated marker (top) are given. (B) Flow cytometry of sorted CD25highCD27posCD45RAnegCD4pos (CD25highCD27pos) Tregs and CD25negCD27posCD45RAnegCD4pos (CD25negCD27pos) Teffs. CD4 cells were isolated by magnetic bead–based negative selection. The enriched cells were labeled with anti-CD25, anti-CD27, and anti-CD45RA mAb and next, CD25highCD27posCD45RAneg and CD25negCD27posCD45RAneg cell populations were isolated by high-purity flow cytometric cell sorting. Density plots show surface staining of CD127 (x-axis) and intracellular staining of Foxp3 (y-axis). (C) Real-time quantitative reverse-transcriptase (RT)–PCR of the mRNA expression of Tbet, GATA3, RORγt, FOXP3, and TGFβ in freshly sorted CD25highCD27pos Tregs and CD25negCD27pos Teffs. The RT-PCR data shown were normalized to human HPRT1 levels, and expression in nonstimulated conditions of CD25negCD27pos cells was set as 1.0, and fold reduction or increase in gene expression was calculated. Cells obtained from 3 to 5 different donors were used. Mean and SD from different experiments are shown. * indicates statistically significant differences. (D) 3H-thymidine incorporation–based suppression assay of sorted CD25highCD27pos Tregs and CD25negCD27pos Teffs. Sorted cells were titrated (x-axis) into cultures with CD4pos responder T cells (25 × 103) and subsequently stimulated with anti-CD3 plus anti-CD28 mAb–coated beads. Proliferation (y-axis) was measured at day 3 after the start of the culture. A representative experiment is shown. Mean and SD of triplicate measurements are shown. Data are from n = 6 different healthy volunteers (A), or show representative experiments of 2 (C,D) or 3 (D) separate experiments performed with cells obtained from different cell donors.

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