Figure 1
Figure 1. Abnormally differentiated ALPS DNT cells show high proliferative activity in vivo. (A) PBMC from patients with ALPS and healthy controls were gated for CD4+, CD8+, and DNT cells and analyzed for Ki67 expression. Histograms show a representative experiment, y-axis is normalized to mode. Cumulative data of all untreated patients with ALPS and healthy controls are graphed; each symbol represents an individual subject. ***P < .001 (Mann-Whitney U test). (B) Expression of proliferating cell nuclear antigen and cyclin A was determined in ALPS CD4+ (gray, filled), CD8+ (black, dotted), and DNT (black, solid) cells. Overlays show representative data from 1 of 5 independent experiments with similar results. (C) PBMC of patients with ALPS (n = 12) were gated for Ki67+ lymphocytes. Frequencies of B cells (CD3−/CD19+), NK cells (CD3−/CD56+), NKT cells (CD3+/CD56+ or TCRVα24−Jα18+), γδ T cells (CD3+/TCRγδ+), CD4+ T cells (CD3+/TCRαβ+/CD4+), CD8+ T cells (CD3+/TCRαβ+/CD8+), and DNT cells (CD3+/TCRαβ+/CD4−/CD8−) among all Ki67+ lymphocytes were determined by flow cytometry. Box plots depict the 75th percentile, median, and 25th percentile values; whiskers represent maximum and minimum values. (D) Correlation of percentage of Ki67+ DNT cells and frequency of CCR7−/CD45RA+ DN T cells among all ALPS DNT cells is shown; r = .7471; ***P < .001 (Spearman’s test). (E) Expression of CD27, CD28, CD57, and Ki67 were determined in ALPS DNT cells. Plots show representative data from 1 of 3 independent experiments with similar results.

Abnormally differentiated ALPS DNT cells show high proliferative activity in vivo. (A) PBMC from patients with ALPS and healthy controls were gated for CD4+, CD8+, and DNT cells and analyzed for Ki67 expression. Histograms show a representative experiment, y-axis is normalized to mode. Cumulative data of all untreated patients with ALPS and healthy controls are graphed; each symbol represents an individual subject. ***P < .001 (Mann-Whitney U test). (B) Expression of proliferating cell nuclear antigen and cyclin A was determined in ALPS CD4+ (gray, filled), CD8+ (black, dotted), and DNT (black, solid) cells. Overlays show representative data from 1 of 5 independent experiments with similar results. (C) PBMC of patients with ALPS (n = 12) were gated for Ki67+ lymphocytes. Frequencies of B cells (CD3/CD19+), NK cells (CD3/CD56+), NKT cells (CD3+/CD56+ or TCRVα24Jα18+), γδ T cells (CD3+/TCRγδ+), CD4+ T cells (CD3+/TCRαβ+/CD4+), CD8+ T cells (CD3+/TCRαβ+/CD8+), and DNT cells (CD3+/TCRαβ+/CD4/CD8) among all Ki67+ lymphocytes were determined by flow cytometry. Box plots depict the 75th percentile, median, and 25th percentile values; whiskers represent maximum and minimum values. (D) Correlation of percentage of Ki67+ DNT cells and frequency of CCR7/CD45RA+ DN T cells among all ALPS DNT cells is shown; r = .7471; ***P < .001 (Spearman’s test). (E) Expression of CD27, CD28, CD57, and Ki67 were determined in ALPS DNT cells. Plots show representative data from 1 of 3 independent experiments with similar results.

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