Figure 1
Figure 1. Evaluation of the pDCs and mDCs in WHIM patients. (A) Percentages of mDCs and pDCs (calculated as the percentage of the lymphocyte population) in 5 WHIM patients compared with 24 healthy subjects. To identify pDCs and mDCs via flow cytometry, we used the following gating strategy. Side scatter and staining with anti-CD4-peridinin chlorophyll protein and anti-CD14/anti-CD15/anti-CD19/anti-CD20-fluorescein isothiocyanate were used to exclude B cells, neutrophils, and monocytes. (B) IFN-α production was evaluated after HSV1 infection (dose ranging from 10 to 10 000 pfu/mL, for 24 hours; B) or CpG (Toll-like receptor 9 ligand, 5μM for 24 hours) stimulation (C) in PBMCs of 3 WHIM patients compared with healthy subjects. PBMCs (2.5 × 106/mL) were plated in U-bottomed 96-well plates and cultured with 5μM CpG (ODN2216, InvivoGen) or infected with HSV1 (strain MacIntyre; from 10 up to 10 000 pfu/mL) for 24 hours. IFN-α levels in culture supernatants were determined using a VeriKine human IFN-α ELISA Kit (PBL InterferonSource) according to the manufacturer's instructions. (B-C) Results are presented as average of duplicate data. Error bars represent SE. Comparison of cytokine production by nonparametric analysis shows significant differences between WHIM patients and control subjects.

Evaluation of the pDCs and mDCs in WHIM patients. (A) Percentages of mDCs and pDCs (calculated as the percentage of the lymphocyte population) in 5 WHIM patients compared with 24 healthy subjects. To identify pDCs and mDCs via flow cytometry, we used the following gating strategy. Side scatter and staining with anti-CD4-peridinin chlorophyll protein and anti-CD14/anti-CD15/anti-CD19/anti-CD20-fluorescein isothiocyanate were used to exclude B cells, neutrophils, and monocytes. (B) IFN-α production was evaluated after HSV1 infection (dose ranging from 10 to 10 000 pfu/mL, for 24 hours; B) or CpG (Toll-like receptor 9 ligand, 5μM for 24 hours) stimulation (C) in PBMCs of 3 WHIM patients compared with healthy subjects. PBMCs (2.5 × 106/mL) were plated in U-bottomed 96-well plates and cultured with 5μM CpG (ODN2216, InvivoGen) or infected with HSV1 (strain MacIntyre; from 10 up to 10 000 pfu/mL) for 24 hours. IFN-α levels in culture supernatants were determined using a VeriKine human IFN-α ELISA Kit (PBL InterferonSource) according to the manufacturer's instructions. (B-C) Results are presented as average of duplicate data. Error bars represent SE. Comparison of cytokine production by nonparametric analysis shows significant differences between WHIM patients and control subjects.

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