[33]. Cells were washed
three times in media and counted. PBMC from cutaneous leishmaniasis patients and non-infected individuals were used for in vitro culture TCR-usage analysis. Cultures were set up using a concentration of 2·5 × 105 cells in 96-well plates in the presence or absence of SLA (10 µg/ml final concentration) and were incubated for approximately 20 h. During the last 4 h of culture, Brefeldin-A (Sigma-Aldrich) (1 µg/ml), which impairs protein secretion by the Golgi complex, was added to the cultures. After the incubation period, cultures were harvested and submitted to flow cytometric analysis to evaluate T cell repertoire, surface markers and cytokine profile. The antibodies used for staining were immunoglobulin fluorescein isothiocyanate (FITC) and phycoerythrin (PE) controls (PharMingen, San find more Diego, CA, USA), anti-Vβ2-biot, anti-Vβ3-biot,
anti-Vβ5·1-biot, anti-Vβ5·2-biot, anti-Vβ11-biot, anti-Vβ17-biot, anti-Vβ 24-biot (Immunotech, Burlingame, CA, USA) anti-Vβ8-FITC, anti-Vβ 12-FITC (Immunotech), SA-FITC (PharMingen), anti-CD69 PE (Ebioscience, San Diego, CA, USA), selleck inhibitor anti-HLA-DR-PE, anti-CD45RO-PE (PharMingen) and anti-CD4-PE-Cy5 (Ebioscience). The anti-cytokines antibodies used were PE-labelled anti-IFN-γ, anti-TNF-α (PharMingen) and anti-IL-10 (Caltag, Carlsbad, CA, USA). PBMC were analysed for their repertoire, surface markers and intracellular cytokine expression pattern. Briefly, 2·5 × 105 PBMC were cultured in 96-well plates in
200 µl cultures for 20 h with either media alone or SLA (at 10 µg/ml final concentration). Brefeldin-A (1 µg/ml) was added during the last 4 h of culture to impair protein secretion, allowing for cytokine intracellular staining, as performed previously by us [11]. The cells were then stained for T cell receptor Vβ repertoire and surface markers, and fixed using 4% formaldehyde (Sigma-Aldrich). Cells were then permeabilized with a solution of saponin (Sigma-Aldrich) and stained, for 30 min at 4°C, using anti-cytokine monoclonal antibodies directly medroxyprogesterone conjugated with PE. PE-labelled immunoglobulin control antibodies and a control of unstimulated PBMC were included in all experiments. Preparations were washed and fixed as described in the previous section and analysed using fluorescence activated cell sorter analysis (FACS), selecting the total lymphocyte population (Fig. 1). In all cases both cytokine and surface marker staining were associated with T cell receptor Vβ repertoire staining for studying the expression of cytokines and surface markers together and the phenotype of the cells that produced them. At least 40 000 gated events were acquired for later analysis.