2 : 07 : 66 : 18 : 05 : 686 : 47 : 159, as described previ

2 : 0.7 : 6.6 : 1.8 : 0.5 : 68.6 : 4.7 : 15.9, as described previously (Eyngor et al., 2008). The purity of the EPS was determined by measuring the protein and endotoxin contents by conventional silver staining after polyacrylamide gel electrophoresis and by Limulus amebocyte lysate assay (BioWhittaker, Walkersville, MD), respectively. DNA or RNA contaminations were excluded by

measuring UV adsorption at 260 and 280 nm. The salmonid RTS11, a functional macrophage cell line (Ganassin & Bols, 1998; Brubacher et al., 2000), was a gift from Dr N. Bols (Waterloo, Canada). RTS11 cells were cultured at 18 °C in Leibovitz (L-15) medium (Gibco Laboratories, Grand Island, NY) supplemented with 10% fetal calf serum (Gibco Laboratories), l-glutamine (300 mg L−1), HEPES (1%), penicillin learn more (100 μg mL−1), streptomycin (100 μg mL−1) and amphotericin B (0.25 μg mL−1). The cell line was subcultured every 3 weeks by dividing cells and conditioned medium evenly between two flasks, and adding an equal volume of fresh medium. Cells used in this study had been passaged between 15 and 25 times. For stimulation of RTS11 macrophages, cells were seeded at 5 × 106

cells per well in a six-well tissue culture-treated plate (Costar), in serum-free and http://www.selleckchem.com/Caspase.html antibiotic-free L-15 medium. Cells were left undisturbed

at 18 °C for 48 h to allow for any manipulation-induced gene expression to return to constitutive levels. For infection assays with viable bacteria cells, RTS11 cells were infected with 20 μL of bacterial suspension (MOI of 100) for different time intervals. LPS (50 mg mL−1 of LPS 0127:B8 purchased from Sigma) stimulated cells Decitabine datasheet were used as positive controls. Phosphate-buffered saline (PBS)-stimulated macrophages were used as negative controls. Macrophages with medium alone served as controls for spontaneous cytokine release. At different time intervals (0, 3, 6, 9, 12 and 24 h), cells were harvested from individual wells, aliquoted and kept frozen in liquid nitrogen until RNAs were extracted. All experiments were performed three times (in triplicates). For EPS stimulation assays, 20 μL of fresh medium containing EPS (50 mg mL−1) was added to each well. Positive and negative controls are the same as listed above. All cytokine induction mixtures were incubated at 18 °C and assessed at the intervals specified above. Experiments comparing cytokine production in response to the viable bacteria EPS were always run concurrently.

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