Membranes were blocked overnight at 4 C with 2% BSA in TBST. After washing three times with TBST, blots were incu bated for 1 h at room temperature with primary antibody diluted with 2% BSA in TBST. After washing six times with TBST, the blots were then incubated with HRP labeled secondary antibody for 1 h at room temperature. Membranes were rewashed extensively and binding was detected using Enhanced Chemiluminescense western blotting detection system, according to the manufacturers instructions. Anti ERK12 and phospho ERK12 antibodies were from Cell Signaling Tech nology. Mouse monoclonal antibody tubulin Ab 4 served as internal control. The band was semiquantified by densitometry using systems as described above. Activation of NFB by electrophoretic mobility shift assay Cells were infected with 2105 C.
albicans at 37 C for 6 h. Nuclear and cytoplasmic extracts of synovial fibroblasts were prepared using NE PER nuclear and cytoplasmic extraction reagents according to the manufacturers selelck kinase inhibitor protocols. A non radioactive EMSA was performed using an EMSA kit according to the manufacturers instruc tions. Nuclear protein was used to bind biotinylated oligonucleotides containing the NFB binding site for 30 minutes at room temperature. The blank control was nuclear extracts being replaced with water. A competitioncold control was set up by adding non biotin labeled cold probes to the reaction. Samples were separated in a non denaturing polyacrylamide gel and blotted on a Biodyne B Pre cut Modified Nylon mem brane.
The biotin was labeled with alkaline phosphatase conjugated streptavidin and alkaline phos phatase was detected with Enhanced Chemiluminescense western blotting detection system. The band was semiquantified by densitometry using systems as described above. Measurement of PGE2, IL1 , and TNF selleckchem production in culture medium Cells were infected with 2105 C. albicans in the presence or absence of U0126 at 37 C for 12 h. The culture supernatant was harvested, and PGE2, IL1 , and TNF concentrations were measured by ELISA according to the man ufacturers instructions. Results COX 2 induction by C. albicans infection The effect of C. albicans on COX 2 expression by synovial fibroblasts was assessed at the molecular and protein level. Extraction of total RNA from synovial fibroblasts was per formed after 12 h co culture of synovial fibroblasts with differ ent seeding densities of C.
albicans and COX 2 induction examined by RT PCR. Addition of C. albicans to synovial fibroblasts increased COX 2 expression in a dose dependent manner. A significant increase in COX 2 expression over basal conditions was seen at a dose of 2104 yeastsdish with no further increase when higher numbers of yeast were added. The expres sion of COX 2 protein showed a similar pattern to that of mRNA expression.