d Viability measurement Cells seeded in 24 well plates were trea

d. Viability measurement Cells seeded in 24 well plates were treated with different concentrations of curcuma DMSO e tract, curcuma sellectchem ethanol e tract or curcumin. All e peri ments were performed in triplicates on cells from 5 inde pendent biopsies. After 6, 18 and 30 hours, to icity was analyzed using the MTT assay A fresh sterile solution of MTT with a concentration of 0. 5 mg ml in DMEM F12 was prepared, 500 ul were added to each well and incubated for 4 hours at 37 C. MTT was discarded, cells were lysed with DMSO for 5 min at 37 C and absorbance was measured at 565 nm. Absorbance of treated cells was calculated relative to ab sorbance of untreated control cells, which was set to 100%. Con centrations that were non to ic even at late time points were chosen for subsequent e periments.

Results of the MTT assay were previously shown to be comparable to other viability measurement techniques. Gene e pression analysis Human intervertebral disc cells were serum starved for 2 hours and then e posed to 5 ng ml IL 1B for 2 hours before adding 100 ug ml cur cuma DMSO e tract or 100 ug ml curcuma EtOH e tract for 6 hours. Untreated control cells were included to verify the inflammatory and catabolic response induced by IL 1B treatment. As we were able to show that the solvents did not influence cellular behavior, all groups were treated with the respective volume of either DMSO or EtOH in all e peri ments. Therefore, changes in gene e pression are either calculated relative to controls or relative to IL 1B prestimulated cells.

Based on the results with curcuma e tracts and data obtained by HPLC MS analysis, a 25 mM stock solution of curcumin was prepared and cells were treated with final concentrations of 5, 10 or 20 uM curcumin for 6 hours after IL 1B prestimula tion. Taking the appro imate percentage of curcumin in curcuma powder into account, the applied range of curcumin was predicted to be similar to the final concentration of curcumin when using the above mentioned curcuma e tracts. All gene e pression e periments were performed on cells from five independent biopsies. After treatment, cells were harvested by trypsin treat ment and total RNA was isolated using the PureLink RNA Mini Kit according to the manufac turers instructions. cDNA was synthesized using TaqMan Reverse Transcription Reagents and gene e pression of IL 1B, IL 6, IL 8, TNF, MMP1, MMP3, MMP13, TLR2 and TBP was analyzed.

Human specific probes and primers, TaqMan real time RT PCR Mi and 10 30 ng of cDNA were mi ed and measured in duplicates using the StepOne Plus Real Time PCR System . The comparative ct method was used to quantify PCR data. In order Entinostat to calculate changes in gene e pression induced by curcuma curcumin, gene e pression in IL 1B treated cells was set to 100% and gene e pression of IL 1B curcuma or IL 1B curcumin treated cells was calculated relative to IL 1B treated cells. Western Blot for NF ��B In order to investigate selleck catalog whether changes in NF ��B p65 translocation occur after

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