ABSTRACT
Background: Inflammation is one of an important biological response toward injury. Cytokine and mediator are produced by macrophage during the inflammatory process. Anti-inflammatory is important to treat the dangerous of chronic inflammation associated with chronic disease. Various plants and their derived compounds have been used in the treatment of inflammation including Myristica fragrans. The present study was designed to determine anti-inflammatory potential of M. fragrans seed (Nutmeg) ethanolic extract and pure quercetin extract from M. fragrans on LPS stimulated-murine macrophage cell line (RAW 264.7). Methods: Cell viability assay to evaluate the non toxic concentration in cell line was performed by MTS assay. The anti-inflammatory potential was assayed through the inhibitory activity of M. fragrans seed extract and quercetin on NO, TNF-α, IL-6, and IL-1β production. Results: The lowest cytotoxic activity and safe substance on RAW 264.7 cell were 50 and 10 μg/mL concentration of the M. fragrans seed ethanolic extract and quercetin compound. M. fragrans dose-dependently inhibited NO, TNF-α, IL-6 and IL-1β production on LPS stimulated-RAW 264.7. The 50 μg/mL of M. fragrans seed ethanolic extract showed the highest TNF-α, IL-6, IL-1β and nitrite-associated with NO inhibitory activity. Conclusions: This research suggested that M. fragrans seed extract and quercetin compound possess the anti-inflammatory potential showed through the inhibition of TNF-α, IL-6, IL-1β and NO secretion.
ABSTRACT
Background: Adipocytes accumulate triacylglycerol when excessive food consumption. Adipocyte dysfunction plays an important role in the obesity development. People with a body weight 40 % heavier than the average body weight population at risk of death two times greater than the average body weight. The use of anti-obesity drugs have many side effects, so it is necessary to find the anti-obesity drug with low toxicity. This ex vivo study was conducted to determine the activity of C. longa L. extract in inhibiting triglycerides and cholesterol synthesis and lipid droplet formation on HepG2 cells compared to curcumin. Methods: Anti-obesity activity includes reduced formation of lipid droplet in HepG2 cells can be observed using oil red O staining method. The measurement of triglyceride level was performed according to Randox protocol using Randox TR 210 assay kit. Lipolytic activity by measuring cholesterol levels was performed based on Randox CH 200 kits. Results: This study suggested that the extract of C. longa L. and curcumin have potential anti-obesity compounds. C. longa L. extract have higher activity in inhibiting triglycerides and cholesterol synthesis compared to curcumin with inhibition activities 70.43% and 66.38% respectively in the highest concentration. Conclusion: The C. longa extract posses the anti-adipogenesis potential on inhibiting the synthesis of triglycerides and cholesterol and lipid droplet formation in HepG2 cell as anti-obesity parameters better than curcumin.