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KMID : 1040620180240010077
Clinical and Molecular Hepatology
2018 Volume.24 No. 1 p.77 ~ p.87
Picroside II attenuates fatty acid accumulation in HepG2 cells via modulation of fatty acid uptake and synthesis
Dhami-Shah Hiteshi

Vaidya Rama
Udipi Shobha
Raghavan Srividhya
Abhijit Shiny
Mohan Viswanathan
Balasubramanyam Muthuswamy
Vaidya Ashok
Abstract
Background/Aims: Hepatic steatosis is caused by an imbalance between free fatty acids (FFAs) uptake, utilization, storage, and disposal. Understanding the molecular mechanisms involved in FFAs accumulation and its modulation could drive the development of potential therapies for Nonalcoholic fatty liver disease. The aim of the current study was to explore the effects of picroside II, a phytoactive found in Picrorhiza kurroa, on fatty acid accumulation vis-a-vis silibinin, a known hepatoprotective phytoactive from Silybum marianum.

Methods: HepG2 cells were loaded with FFAs (oleic acid:palmitic acid/2:1) for 20 hours to mimic hepatic steatosis. The FFAs concentration achieving maximum fat accumulation and minimal cytotoxicity (500 ¥ìM) was standardized. HepG2 cells were exposed to the standardized FFAs concentration with and without picroside II pretreatment.

Results: Picroside II pretreatment inhibited FFAs-induced lipid accumulation by attenuating the expression of fatty acid transport protein 5, sterol regulatory element binding protein 1 and stearoyl CoA desaturase. Preatreatment with picroside II was also found to decrease the expression of forkhead box protein O1 and phosphoenolpyruvate carboxykinase.

Conclusions: These findings suggest that picroside II effectively attenuated fatty acid accumulation by decreasing FFAs uptake and lipogenesis. Picroside II also decreased the expression of gluconeogenic genes.
KEYWORD
Nonalcoholic fatty liver disease, Picrorhiza kurroa, Picroside II, Reverse pharmacology, Silibinin
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