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乙醇对Hep G2人肝癌细胞中甘油脂质和脂肪酸代谢的影响。

Effect of ethanol on glycerolipid and fatty acid metabolism in Hep G2 human-hepatoma cells.

作者信息

Angeletti C, de Alaniz M J

机构信息

Instituto de Investigaciones Bioquímicas de La Plata (INIBIOLP), CONICET-UNLP, Argentina.

出版信息

Acta Physiol Pharmacol Ther Latinoam. 1996;46(2):57-69.

PMID:8998370
Abstract

It is well-known that ethanol alters fatty acid and glycerolipid metabolism in liver, but most of the studies have been developed on rats, so little is known about the corresponding effects on human liver. We have chosen the Hep G2 human hepatoma cell line, which appears to be an excellent in vitro model system. Cells were incubated in ethanol containing medium (0-400 mM) for 48 h. Incorporation and metabolism of radioactive substrates (14C(U) glycerol,[1-14C] palmitic acid and [1-14C] eicosatrienoic acid (n-6) were analyzed in cellular and conditioned medium lipids. Cellular growth rate and lipid composition of control and ethanol-treated cells were also studied. The results showed that ethanol inhibited logarithmic cellular growth rate in a concentration dependent manner, without affecting viability. Ethanol (400 mM) did not modify cellular major lipid composition except for an increase of cholesteryl esters, but produced a decrease in the proportions of myristic, palmitic and palmitoleic acids. Ethanol enhanced the incorporation of radioactive fatty acids into cellular glycerolipids but did not alter the rate of incorporation of 14C(U) glycerol. This was attributed to an isotopic solution of the radioactive glycerol as a result of increased alpha-glycerophosphate biosynthesis. Incorporation of radioactive fatty acids and glycerol into conditioned medium glycerolipids were increased in cells incubated in presence of ethanol. The increased incorporation of 14C glycerol into conditioned medium together with a simultaneous diminution in labeling cellular glycerides suggest that there would be a stimulation of the export of these lipid classes to conditioned medium. Conversion of [1-14C] palmitic to oleic acid and eicosatrienoic to arachidonic acid were inhibited in 400 mM ethanol treated cells suggesting an inhibition of delta 9 and delta 5 desaturase activity.

摘要

众所周知,乙醇会改变肝脏中的脂肪酸和甘油脂质代谢,但大多数研究是在大鼠身上进行的,因此对其对人类肝脏的相应影响了解甚少。我们选择了Hep G2人肝癌细胞系,它似乎是一个优秀的体外模型系统。将细胞在含乙醇的培养基(0 - 400 mM)中孵育48小时。分析了细胞和条件培养基脂质中放射性底物(14C(U)甘油、[1-14C]棕榈酸和[1-14C]二十碳三烯酸(n-6))的掺入和代谢情况。还研究了对照细胞和乙醇处理细胞的细胞生长速率和脂质组成。结果表明,乙醇以浓度依赖的方式抑制对数期细胞生长速率,但不影响细胞活力。400 mM乙醇除了使胆固醇酯增加外,并未改变细胞主要脂质组成,但使肉豆蔻酸、棕榈酸和棕榈油酸的比例降低。乙醇增强了放射性脂肪酸掺入细胞甘油脂质的过程,但未改变14C(U)甘油的掺入速率。这归因于由于α-甘油磷酸生物合成增加导致放射性甘油的同位素溶解。在乙醇存在下孵育的细胞中,放射性脂肪酸和甘油掺入条件培养基甘油脂质的量增加。14C甘油掺入条件培养基的量增加,同时细胞甘油酯标记减少,这表明这些脂质类向条件培养基的输出会受到刺激。在400 mM乙醇处理的细胞中,[1-14C]棕榈酸向油酸以及二十碳三烯酸向花生四烯酸的转化受到抑制,这表明δ9和δ5去饱和酶活性受到抑制。

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