Gupta A, Sexton R C, Rudney H
J Biol Chem. 1986 Jun 25;261(18):8348-56.
The effects of ketoconazole, a lanosterol demethylase and cytochrome P450 inhibitor, on the regulation of 3-hydroxy-3-methylglutaryl coenzyme A reductase (EC 1.1.1.34, reductase) activity and sterol biosynthesis were studied in rat intestinal epithelial cell cultures (IEC-6). Incubation of cells with 0.15-2 microM ketoconazole resulted in a concentration-dependent inhibition of reductase activity. As the drug concentration approached 15 microM, the reductase activity returned to control values, and at 30 microM ketoconazole, a stimulation of enzyme activity was observed. The drug had no effect on reductase activity in homogenates of IEC-6 cells. Ketoconazole (0.15-30 microM) caused a concentration-dependent inhibition of the incorporation of [3H] mevalonolactone into cholesterol with a concomitant accumulation of radioactivity in methyl sterols; e.g. lanosterol and 24,25-epoxylanosterol. Interestingly, the incorporation of radioactivity into polar sterols showed a biphasic response which was inversely proportional to the biphasic response of reductase activity. Thus, incorporation of [3H]mevalonolactone into polar sterols increased at low concentrations of ketoconazole (0.15-2 microM) and decreased to control values at high concentrations of the drug. Treatment of cells with ketoconazole (30 microM) and [3H]mevalonolactone followed by removal of the drug and radiolabel resulted in an inhibition of reductase activity and a redistribution of radioactivity from lanosterol and 24,25-epoxylanosterol to cholesterol and polar sterols. These results suggested that the inhibition of reductase activity at low concentrations of ketoconazole (less than 2 microM) was due to a formation of regulatory polar sterols generated from the methyl sterols. At high concentrations of ketoconazole (30 microM) where no suppression in reductase activity was observed, the conversion of exogenously added [3H]24(S),25-epoxylanosterol to polar sterols was prevented. Exogenously added 24,25-epoxylanosterol inhibited reductase activity in a dose-dependent fashion, and ketoconazole (30 microM) prevented the inhibition caused by low concentrations of epoxylanosterol. The drug, however, was unable to prevent the dose-dependent suppression of reductase activity by 25-hydroxylanosterol, a reduced form of 24,25-epoxylanosterol. These results indicated that 24,25-epoxylanosterol per se was not an inhibitor of reductase activity but could be metabolized to regulatory polar sterols through a cytochrome P-450 dependent reaction which was sensitive to ketoconazole. Treatment of cells with ketoconazole totally abolished the inhibition of reductase activity by low density lipoprotein (LDL).(ABSTRACT TRUNCATED AT 400 WORDS)
研究了羊毛甾醇脱甲基酶和细胞色素P450抑制剂酮康唑对大鼠肠上皮细胞培养物(IEC-6)中3-羟基-3-甲基戊二酰辅酶A还原酶(EC 1.1.1.34,还原酶)活性调节及甾醇生物合成的影响。用0.15 - 2微摩尔酮康唑孵育细胞导致还原酶活性呈浓度依赖性抑制。当药物浓度接近15微摩尔时,还原酶活性恢复到对照值,而在30微摩尔酮康唑时,观察到酶活性增强。该药物对IEC-6细胞匀浆中的还原酶活性无影响。酮康唑(0.15 - 30微摩尔)导致[3H]甲羟戊酸内酯掺入胆固醇的过程呈浓度依赖性抑制,同时甲基甾醇中放射性积累;例如羊毛甾醇和24,25-环氧羊毛甾醇。有趣的是,放射性掺入极性甾醇呈现双相反应,这与还原酶活性的双相反应呈反比。因此,在低浓度酮康唑(0.15 - 2微摩尔)时,[3H]甲羟戊酸内酯掺入极性甾醇增加,而在高浓度药物时降至对照值。用酮康唑(30微摩尔)和[3H]甲羟戊酸内酯处理细胞,然后去除药物和放射性标记,导致还原酶活性受到抑制,且放射性从羊毛甾醇和24,25-环氧羊毛甾醇重新分布到胆固醇和极性甾醇。这些结果表明,低浓度酮康唑(小于2微摩尔)对还原酶活性的抑制是由于甲基甾醇生成了调节性极性甾醇。在高浓度酮康唑(30微摩尔)时未观察到还原酶活性受到抑制,此时外源性添加的[3H]24(S),25-环氧羊毛甾醇向极性甾醇的转化被阻止。外源性添加的24,25-环氧羊毛甾醇以剂量依赖性方式抑制还原酶活性,而酮康唑(30微摩尔)可阻止低浓度环氧羊毛甾醇引起的抑制作用。然而,该药物无法阻止25-羟基羊毛甾醇(24,25-环氧羊毛甾醇的还原形式)对还原酶活性的剂量依赖性抑制。这些结果表明,24,25-环氧羊毛甾醇本身不是还原酶活性的抑制剂,但可通过对酮康唑敏感的细胞色素P-450依赖性反应代谢为调节性极性甾醇。用酮康唑处理细胞完全消除了低密度脂蛋白(LDL)对还原酶活性的抑制作用。(摘要截短至400字)