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>Cholesterol biosynthesis from lanosterol: development of a novel assay method and characterization of rat liver microsomal lanosterol Δ24-reductase
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Cholesterol biosynthesis from lanosterol: development of a novel assay method and characterization of rat liver microsomal lanosterol Δ24-reductase
pThe membrane-bound sterol Δsup24/sup-reductase (24-reductase) catalyses anaerobic reduction of the 24(25)-enes of lanosterol and other obligatory intermediates of cholesterol biosynthesis from lanosterol. A novel assay method and properties of the 24-reductase are described. More than a 120-fold induction of the 24-reductase activity was achieved by feeding rats a diet containing 5% cholestyramine plus 0.1% lovastatin in chow and by modulating diurnal variation. With this enzyme induction condition, lanosterol was converted efficiently into dihydrolanosterol in both intact hepatic microsomes and freshly isolated hepatocytes only when either miconazole or CO was added to inhibit 14α-demethylation of lanosterol. AR45 cells, which are deficient in 14α-methyl demethylase (14α-DM), exhibit lanosterol 24-reductase activity without addition of either CO or miconazole. Conversely, inhibition of the 24-reductase was not required for the expression of 14α-DM activity. Studies on the substrate specificities for the 24-reductase using different 24(25)-enes showed that the most reactive substrate was 5α-cholesta-7,24-dien-3β-ol, which exhibited a maximal 18-fold higher ik/isubcat/sub than that of lanosterol without the aid of the 14α-DM inhibitor. In addition, both the kinetic behaviour of lanosterol substrate in relation to the 24-reductase and a non-competitive inhibition mode of U18666A (iK/isubi/sub 0.157 iμ/iM) as well as Triparanol (iK/isubi/sub 0.523 iμ/iM), two well-known 24-reductase inhibitors, were determined. On the basis of our new findings on the preferred substrate and on the negative effect of 14α-DM on the 24-reductase, we suggest that C-24 reduction of sterols takes place straight after sterol Δsup8→7/sup isomerization of zymosterol, which occurs several steps after C-32 demethylation of lanosterol in the 19-step pathway of cholesterol biosynthesis from lanosterol./p
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机译:>膜结合固醇Δ 24 -还原酶(24-还原酶)催化羊毛甾醇的24(25)-烯和其他必需的胆固醇生物合成中间体的厌氧还原。描述了一种新颖的测定方法和24-还原酶的性质。通过给大鼠喂食含5%胆甾醇胺加0.1%洛伐他汀的饮食并调节昼夜变化,可实现24-还原酶活性的120倍以上诱导。在这种酶诱导条件下,仅当添加咪康唑或CO抑制羊毛脂的14α-去甲基化时,羊毛脂才能在完整的肝微粒体和新鲜分离的肝细胞中有效地转化为二氢羊毛甾醇。缺乏14α-甲基脱甲基酶(14α-DM)的AR45细胞在不添加CO或咪康唑的情况下表现出羊毛甾醇24-还原酶活性。相反,表达14α-DM活性不需要抑制24-还原酶。使用不同的24(25)-烯对24-还原酶的底物特异性的研究表明,反应性最强的底物是5α-cholesta-7,24-dien-3β-ol,其表现出的最高最高18倍 k cat 比羊毛甾醇没有14α-DM抑制剂的帮助。此外,羊毛甾醇底物与24-还原酶有关的动力学行为和U18666A( K i 0.157  μ M)以及Triparanol( K i 0.523  μ M)这两种著名的24-还原酶抑制剂,被确定。根据我们对优选底物的新发现以及14α-DM对24-还原酶的负面影响,我们建议固醇的C-24还原是在固醇Δ 8→7 zyostererol的异构化,发生在羊毛甾醇从胆固醇生物合成的19步途径中,羊毛甾醇C-32脱甲基后的数个步骤。
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