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Cytochrome P-450-dependent 14 α-demethylation of lanosterol in Candida albicans

机译:白色念珠菌中羊毛甾醇的细胞色素P-450依赖性14α-去甲基化

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pA novel assay for cytochrome P-450-dependent 14 alpha-sterol demethylase of the important opportunistic fungal pathogen, Candida albicans, is described. The enzyme was assayed in microsomal preparations (microsomes) by measuring the incorporation of [14C]lanosterol into (4,14)-desmethylated sterols. The efficacy of different cell-breakage methods was compared; desmethylated-sterol biosynthesis was maximal when cells were broken with a Braun disintegrator. The solubilization of [14C]lanosterol with detergent in the assay system was essential for enzyme activity, which was enhanced considerably when microsomes were gassed with O2. Under these conditions, there was a reciprocal relationship between the amount of radioactivity incorporated into desmethylated sterols and that lost from lanosterol. The major radiolabelled desmethylated sterol was ergosterol. The enzyme had an apparent Km of 52.73 +/- 2.80 microM and an apparent Vmax of 0.84 +/- 0.14 nmol/min per mg of protein (n = 3). Enzyme activity was decreased greatly when microsomes were treated with CO or the triazole antifungal ICI 153066./p
机译:描述了一种重要的机会性真菌病原体白色念珠菌的细胞色素P-450依赖性14α-甾醇脱甲基酶的新颖测定法。通过测量[14C]羊毛甾醇向(4,14)-去甲基化固醇中的掺入,在微粒体制剂(微粒体)中测定了该酶。比较了不同细胞破碎方法的功效;当用布劳恩崩解剂破碎细胞时,去甲基化固醇的生物合成最大。在测定系统中用去污剂溶解[14C]羊毛甾醇对于酶的活性是必不可少的,当微粒体中充满O2时,酶的活性会大大提高。在这些条件下,去甲基化固醇中掺入的放射性量与羊毛甾醇所损失的放射性量之间存在相互关系。放射性标记的主要去甲基化固醇是麦角固醇。该酶的表观Km为52.73 +/- 2.80 microM,表观Vmax为0.84 +/- 0.14 nmol / min / mg蛋白质(n = 3)。当用CO或三唑类抗真菌药物ICI 153066处理微粒体时,酶活性大大降低。

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