Pettersson Hanna, Holmberg Lisa, Axelson Magnus, Norlin Maria
Department of Pharmaceutical Biosciences, Division of Biochemistry, University of Uppsala, Sweden.
FEBS J. 2008 Apr;275(8):1778-89. doi: 10.1111/j.1742-4658.2008.06336.x. Epub 2008 Mar 7.
CYP7B1, a cytochrome P450 enzyme, metabolizes several steroids involved in hormonal signaling including 5alpha-androstane-3beta,17beta-diol (3beta-Adiol), an estrogen receptor agonist, and dehydroepiandrosterone, a precursor for sex hormones. Previous studies have suggested that CYP7B1-dependent metabolism involving dehydroepiandrosterone or 3beta-Adiol may play an important role for estrogen receptor beta-mediated signaling. However, conflicting data are reported regarding the influence of different CYP7B1-related steroids on estrogen receptor beta activation. In the present study, we investigated CYP7B1-mediated conversions of dehydroepiandrosterone and 3beta-Adiol in porcine microsomes and human kidney cells. As part of these studies, we compared the effects of 3beta-Adiol (a CYP7B1 substrate) and 7alpha-hydroxy-dehydroepiandrosterone (a CYP7B1 product) on estrogen receptor beta activation. The data obtained indicated that 3beta-Adiol is a more efficient activator, thus lending support to the notion that CYP7B1 catalysis may decrease estrogen receptor beta activation. Our data on metabolism indicate that the efficiencies of CYP7B1-mediated hydroxylations of dehydroepiandrosterone and 3beta-Adiol are very similar. The enzyme catalyzed both reactions at a similar rate and the K(cat)/K(m) values were in the same order of magnitude. A high dehydroepiandrosterone/3beta-Adiol ratio in the incubation mixtures, similar to the ratio of these steroids in many human tissues, strongly suppressed CYP7B1-mediated 3beta-Adiol metabolism. As the efficiencies of CYP7B1-mediated hydroxylation of dehydroepiandrosterone and 3beta-Adiol are similar, we propose that varying steroid concentrations may be the most important factor determining the rate of CYP7B1-mediated metabolism of dehydroepiandrosterone or 3beta-Adiol. Consequently, tissue-specific steroid concentrations may have a strong impact on CYP7B1-dependent catalysis and thus on the levels of different CYP7B1-related steroids that can influence estrogen receptor beta signaling.
细胞色素P450酶CYP7B1可代谢多种参与激素信号传导的类固醇,包括雌激素受体激动剂5α-雄烷-3β,17β-二醇(3β-二醇)以及性激素前体脱氢表雄酮。先前的研究表明,涉及脱氢表雄酮或3β-二醇的CYP7B1依赖性代谢可能在雌激素受体β介导的信号传导中起重要作用。然而,关于不同CYP7B1相关类固醇对雌激素受体β激活的影响,报道的数据相互矛盾。在本研究中,我们研究了猪微粒体和人肾细胞中CYP7B1介导的脱氢表雄酮和3β-二醇的转化。作为这些研究的一部分,我们比较了3β-二醇(一种CYP7B1底物)和7α-羟基-脱氢表雄酮(一种CYP7B1产物)对雌激素受体β激活的影响。获得的数据表明,3β-二醇是一种更有效的激活剂,因此支持了CYP7B1催化可能会降低雌激素受体β激活的观点。我们的代谢数据表明,CYP7B1介导的脱氢表雄酮和3β-二醇羟基化效率非常相似。该酶以相似的速率催化这两种反应,且催化常数与米氏常数的比值处于同一数量级。孵育混合物中脱氢表雄酮/3β-二醇的高比例,类似于许多人体组织中这些类固醇的比例,强烈抑制了CYP7B1介导的3β-二醇代谢。由于CYP7B1介导的脱氢表雄酮和3β-二醇羟基化效率相似,我们认为不同的类固醇浓度可能是决定CYP7B1介导的脱氢表雄酮或3β-二醇代谢速率的最重要因素。因此,组织特异性类固醇浓度可能对CYP7B1依赖性催化有强烈影响,进而影响可影响雌激素受体β信号传导的不同CYP7B1相关类固醇的水平。
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