Kortner Trond M, Arukwe Augustine
Department of Biology, Norwegian University of science and Technology (NTNU) Høgskoleringen 5, 7491 Trondheim, Norway.
Comp Biochem Physiol C Toxicol Pharmacol. 2007 Nov;146(4):569-80. doi: 10.1016/j.cbpc.2007.07.001. Epub 2007 Jul 17.
Steroid hormone (estrogens and androgens) synthesis and regulation involve a large number of enzymes and potential biochemical pathways. In the context of these biochemical pathways, it is believed that the true rate-limiting step in acute steroid production is the movement of cholesterol across the mitochondrial membrane by the steroidogenic acute regulatory (StAR) protein and the subsequent conversion to pregnenolone by cytochrome P450-mediated side-chain cleavage (P450scc) enzyme. Oocyte development is a complex process that is triggered by the maturation-promoting factor (MPF) involving cyclin-B as a regulatory factor. In the present study, we evaluated the endocrine effects of 17alpha-methyltestosterone (MT) on steroidogenic pathways of Atlantic cod (Gadus morhua), using an in vitro previtellogenic oocyte culture technique that is based on an agarose floating method. Tissue was cultured in a humidified incubator at 10 degrees C for 1, 5, 10 and 20 days with different concentrations of the synthetic androgen MT (0 (control), 1, 10, 100 and 1000 microM) dissolved in ethanol (0.3%). Gene expressions for StAR, P450scc, aromatase-alpha (P450aromA) and cyclin-B were detected using validated real-time PCR with specific primer pairs. Cellular localization of the StAR protein and P450scc were performed using the immunohistochemical technique with antisera prepared against synthetic peptide for both proteins. Steroid hormones (estradiol-17beta: E2 and testosterone: T) levels were estimated using enzyme immunoassay. Our data showed significant concentration-specific increase (at day 1 and 5) and decrease (at day 10 and 20) of the StAR mRNA expression after exposure to MT. P450scc expression showed a MT concentration-specific decrease during the exposure periods and cyclin-B mRNA expression was decreased in MT concentration-dependent manner at days 10 and 20 (reaching almost total inhibition after exposure to 1000 microM MT). MT exposure produced variable effects on the P450aromA mRNA expression that can be described as concentration-specific increase (day 1) and decrease (days 5 and 10). Cellular localization of the StAR protein and P450scc demonstrated their expression mainly in ovarian follicular cells. MT produced an apparent concentration-and time-dependent increase of E2 and T levels. Thus, the present study reveals some novel effects of pharmaceutical endocrine disruptor on the development of previtellogenic oocytes in cod. The impaired steroidogenesis and hormonal imbalance reported in the present study may have potential consequences for the vitellogenic process and overt fecundity in teleosts.
类固醇激素(雌激素和雄激素)的合成与调节涉及大量酶和潜在的生化途径。在这些生化途径的背景下,人们认为急性类固醇生成的真正限速步骤是类固醇生成急性调节(StAR)蛋白介导胆固醇穿过线粒体膜,以及随后细胞色素P450介导的侧链裂解(P450scc)酶将其转化为孕烯醇酮。卵母细胞发育是一个复杂的过程,由成熟促进因子(MPF)触发,其中细胞周期蛋白B作为调节因子。在本研究中,我们使用基于琼脂糖漂浮法的体外卵黄生成前卵母细胞培养技术,评估了17α-甲基睾酮(MT)对大西洋鳕鱼(Gadus morhua)类固醇生成途径的内分泌影响。将组织在湿度培养箱中于10℃培养1、5、10和20天,分别添加不同浓度(0(对照)、1、10、100和1000微摩尔)溶解于乙醇(0.3%)中的合成雄激素MT。使用经过验证的实时PCR和特异性引物对检测StAR、P450scc、芳香化酶-α(P450aromA)和细胞周期蛋白B的基因表达。使用针对这两种蛋白质的合成肽制备的抗血清,通过免疫组织化学技术对StAR蛋白和P450scc进行细胞定位。使用酶免疫测定法估计类固醇激素(雌二醇-17β:E2和睾酮:T)水平。我们的数据显示,暴露于MT后,StAR mRNA表达在第1天和第5天显著呈浓度特异性增加,在第10天和第20天显著降低。P450scc表达在暴露期间呈MT浓度特异性降低,细胞周期蛋白B mRNA表达在第10天和第20天呈MT浓度依赖性降低(暴露于1000微摩尔MT后几乎完全抑制)。MT暴露对P450aromA mRNA表达产生了可变影响,可描述为浓度特异性增加(第1天)和降低(第5天和第10天)。StAR蛋白和P450scc的细胞定位表明它们主要在卵巢滤泡细胞中表达。MT使E2和T水平明显呈浓度和时间依赖性增加。因此,本研究揭示了药物内分泌干扰物对鳕鱼卵黄生成前卵母细胞发育的一些新影响。本研究中报道的确类固醇生成受损和激素失衡可能对硬骨鱼的卵黄生成过程和明显繁殖力产生潜在影响。
