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Alteration in sexually dimorphic testosterone biotransformation profiles as a biomarker of chemically induced androgen disruption in mice.

机译:性二态性睾丸激素生物转化谱的变化作为小鼠中化学诱导的雄激素破坏的生物标记。

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摘要

Assessment of the impact of environmental chemicals on androgen homeostasis in rodent models is confounded by high intraindividual and interindividual variability in circulating testosterone levels. Our goal was to evaluate changes in testosterone biotransformation processes as a measure of androgen homeostasis and as a biomarker of exposure to androgen-disrupting chemicals. Sex-specific differences in hepatic testosterone biotransformation enzyme activities were identified in CD-1 mice. Gonadectomy followed by replacement of individual steroid hormones identified specific sex differences in biotransformation profiles that were due to the inductive or suppressive effects of testosterone. Notably, significant androgen-dependent differences in testosterone 6[alpha]- and 15[alpha]-hydroxylase activities were demonstrated, and the ratio of 6[alpha]- and 15[alpha]-hydroxylase activities proved to be an excellent indicator of the androgen status within the animal. The male or "masculinized" testosterone 6[alpha]/15[alpha]-hydroxylase ratio was significantly less than the female or "feminized" ratio. Male mice were exposed to both an antiandrogen, vinclozolin, and to a compound that modulates serum androgen levels, indole-3-carbinol, to test the utility of this ratio as a biomarker of androgen disruption. Treatment with the antiandrogen vinclozolin significantly increased the 6[alpha]/15[alpha]-hydroxylase ratio. Indole-3-carbinol treatment resulted in a dose-dependent, but highly variable, decrease in serum testosterone levels. The 6[alpha]/15[alpha]-hydroxylase ratio increased as serum testosterone levels decreased in these animals. However, the increase in the ratio was much less variable and more sensitive than serum testosterone levels. These investigations demonstrate that the 6[alpha]/15[alpha]-hydroxylase ratio is a powerful measure of androgen modulation and a sensitive indicator of exposure to androgen-disrupting chemicals in CD-1 mice.
机译:啮齿动物模型中环境化学物质对雄激素稳态的影响评估与循环睾丸激素水平的高个体内和个体间变异性混淆。我们的目标是评估睾丸激素生物转化过程的变化,以衡量雄激素的体内稳态,并作为暴露于破坏雄激素的化学物质的生物标记。在CD-1小鼠中鉴定出肝脏睾丸激素生物转化酶活性的性别特异性差异。进行了性腺切除术,然后更换了单独的类固醇激素,从而确定了生物转化谱中的特定性别差异,这是由于睾丸激素的诱导或抑制作用所致。值得注意的是,证明了睾丸激素6α-和15α-羟化酶活性的显着的雄激素依赖性差异,并且6α-和15α-羟化酶活性的比例被证明是该活性的极好的指标。动物体内的雄激素状态。男性或“男性化”睾丸激素6α/15α-羟化酶的比例明显小于女性或“女性化”比例。将雄性小鼠暴露于抗雄激素长春新唑啉和调节血清雄激素水平的化合物吲哚-3-甲醇,以测试该比率作为破坏雄激素的生物标志物的效用。用抗雄激素长春新唑啉治疗显着增加了6α/15α-羟化酶的比例。吲哚-3-甲醇的治疗导致血清睾丸激素水平呈剂量依赖性但高度可变。在这些动物中,随着血清睾丸激素水平的降低,6α/15α-羟化酶的比例增加。但是,该比值的增加与血清睾丸激素水平相比变化不大且更敏感。这些研究表明,6α/15α-羟化酶比率是雄激素调节的有效量度,并且是在CD-1小鼠中暴露于破坏雄激素的化学物质的敏感指标。

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