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首页> 外文期刊>Archives of Toxicology >Role of cytochrome P450c17alpha in dibromoacetic acid-induced testicular toxicity in rats.
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Role of cytochrome P450c17alpha in dibromoacetic acid-induced testicular toxicity in rats.

机译:细胞色素P450c17alpha在二溴乙酸诱导的大鼠睾丸毒性中的作用。

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Dibromoacetic acid (DBAA), a by-product formed during disinfection of drinking water, alters spermatogenesis in rats through defective spermiation. The mechanism underlying this toxicity is not fully understood. In this study, gene expression data generated with microarrays from testes were used to generate a mechanistic understanding of DBAA-induced testicular toxicity. Testes were collected from male Sprague-Dawley rats dosed orally for 1 and 4 days with DBAA at 250 mg/kg/day. At both time points, DBAA administration induced delayed spermiation in Stage X tubules and regulated the expression of a small number of genes, including a mild but consistent downregulation of cytochrome P450c17alpha (CYP17) mRNA, an enzyme expressed by Leydig cells and essential for the production of testicular androgens. Downregulation of CYP17 was confirmed at the protein level and its biological significance was substantiated by demonstrating reduced testicular testosterone levels in DBAA-dosed rats. Furthermore, testosterone production by human chorionic gonadotrophin (hCG)-stimulated rat primary Leydig cells was reduced following treatment with 100 muM DBAA. Collectively, these results indicate that DBAA can directly target rat Leydig cells and downregulate testicular CYP17 expression with a resulting decreased testicular testosterone production. This disruption of testicular steroidogenesis is likely to contribute to the mechanism of failed spermiation observed in rats following exposure to DBAA.
机译:二溴乙酸(DBAA)是在饮用水消毒过程中形成的副产物,可通过有缺陷的精子代谢改变大鼠的精子发生。这种毒性的潜在机制尚不完全清楚。在这项研究中,使用由睾丸微阵列产生的基因表达数据来产生对DBAA诱导的睾丸毒性的机械理解。从雄性Sprague-Dawley大鼠中收集睾丸,口服250 mg / kg /天的DBAA,持续1天和4天。在两个时间点,DBAA给药均可诱导X期肾小管的精子延迟发育,并调节少数基因的表达,包括轻度但持续下调细胞色素P450c17alpha(CYP17)mRNA,这是Leydig细胞表达的一种酶,对生产至关重要睾丸雄激素。 CYP17的下调在蛋白质水平得到证实,其生物学意义通过证明DBAA给药大鼠睾丸睾丸激素水平降低而得以证实。此外,用100μMDBAA处理后,人绒毛膜促性腺激素(hCG)刺激的大鼠原代Leydig细胞产生的睾丸激素减少。总体而言,这些结果表明DBAA可以直接靶向大鼠Leydig细胞并下调睾丸CYP17表达,从而导致睾丸睾丸激素产生减少。睾丸类固醇生成的这种破坏很可能导致了在暴露于DBAA后在大鼠中观察到的精子失败机制。

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