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首页> 外文期刊>Archives of Toxicology >Ability of the Hershberger assay protocol to detect thyroid function modulators.
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Ability of the Hershberger assay protocol to detect thyroid function modulators.

机译:Hershberger分析规程检测甲状腺功能调节剂的能力。

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In vivo screening methods for detection of thyroid function modulators are now under development in many research laboratories. We assessed the applicability of the Hershberger assay protocol to screen for thyroid function modulators. In experiment 1, castrated male BrlHan WIST@Jcl (GALAS) rats were administered a potent thyroid peroxidase inhibitor, 3-amino-1,2,4-triazole (AT), in doses of 0, 40, 200, and 1,000 mg/kg/day with gravimetric endpoint, and in experiment 2, castrated and intact male rats were administered in doses of 0, 40, and 200 mg/kg/day, with quantification of the extent of hypertrophy of the thyroid epithelium, to assess the effects of castration, by gavage to 8-week-old for 10 consecutive days. At necropsy of both experiments, the thyroid glands and hypophysis were collected and fixed with 10% neutral-buffered formalin. To avoid crushing during weighing because of their fragility, the thyroid glands and hypophysis were weighed approximately 24 h after fixation with 10% neutral-buffered formalin. All animals were sacrificed approximately 24 h after the final dose. In experiment 2, the thyroid glands of all animals were stained with hematoxylin and eosin for histological examination and morphometry of follicular epithelial height. In experiment 1, absolute and relative thyroid weights in all of the AT groups were statistically increased in a dose-dependent manner, regardless of the testosterone propionate (TP)-injection. In experiment 2, the results showed a significant increase in thyroid weight in the 200 mg/kg groups of both castrated and intact rats. Hypophyseal weight was unaltered by AT, but comparison of vehicle-treated groups showed that the hypophyseal weight of the castrated rats was greater than that of the intact rats. Enlarged thyroid glands were observed in the AT-treated rats at necropsy. Histological examination of the thyroid glands of all the AT-treated animals showed hypertrophy and hyperplasia of the follicular epithelial cells, and the height of follicular epithelium of the thyroid glands increased in a dose-dependent manner in both the castrated and intact rats. In experiment 1, assessment of the (anti-) androgenic action of AT in seminal vesicle weight revealed a significant increase in the 200 and 1,000 mg/kg + TP groups in a dose-dependent manner. These results suggest that the effect of AT can be detected by the Hershberger assay 10-day administration protocol and may be useful for screening for thyroid function modulators regardless of whether the animals have been castrated.
机译:现在,许多研究实验室正在开发用于检测甲状腺功能调节剂的体内筛选方法。我们评估了Hershberger分析规程筛查甲状腺功能调节剂的适用性。在实验1中,给去势雄性BrlHan WIST @ Jcl(GALAS)雄性大鼠施用了一种有效的甲状腺过氧化物酶抑制剂3-氨基-1,2,4-三唑(AT),剂量为0、40、200和1,000 mg / kg /天,具有重量终点,在实验2中,以0、40和200 mg / kg /天的剂量给予cast割和完整的雄性大鼠,量化甲状腺上皮的肥大程度,以评估其作用连续10天对8周大的鸡进行cast割。在两个实验的尸检中,收集甲状腺和垂体并用10%中性缓冲的福尔马林固定。为避免称量过程中因其易碎而压碎,在用10%中性缓冲福尔马林固定后约24小时,称量甲状腺和垂体。在最终剂量后约24小时处死所有动物。在实验2中,所有动物的甲状腺均用苏木精和曙红染色,以进行组织学检查和卵泡上皮高度的形态测定。在实验1中,无论是否注射丙酸睾丸激素(TP),所有AT组的甲状腺绝对重量和相对甲状腺重量均以剂量依赖性方式统计增加。在实验2中,结果显示,在200 mg / kg的rated割和完整大鼠组中,甲状腺重量显着增加。垂体后叶的重量并没有被AT所改变,但是对媒介物治疗组的比较显示,去势大鼠的下垂肌的重量大于完整大鼠的。尸检时在经AT处理的大鼠中观察到甲状腺增大。组织学检查的所有接受AT治疗的动物的甲状腺均显示卵泡上皮细胞肥大和增生,并且在the割和完整的大鼠中,甲状腺的卵泡上皮高度均呈剂量依赖性增加。在实验1中,对AT对精囊重量的(抗)雄激素作用的评估显示,200和1,000 mg / kg + TP组的剂量依赖性显着增加。这些结果表明,可以通过Hershberger分析10天给药方案来检测AT的作用,并且不管是否已cast割动物,对于筛选甲状腺功能调节剂都可能有用。

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