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大鼠肝微粒体和分离的肝细胞制剂中的雌激素代谢——I. 代谢物形成及与细胞大分子的不可逆结合

Estrogen metabolism in rat liver microsomal and isolated hepatocyte preparations--I. Metabolite formation and irreversible binding to cellular macromolecules.

作者信息

Brueggemeier R W, Kimball J G, Kraft F

出版信息

Biochem Pharmacol. 1984 Dec 1;33(23):3853-9. doi: 10.1016/0006-2952(84)90051-0.

DOI:10.1016/0006-2952(84)90051-0
PMID:6508837
Abstract

The metabolism of endogenous estrogens, estradiol and estrone, and the irreversible binding of estrogens to cellular macromolecules have been examined and compared in subcellular microsomal and in intact hepatocyte preparations. In studies with rat liver microsomal preparations containing estradiol, an NADPH-generating system, and denatured DNA, the irreversible binding of radiolabeled steroid metabolite(s) to the microsomal proteins was 3.26 nmoles/mg protein in 1 hr (S.D. 0.39; 7.9% of total steroid) while binding to DNA was found to be 0.288 nmole/mg DNA/mg protein (S.D. 0.025; 0.39% of total steroid). No significant difference was observed between microsomal preparations from untreated, phenobarbital-treated or 3-methylcholanthrene-treated rats. Irreversible binding to proteins was also demonstrated in the intact hepatocyte cell incubations. After 2-hr incubations of estradiol with hepatocytes, 5.9% (S.D. 1.4%) of the steroid(s) was irreversibly associated with cellular proteins (approximately 1.43 pmoles/mg/min). Analysis of the organic-soluble metabolites demonstrated the presence of the catechol estrogens and their metabolites, 2-hydroxyestradiol, 2-hydroxyestrone, 2-methoxyestradiol, and 2-methoxyestrone. Estrone and estriol were also identified. The aqueous-soluble materials isolated from hepatocyte incubations contained glucuronide, sulfate, and apparent thioether conjugates, as determined by liberation from estrogen metabolites by treatment with beta-glucuronidase, sulfatase, and Raney nickel. Thus, extensive primary and secondary metabolism of estrogens occurs in intact hepatocyte incubations. Furthermore, irreversible binding of estrogens to cellular proteins occurs in these intact cells having demonstrated conjugative pathways of metabolism.

摘要

在内源性雌激素(雌二醇和雌酮)的代谢以及雌激素与细胞大分子的不可逆结合方面,已在亚细胞微粒体和完整肝细胞制剂中进行了检测和比较。在含有雌二醇、NADPH生成系统和变性DNA的大鼠肝脏微粒体制剂研究中,放射性标记的类固醇代谢物与微粒体蛋白的不可逆结合在1小时内为3.26纳摩尔/毫克蛋白(标准差0.39;占总类固醇的7.9%),而与DNA的结合为0.288纳摩尔/毫克DNA/毫克蛋白(标准差0.025;占总类固醇的0.39%)。在未处理、苯巴比妥处理或3-甲基胆蒽处理的大鼠的微粒体制剂之间未观察到显著差异。在完整肝细胞培养中也证明了与蛋白质的不可逆结合。雌二醇与肝细胞孵育2小时后,5.9%(标准差1.4%)的类固醇与细胞蛋白不可逆结合(约1.43皮摩尔/毫克/分钟)。对有机可溶性代谢物的分析表明存在儿茶酚雌激素及其代谢物、2-羟基雌二醇、2-羟基雌酮、2-甲氧基雌二醇和2-甲氧基雌酮。还鉴定出了雌酮和雌三醇。通过用β-葡萄糖醛酸酶、硫酸酯酶和雷尼镍处理从雌激素代谢物中释放出来确定,从肝细胞培养物中分离出的水溶性物质含有葡萄糖醛酸苷、硫酸盐和明显的硫醚共轭物。因此,在完整肝细胞培养中发生了广泛的雌激素一级和二级代谢。此外,在这些已证明存在共轭代谢途径的完整细胞中,雌激素与细胞蛋白发生不可逆结合。

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