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Effect of cytochrome P450 and aldo-keto reductase inhibitors on progesterone inactivation in primary bovine hepatic cell cultures1

机译:细胞色素P450和醛基酮还原酶抑制剂对牛肝细胞原代孕酮失活的影响1

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摘要

Progesterone is required for maintenance of pregnancy, and peripheral concentrations of progesterone are affected by both production and inactivation. Hepatic cytochrome P450 (EC 1.14.14.1) and aldo-keto reductase (EC 1.1.1.145-151) enzymes play a pivotal role in the first step of steroid inactivation, which involves the addition of hydroxyl groups to various sites of the cyclopentanoperhydrophenanthrene nucleus. The current objective was to discern the proportional involvement of hepatic progesterone inactivating enzymes on progesterone decay using specific enzyme inhibitors. Ticlopidine, diltiazem, curcumin, dicumarol, and naproxen were used because of their selective inhibition of cytochrome P450s, aldo-keto reductases, and glucuronosyltransferases. Liver biopsies were collected from 6 lactating Holstein dairy cows, and cells were dissociated using a nonperfusion technique. Confluent wells were preincubated for 4 h with enzyme inhibitor and then challenged with progesterone for 1 h. Cell viability was unaffected by inhibitor treatment and averaged 84 ± 1%. In control wells, 50% of the progesterone had been inactivated after a 1-h challenge with 5 ng/mL of progesterone. Preincubation with curcumin, ticlopidine, or naproxen caused the greatest reduction in progesterone inactivation compared with controls and averaged 77, 39, or 37%, respectively. Hydroxyla-tion of 4-nitrophenol to 4-nitrocatechol in intact cells was inhibited by approximately 65% after treatment with curcumin or ticlopidine. Glucuronidation of phenol red or 4-nitrocatechol in intact cells was inhibited by treatment with curcumin, dicumarol, or naproxen. In cytoplasmic preparations, aldo-keto reductase 1C activity was inhibited by curcumin, dicumarol, or naproxenrntreatment. Microsomal cytochrome P450 2C activity was inhibited by treatment with curcumin or ticlopidine, whereas cytochrome P450 3A activity was inhibited by treatment with curcumin or diltiazem. The contribution of cytochrome P450 2C and cytochrome P450 3A enzymes to progesterone inactivation in bovine hepatic cell cultures was 40 and 15%, respectively. Depending on the inhibitor used, it would appear that the aldo-keto reductase enzymes contribute approximately 40% to the observed progesterone inactivation, although a portion of this inactivation may be attributed to the loss of glucuronosyltransferase activity. Future work focusing on decreasing the activity of these enzymes in vivo could lead to an increase in the bioavailability of progesterone.
机译:维持妊娠需要孕酮,孕酮的外周浓度受生产和失活的影响。肝细胞色素P450(EC 1.14.14.1)和醛基酮还原酶(EC 1.1.1.145-151)酶在类固醇失活的第一步中起关键作用,该过程涉及在环戊烷过氢菲核的各个位置添加羟基。目前的目标是使用特定的酶抑制剂来识别肝孕酮失活酶与孕酮衰变的比例关系。之所以使用噻氯匹定,地尔硫卓,姜黄素,地美洛尔和萘普生,是因为它们选择性抑制细胞色素P450,醛基酮还原酶和葡萄糖醛糖基转移酶。从6头泌乳的荷斯坦奶牛收集肝活检,并使用非灌注技术分离细胞。将融合孔与酶抑制剂预孵育4小时,然后用孕酮攻击1小时。细胞活力不受抑制剂处理的影响,平均为84±1%。在对照孔中,用5 ng / mL的孕酮激发1小时后,已使50%的孕酮失活。与姜黄素,噻氯匹定或萘普生的预孵育与对照组相比,孕酮失活的减少最大,平均分别为77%,39%或37%。用姜黄素或噻氯匹定处理后,完整细胞中的4-硝基苯酚羟基化为4-硝基邻苯二酚被抑制约65%。姜黄素,地美洛尔或萘普生处理可抑制完整细胞中酚红或4-硝基儿茶酚的葡萄糖醛酸苷化。在细胞质制剂中,姜黄素,二豆香酚或萘普生治疗可抑制醛酮还原酶1C的活性。姜黄素或噻氯匹定可抑制微粒体细胞色素P450 2C活性,姜黄素或地尔硫卓可抑制细胞色素P450 3A活性。细胞色素P450 2C和细胞色素P450 3A酶对牛肝细胞培养物中孕酮失活的贡献分别为40%和15%。取决于所使用的抑制剂,似乎醛-酮还原酶对观察到的孕酮失活贡献约40%,尽管这种失活的一部分可能归因于葡糖醛酸糖基转移酶活性的丧失。专注于降低体内这些酶活性的未来工作可能会导致孕酮的生物利用度增加。

著录项

  • 来源
    《Journal of dairy science》 |2010年第10期|p.4613-4624|共12页
  • 作者

    C. O. Lemley; M. E. Wilson;

  • 作者单位

    Division of Animal and Nutritional Sciences, Davis College of Agriculture, Natural Resources and Design, West Virginia University,Morgantown 26506;

    rnDivision of Animal and Nutritional Sciences, Davis College of Agriculture, Natural Resources and Design, West Virginia University,Morgantown 26506;

  • 收录信息 美国《科学引文索引》(SCI);美国《生物学医学文摘》(MEDLINE);美国《化学文摘》(CA);
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    cytochrome P450; aldo-keto reductase; progesterone decay; hepatic cell isolation;

    机译:细胞色素P450;醛酮还原酶;孕酮衰变;肝细胞分离;
  • 入库时间 2022-08-17 23:24:49

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