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卵巢蛋白在无细胞试验中对胎盘芳香化酶活性的抑制作用。

Inhibition of placental aromatase activity in a cell free assay by ovarian protein.

作者信息

Campeau J D, Myint T T, Ono T, Holmberg E A, Frederick J J, Kling O R, diZerega G S

出版信息

Exp Clin Endocrinol. 1986 Aug;87(3):247-55. doi: 10.1055/s-0029-1210553.

DOI:10.1055/s-0029-1210553
PMID:3780864
Abstract

Previously we identified a fraction of follicular fluid (follicle regulatory protein: FRP) which inhibits granulosa cell aromatase activity. During the course of these studies the question of FRP acting via autocrine as well as paracrine mechanisms arose in addition to the need for a more efficient method of screening for aromatase inhibitory activity during the purification of FRP. Accordingly, we assessed the effects of FRP on aromatase activity in a microsomal assay. Placental microsome preparations were preincubated for 20 minutes with or without FRP prior to a 20 minute incubation with testosterone. Significantly less conversion of testosterone to estrogen occurred with FRP compared to control preincubation. When follicular protein was added without pre-incubation, there was no apparent change in microsomal aromatase activity, whereas after a 20 minute pre-incubation with the follicular protein fraction, significantly less testosterone was converted into estrogen. When various concentrations of FRP were assayed in the placental aromatase assay, a dose-response curve demonstrated a 50% inhibitory dose (ID50) of approximately 400 micrograms/ml. To further purify the aromatase inhibitory activity, 5 mg of the crude follicular fluid preparation was eluted through an anion exchange column via HPLC using a sodium acetate gradient. The fractions in the central elution peak contained aromatase inhibitor activity with ID50 values of 25-160 micrograms/ml. Thus Fractions were further purified by elution through a gel exclusion column via HPLC which demonstrated inhibition of cell free placental aromatase activity in the 15,000-18,000 molecular weight range with an ID50 of 5 micrograms/ml.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

此前我们鉴定出了卵泡液中的一部分(卵泡调节蛋白:FRP),它可抑制颗粒细胞芳香化酶的活性。在这些研究过程中,除了在纯化FRP期间需要一种更有效的筛选芳香化酶抑制活性的方法外,还出现了FRP通过自分泌以及旁分泌机制发挥作用的问题。因此,我们在微粒体测定中评估了FRP对芳香化酶活性的影响。在与睾酮孵育20分钟之前,将胎盘微粒体制剂与或不与FRP预孵育20分钟。与对照预孵育相比,FRP存在时睾酮向雌激素的转化明显减少。当未预孵育就添加卵泡蛋白时,微粒体芳香化酶活性没有明显变化,而在用卵泡蛋白组分预孵育20分钟后,转化为雌激素的睾酮明显减少。当在胎盘芳香化酶测定中检测不同浓度的FRP时,剂量反应曲线显示50%抑制剂量(ID50)约为400微克/毫升。为了进一步纯化芳香化酶抑制活性,使用醋酸钠梯度通过HPLC将5毫克粗卵泡液制剂通过阴离子交换柱洗脱。中心洗脱峰中的组分含有芳香化酶抑制剂活性,ID50值为25 - 160微克/毫升。因此,通过HPLC通过凝胶排阻柱洗脱进一步纯化这些组分,其显示在分子量15,000 - 18,000范围内对无细胞胎盘芳香化酶活性有抑制作用,ID50为5微克/毫升。(摘要截断于250字)

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