Uilenbroek J T, Durlinger A L, Tebar M, Kramer P, van Schaik R H, Wierikx C D, de Jong F H
Department of Endocrinology and Reproduction, Faculty of Medicine and Health Sciences, Erasmus University, Rotterdam, The Netherlands.
J Endocrinol. 1998 Nov;159(2):331-40. doi: 10.1677/joe.0.1590331.
This study aimed to investigate the time course of disappearance of the mRNAs of the various subunits of inhibin in follicles which become atretic. An animal model was used in which atresia of preovulatory follicles could be studied in a chronological order. Injection of gonadotrophin-releasing hormone (GnRH) antagonist (20 microg) at the morning of pro-oestrus (P) blocked ovulation and the 10-12 preovulatory follicles became gradually atretic. A second injection was given the next day to prevent delayed ovulation. The rate of atresia could be delayed by simultaneous administration of a subovulatory dose of human chorionic gonadotrophin (hCG) (0.5 IU) and could be advanced by administration of a fivefold larger amount of GnRH antagonist. Functional activity of follicles becoming atretic was studied by measuring oestradiol production after incubation of individual follicles for 4 h. Follicles isolated 24 h after the first injection of GnRH antagonist (P+24) already secreted significantly less oestradiol in vitro than follicles isolated at pro-oestrus, although they were morphologically not different from pro-oestrous follicles. Follicles isolated at P+24 from hCG-treated rats secreted more oestradiol compared with follicles from rats not treated with hCG. In contrast, follicles isolated at P+24 from rats that were given a fivefold larger amount of GnRH antagonist secreted less oestradiol. Once this model was validated, temporal changes in inhibin subunit mRNAs in follicles undergoing atresia were measured by in situ hybridization and RNase protection assay. In situ hybridization showed abundant alpha- and betaA-subunit mRNA in the whole granulosa layer of preovulatory follicles at P and P+24, while betaB-subunit mRNA was restricted to the antral layer and cumulus. At P+48 the amount of alpha- and betaA-subunit mRNA had declined and was restricted to the cumulus, whereas betaB-subunit mRNA was absent. In the atretic follicles present at P+72 and P+96, mRNAs of all three inhibin subunits were absent. Administration of 0.5 IU hCG delayed the decline in the amount of alpha, betaA and betaB mRNA in preovulatory follicles at P+48. RNase protection assay of inhibin subunits in isolated follicles revealed no changes between P and P+24. However, at P+48, the mRNAs of alpha- and betaA-subunits were decreased. Expression of the mRNA of betaB-subunit declined gradually from P to P+48. The present study demonstrates that in follicles which are becoming atretic, mRNAs of alpha- and betaA-subunits decline simultaneously with the appearance of pycnotic cells in the granulosa layer, while betaB-subunit mRNA declines earlier, simultaneously with the decrease in the ability to secrete oestradiol in vitro.
本研究旨在探讨闭锁卵泡中抑制素各亚基mRNA消失的时间进程。采用了一种动物模型,在该模型中可按时间顺序研究排卵前卵泡的闭锁情况。在动情前期(P)上午注射促性腺激素释放激素(GnRH)拮抗剂(20微克)可阻断排卵,10 - 12个排卵前卵泡逐渐闭锁。次日进行第二次注射以防止排卵延迟。同时给予低于排卵剂量的人绒毛膜促性腺激素(hCG)(0.5国际单位)可延缓闭锁速率,而给予五倍剂量的GnRH拮抗剂则可加速闭锁。通过测量单个卵泡孵育4小时后的雌二醇分泌量来研究闭锁卵泡的功能活性。首次注射GnRH拮抗剂后24小时(P + 24)分离的卵泡,尽管其形态与动情前期卵泡无差异,但体外分泌的雌二醇明显少于动情前期分离的卵泡。与未用hCG处理的大鼠卵泡相比,hCG处理的大鼠在P + 24分离的卵泡分泌的雌二醇更多。相反,给予五倍剂量GnRH拮抗剂的大鼠在P + 24分离的卵泡分泌的雌二醇较少。该模型验证后,通过原位杂交和核糖核酸酶保护试验测量闭锁卵泡中抑制素亚基mRNA的时间变化。原位杂交显示,在P和P + 24时,排卵前卵泡的整个颗粒层中存在丰富的α - 和βA - 亚基mRNA,而βB - 亚基mRNA局限于卵泡腔层和卵丘。在P + 48时,α - 和βA - 亚基mRNA的量下降并局限于卵丘,而βB - 亚基mRNA消失。在P + 72和P + 96时存在的闭锁卵泡中,所有三种抑制素亚基的mRNA均不存在。给予0.5国际单位hCG可延缓P + 48时排卵前卵泡中α、βA和βB mRNA量的下降。对分离卵泡中抑制素亚基的核糖核酸酶保护试验显示,P和P + 24之间无变化。然而,在P + 48时,α - 和βA - 亚基的mRNA减少。βB - 亚基mRNA的表达从P到P + 48逐渐下降。本研究表明,在正在闭锁的卵泡中,α - 和βA - 亚基的mRNA与颗粒层中固缩细胞的出现同时下降,而βB - 亚基mRNA下降较早,与体外雌二醇分泌能力的下降同时发生。
