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绵羊垂体前叶体外产生卵泡抑素。

Ovine anterior pituitary production of follistatin in vitro.

作者信息

Farnworth P G, Thean E, Robertson D M, Schwartz J

机构信息

Prince Henry's Institute of Medical Research, Clayton, Victoria, Australia.

出版信息

Endocrinology. 1995 Oct;136(10):4397-406. doi: 10.1210/endo.136.10.7664660.

Abstract

Rat pituitary cells express messenger RNA for the activin-binding protein, follistatin (FS), and rat and bovine pituitary cell cultures secrete FS into the medium. In the present study, a previously validated, heterologous RIA for ovine FS was employed to investigate FS synthesis, secretion, and regulation in cultures of ovine anterior pituitary cells. The validity of the RIA was confirmed by the finding that FS immunoreactivity in ovine pituitary cell culture-conditioned medium diluted in parallel with purified bovine FS, and fractionation of the conditioned medium resulted in the coelution of activin-binding activity with the FS immunoactivity. The concentration of endogenous ovine FS achieved in the culture medium (0.08-0.6 nM) was in the range over which bovine FS suppresses FSH secretion in these cultures (IC50 = 0.5 nM). To characterize the relationship between endogenous FS and FSH secretion, dispersed ovine pituitary cells were preincubated with 10% fetal bovine serum for 2 days, then cultured between days 2-5 in the presence of a chemically defined serum substitute. Under these conditions, FS was continuously secreted at a rate of 12.1 +/- 1.8 ng/10(6) cells.day (mean +/- SEM; n = 18), whereas FSH was secreted at 64 +/- 13 ng/10(6) cells.day (n = 7). The secretion of FS and FSH changed in a reciprocal way as culture conditions were altered either by maintaining exposure of the cells to fetal bovine serum or by plating the cells at a 6- to 10-fold higher seeding density. Under the latter circumstance, for instance, FS secretion during the 3-day test period decreased to 47 +/- 14% (n = 10) and FSH secretion increased to 137 +/- 6% (n = 6) of the respective values in cultures of dispersed cells. FS secretion was increased nearly 3-fold (P < 0.05) in a dose-dependent manner by continuous exposure of ovine pituitary cells between days 2-5 to recombinant human activin A (1-10 nM), which concomitantly increased FSH secretion. Recombinant human inhibin A (0.003-10 nM); the synthetic glucocorticoids, RU28362 and dexamethasone (each 1-100 nM); the sex steroids, testosterone (1-100 nM), 17 beta-estradiol (0.001-5 nM), and progesterone (4-2500 nM); and the vitamin A derivative, retinoic acid (0.3-32 microM), each inhibited FSH secretion from these cultures, but only the last agent significantly (P < 0.05) increased FS secretion. Inhibin prevented the stimulation of FSH secretion by activin A without affecting its stimulation of FS secretion.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

大鼠垂体细胞表达激活素结合蛋白卵泡抑素(FS)的信使核糖核酸,并且大鼠和牛的垂体细胞培养物会将FS分泌到培养基中。在本研究中,使用一种先前经验证的、用于绵羊FS的异源放射免疫分析法(RIA)来研究绵羊垂体前叶细胞培养物中FS的合成、分泌及调控。通过以下发现证实了该RIA的有效性:绵羊垂体细胞培养条件培养基中的FS免疫反应性与纯化的牛FS呈平行稀释,并且对条件培养基进行分级分离后,激活素结合活性与FS免疫活性共洗脱。培养基中内源性绵羊FS达到的浓度(0.08 - 0.6 nM)处于牛FS抑制这些培养物中促卵泡激素(FSH)分泌的浓度范围内(半数抑制浓度[IC50] = 0.5 nM)。为了表征内源性FS与FSH分泌之间的关系,将分散的绵羊垂体细胞用10%胎牛血清预孵育2天,然后在第2 - 5天于化学限定的血清替代物存在的情况下进行培养。在这些条件下,FS以12.1±1.8 ng/10⁶细胞·天的速率持续分泌(平均值±标准误;n = 18),而FSH以64±13 ng/10⁶细胞·天的速率分泌(n = 7)。当通过维持细胞与胎牛血清的接触或通过以高6至10倍的接种密度接种细胞来改变培养条件时,FS和FSH的分泌呈相反变化。例如,在后者情况下,3天测试期内FS分泌降至分散细胞培养物中各自值的47±14%(n = 10),而FSH分泌增至137±6%(n = 6)。通过在第2 - 5天将绵羊垂体细胞持续暴露于重组人激活素A(1 - 10 nM),FS分泌以剂量依赖性方式增加近3倍(P < 0.05),同时FSH分泌也增加。重组人抑制素A(0.00³ - 10 nM);合成糖皮质激素RU28362和地塞米松(各1 - 100 nM);性类固醇睾酮(1 - 100 nM)、17β - 雌二醇(0.001 - 5 nM)和孕酮(4 - 2500 nM);以及维生素A衍生物视黄酸(0.3 - 32 μM),均抑制这些培养物中FSH的分泌,但只有最后一种试剂显著(P < 0.05)增加FS分泌。抑制素可阻止激活素A对FSH分泌的刺激,而不影响其对FS分泌的刺激。(摘要截断于400字)

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