Choi D, Putowski L T, Fielder P J, Rosenfeld R G, Rohan R M, Adashi E Y
Department of Obstetrics and Gynecology, University of Maryland School of Medicine, Baltimore 21201, USA.
J Soc Gynecol Investig. 1996 May-Jun;3(3):145-51.
Because of the potential importance of insulin-like growth factor binding protein-4 (IGFBP-4) to ovarian physiology and the obvious limitations imposed by in vivo-exclusive experimental paradigms, we set out to delineate the characteristics and hormonal regulation of granulosa cell-derived IGFBP-4 under in vitro circumstances.
Granulosa cells obtained by follicular puncture of the ovaries from diethylstilbestrol-primed intact immature rats were subjected to culture for up to 72 hours. Insulin-like growth factor binding protein-4 mRNA extracted from culture was subjected to Northern blot hybridization. Data normalization was assured by reprobing with the hamster Chinese hamster ovary B (CHOB) cDNA, and the IGFBP-4/CHOB ratio was calculated. Conditioned culture media were subjected to Western ligand blot before and after immunoprecipitation with a rat IGFBP-4-directed polyclonal antiserum (alpha-B104).
Immunoprecipitation studies revealed granulosa cell-derived IGFBP-4 to be composed of a major 24-kDa species as well as a relatively minor 27-kDa moiety. Given cultures of untreated granulosa cells from immature estrogen-treated rats, transcripts corresponding to IGFBP-4 displayed an initial temporary decline culminating in a 6-hour nadir (a decrease of 67%; P < .05) followed by relatively prompt recovery (within 24 hours) to levels comparable to those noted at the outset of the culture (time 0). However, additional (albeit statistically insignificant) increments were noted at the 48-hour (but not 72-hour) time point. Treatment of granulosa cells with increasing concentration of FSH resulted in decrements of up to 30% (P < .05) in the steady-state levels of IGFBP-4 transcripts. A modest, biphasic, time-dependent response was noted for IGFBP-4 transcripts after treatment with high-dose FSH (100 ng/mL), an effect characterized by 24- and 48-hour increments (51% [P < .05] and 26% [P = .052] over untrated controls, respectively) and a 72-hour decrement (25%; P = .16). The concurrent provision of the C19 aromatase substrate androstenedione (10(-7) mol/L) to the culture medium from 72 hours enhanced the inhibitory effect of FSH (100 ng/mL) for a maximal decrement in IGFBP-4 transcripts of 49% (P < .05). Treatment with insulin-like growth factor (IGF)-I produced limited inhibition (up to 26%) of the steady-state levels of IGFBP-4 transcripts (P < .05).
Findings indicate the existence of heterogeneously-sized IGFBP-4 species, of which the 27-kDa (as distinct from the 24-kDa) IGFBP-4 moiety constitutes a relatively minor component. The steady-state levels of granulosa cell-derived IGFBP-4 transcripts display relatively limited regulation in response to treatment with either FSH or IGF-I.
鉴于胰岛素样生长因子结合蛋白4(IGFBP - 4)对卵巢生理具有潜在的重要性,且仅采用体内实验模式存在明显局限性,我们着手在体外环境中描绘颗粒细胞来源的IGFBP - 4的特征及激素调节情况。
从经己烯雌酚预处理的未成熟完整大鼠卵巢穿刺获取的颗粒细胞进行长达72小时的培养。从培养物中提取的胰岛素样生长因子结合蛋白4信使核糖核酸进行Northern印迹杂交。通过用仓鼠中国仓鼠卵巢B(CHOB)互补脱氧核糖核酸再次杂交确保数据标准化,并计算IGFBP - 4/CHOB比率。在用大鼠IGFBP - 4定向多克隆抗血清(α - B104)进行免疫沉淀前后,对条件培养基进行Western配体印迹分析。
免疫沉淀研究显示颗粒细胞来源的IGFBP - 4由一个主要的24 kDa成分以及一个相对较小的27 kDa部分组成。对于来自未成熟雌激素处理大鼠的未处理颗粒细胞培养物,与IGFBP - 4对应的转录本最初出现暂时下降,在6小时达到最低点(下降67%;P <.05),随后相对迅速恢复(24小时内)至与培养开始时(时间0)相当的水平。然而,在48小时(而非72小时)时间点观察到额外的(尽管在统计学上无显著意义)增加。用浓度递增的促卵泡激素(FSH)处理颗粒细胞导致IGFBP - 4转录本的稳态水平下降高达30%(P <.05)。用高剂量FSH(100 ng/mL)处理后,IGFBP - 4转录本出现适度的双相、时间依赖性反应,其特征为24小时和48小时增加(分别比未处理对照高51%[P <.05]和26%[P =.052])以及72小时下降(25%;P =.16)。从72小时起向培养基中同时添加C19芳香化酶底物雄烯二酮(10⁻⁷ mol/L)增强了FSH(100 ng/mL)的抑制作用,使IGFBP - 4转录本最大下降49%(P <.05)。用胰岛素样生长因子(IGF)-I处理对IGFBP - 4转录本的稳态水平产生有限抑制(高达26%)(P <.05)。
研究结果表明存在大小各异的IGFBP - 4种类,其中27 kDa(与24 kDa不同)的IGFBP - 4部分构成相对较小的成分。颗粒细胞来源的IGFBP - 4转录本的稳态水平在对FSH或IGF - I处理的反应中显示出相对有限的调节。
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