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大鼠卵巢中胰腺型磷脂酶A2的基因表达:对孕酮释放的刺激作用。

Gene expression of pancreatic-type phospholipase-A2 in rat ovaries: stimulatory action on progesterone release.

作者信息

Nomura K, Fujita H, Arita H

机构信息

Shionogi Research Laboratories, Shionogi Co., Osaka, Japan.

出版信息

Endocrinology. 1994 Aug;135(2):603-9. doi: 10.1210/endo.135.2.8033809.

Abstract

We reported previously that pancreatic-type group I phospholipase-A2 (PLA2-I) stimulates DNA synthesis or prostaglandin E2 production in various cell types via its specific receptors on the cell surface. In the present study we examined the effect of PLA2-I on corpus luteum, which possesses specific PLA2-I receptors, and demonstrated gene expression of PLA2-I in rat ovaries. PLA2-I stimulated progesterone release from incubated corpora lutea at concentrations above 10 nM in a dose-dependent manner. Northern blot analysis revealed the presence of PLA2-I messenger RNA (mRNA) in rat ovaries. The level of PLA2-I mRNA was elevated during diestrus to proestrus, and decreased to almost nothing on the day of estrus. To further evaluate the timing of PLA2-I expression, we analyzed RNAs extracted from small follicles, large preovulatory follicles, and corpora lutea obtained from various phases of hCG-treated immature rats. During follicular development, mRNA levels remained negligible. The level of PLA2-I mRNA began to rise after luteinization of follicles and increased during the maturation of the corpora lutea. Levels of PLA2-I mRNA in ovaries from day 5 and day 10 pregnant rats were 5- to 10-fold higher than those in diestrous rats, whereas on day 21, the mRNA level was decreased. Immunocytochemical studies were performed to clarify the synthesis and localization of PLA2-I in the ovary using polyclonal anti-PLA2-I antibodies. Intense immunoreactivity was detected only in luteal cells of newly formed corpora lutea. However, the number and intensity of immunoreactive cells decreased in old corpora lutea. No immunoreactivity was detected in follicular cells of small- or middle-sized follicles. These results demonstrate the correlation among PLA2-I gene expression, estrous cycle, and progesterone secretion in rat ovaries and suggest a new function of PLA2-I as an intragonadal regulatory factor for steroidogenesis.

摘要

我们之前报道过,胰腺型I组磷脂酶A2(PLA2-I)通过其在细胞表面的特异性受体刺激多种细胞类型中的DNA合成或前列腺素E2的产生。在本研究中,我们检测了PLA2-I对具有特异性PLA2-I受体的黄体的影响,并证实了PLA2-I在大鼠卵巢中的基因表达。PLA2-I以剂量依赖的方式刺激孵育的黄体释放孕酮,浓度高于10 nM。Northern印迹分析显示大鼠卵巢中存在PLA2-I信使核糖核酸(mRNA)。PLA2-I mRNA的水平在间情期到动情前期升高,在发情当天降至几乎检测不到。为了进一步评估PLA2-I表达的时间,我们分析了从经人绒毛膜促性腺激素(hCG)处理的未成熟大鼠不同阶段获得的小卵泡、大排卵前卵泡和黄体中提取的RNA。在卵泡发育过程中,mRNA水平仍然可以忽略不计。PLA2-I mRNA的水平在卵泡黄体化后开始升高,并在黄体成熟过程中增加。妊娠第5天和第10天大鼠卵巢中PLA2-I mRNA的水平比间情期大鼠高5至10倍,而在第21天,mRNA水平下降。使用多克隆抗PLA2-I抗体进行免疫细胞化学研究,以阐明PLA2-I在卵巢中的合成和定位。仅在新形成的黄体的黄体细胞中检测到强烈的免疫反应性。然而,在老化的黄体中,免疫反应性细胞的数量和强度下降。在中小卵泡的卵泡细胞中未检测到免疫反应性。这些结果证明了大鼠卵巢中PLA2-I基因表达、发情周期和孕酮分泌之间的相关性,并提示PLA2-I作为类固醇生成的性腺内调节因子具有新功能。

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