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增加细胞接种密度模拟了培养牛颗粒细胞的黄体生成素后期早期阶段。

Increasing cell plating density mimics an early post-LH stage in cultured bovine granulosa cells.

机构信息

Reproductive Biology, Leibniz Institute for Farm Animal Biology (FBN), Wilhelm-Stahl-Allee 2, 18196, Dummerstorf, Germany.

出版信息

Cell Tissue Res. 2013 Dec;354(3):869-80. doi: 10.1007/s00441-013-1712-9. Epub 2013 Sep 13.

DOI:10.1007/s00441-013-1712-9
PMID:24026437
Abstract

Cultured ovarian granulosa cells are essential models to study molecular mechanisms of gene regulation during folliculogenesis. Here, we characterize primary tissue culture models for bovine granulosa cells by morphological and physiological parameters and by novel molecular luteinization markers, as transcript abundance and DNA methylation levels. The data show that: (1) collagen substrate increased the number of attached, viable cells; (2) the expression of the key transcripts of estrogen synthesis, CYP19A1, could be induced and maintained in granulosa cells from small to medium but not from large follicles, whereas (3) only granulosa cells from large but not from smaller follicles were responsive to LH; (4) serum supplementation unfavorably transformed the cellular phenotype, induced proliferation and PCNA expression, reduced or abolished the transcript abundance of steroidogenic key genes and of gonadotropin receptor genes, CYP11A1, CYP19A1, FSHR and LHCGR but, however, did not increase the abundance of the luteinization-specific marker transcripts PTGS2, PTX3, RGS2 and VNN2; but (5) by increasing the plating density, estradiol production and the abundance of CYP19A1 transcripts, in particular those derived from the main ovarian promoter P2, were decreased concurrently leaving P2-specific DNA methylation levels unchanged, whereas progesterone secretion was stimulated and the expression of both luteinization-specific marker transcripts, RGS2 and VNN2, was significantly induced. From these data, we conclude that increasing the plating density induces a different, partly complementary, physiological and gene expression profile in cultured bovine granulosa cells and drives the cells towards an early post-LH stage of luteinization, even in the absence of luteinizing agents.

摘要

培养的卵巢颗粒细胞是研究卵泡发生过程中基因调控分子机制的重要模型。在这里,我们通过形态和生理参数以及新的分子黄体化标记物(如转录物丰度和 DNA 甲基化水平)来描述牛颗粒细胞的原代组织培养模型。数据表明:(1)胶原基质增加了附着的、存活的细胞数量;(2)从小到中等大小的卵泡中,雌激素合成的关键转录物 CYP19A1 的表达可以被诱导并维持,但(3)只有大卵泡而不是小卵泡的颗粒细胞对 LH 有反应;(4)血清补充不利于细胞表型转化,诱导增殖和 PCNA 表达,减少或消除类固醇生成关键基因和促性腺激素受体基因(CYP11A1、CYP19A1、FSHR 和 LHCGR)的转录物丰度,但(5)通过增加接种密度,雌二醇的产生和 CYP19A1 转录物的丰度,特别是来自主要卵巢启动子 P2 的转录物,同时减少了 P2 特异性 DNA 甲基化水平不变,而孕激素的分泌受到刺激,黄体化特异性标记物转录物 RGS2 和 VNN2 的表达显著诱导。从这些数据中,我们得出结论,增加接种密度会导致培养的牛颗粒细胞中出现不同的、部分互补的生理和基因表达谱,并促使细胞向黄体化的早期 LH 后阶段发展,即使在没有黄体生成素的情况下也是如此。

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