细胞微环境决定原代培养的小鼠胎儿睾丸间质细胞的雄激素生成。
Cellular microenvironment dictates androgen production by murine fetal Leydig cells in primary culture.
作者信息
Carney Colleen M, Muszynski Jessica L, Strotman Lindsay N, Lewis Samantha R, O'Connell Rachel L, Beebe David J, Theberge Ashleigh B, Jorgensen Joan S
机构信息
Department of Comparative Bioscience, School of Veterinary Medicine, University of Wisconsin-Madison, Madison, Wisconsin.
Department of Biomedical Engineering, University of Wisconsin-Madison, Madison, Wisconsin Carbone Cancer Center, University of Wisconsin-Madison, Madison, Wisconsin.
出版信息
Biol Reprod. 2014 Oct;91(4):85. doi: 10.1095/biolreprod.114.118570. Epub 2014 Aug 20.
Despite the fact that fetal Leydig cells are recognized as the primary source of androgens in male embryos, the mechanisms by which steroidogenesis occurs within the developing testis remain unclear. A genetic approach was used to visualize and isolate fetal Leydig cells from remaining cells within developing mouse testes. Cyp11a1-Cre mice were bred to mT/mG dual reporter mice to target membrane-tagged enhanced green fluorescent protein (GFP) within steroidogenic cells, whereas other cells expressed membrane-tagged tandem-dimer tomato red. Fetal Leydig cell identity was validated using double-labeled immunohistochemistry against GFP and the steroidogenic enzyme 3beta-HSD, and cells were successfully isolated as indicated by qPCR results from sorted cell populations. Because fetal Leydig cells must collaborate with neighboring cells to synthesize testosterone, we hypothesized that the fetal Leydig cell microenvironment defined their capacity for androgen production. Microfluidic culture devices were used to measure androstenedione and testosterone production of fetal Leydig cells that were cultured in cell-cell contact within a mixed population, were isolated but remained in medium contact via compartmentalized co-culture with other testicular cells, or were isolated and cultured alone. Results showed that fetal Leydig cells maintained their identity and steroidogenic activity for 3-5 days in primary culture. Microenvironment dictated proficiency of testosterone production. As expected, fetal Leydig cells produced androstenedione but not testosterone when cultured in isolation. More testosterone accumulated in medium from mixed cultures than from compartmentalized co-cultures initially; however, co-cultures maintained testosterone synthesis for a longer time. These data suggest that a combination of cell-cell contact and soluble factors constitute the ideal microenvironment for fetal Leydig cell activity in primary culture.
尽管胎儿睾丸间质细胞被认为是雄性胚胎中雄激素的主要来源,但在发育中的睾丸内发生类固醇生成的机制仍不清楚。采用遗传学方法从发育中的小鼠睾丸内的其余细胞中可视化并分离胎儿睾丸间质细胞。将Cyp11a1-Cre小鼠与mT/mG双报告基因小鼠杂交,以靶向类固醇生成细胞内的膜标记增强型绿色荧光蛋白(GFP),而其他细胞则表达膜标记串联二聚体番茄红色荧光蛋白。使用针对GFP和类固醇生成酶3β-HSD的双标记免疫组织化学验证胎儿睾丸间质细胞的身份,并且如分选细胞群体的qPCR结果所示,细胞被成功分离。由于胎儿睾丸间质细胞必须与相邻细胞协作以合成睾酮,我们推测胎儿睾丸间质细胞微环境决定了它们产生雄激素的能力。使用微流控培养装置来测量在混合群体中进行细胞间接触培养、分离但通过与其他睾丸细胞进行分隔共培养仍保持与培养基接触或分离并单独培养的胎儿睾丸间质细胞的雄烯二酮和睾酮产量。结果表明,胎儿睾丸间质细胞在原代培养中维持其身份和类固醇生成活性3至5天。微环境决定了睾酮产生的效率。正如预期的那样,胎儿睾丸间质细胞在单独培养时产生雄烯二酮但不产生睾酮。最初,混合培养的培养基中积累的睾酮比分隔共培养的更多;然而,共培养维持睾酮合成的时间更长。这些数据表明,细胞间接触和可溶性因子的组合构成了原代培养中胎儿睾丸间质细胞活动的理想微环境。
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