成年猕猴睾丸培养物中生殖细胞的特征和群体动力学。
Characterization and population dynamics of germ cells in adult macaque testicular cultures.
机构信息
Center of Reproductive Medicine and Andrology, Institute of Reproductive and Regenerative Biology, Münster, North Rhine-Westphalia, Germany.
Center for Reproductive Medicine, Amsterdam UMC Location AMC, University of Amsterdam, Amsterdam, the Netherlands.
出版信息
PLoS One. 2019 Jun 21;14(6):e0218194. doi: 10.1371/journal.pone.0218194. eCollection 2019.
BACKGROUND
From a biological and clinical perspective, it is imperative to establish primate spermatogonial cultures. Due to limited availability of human testicular tissues, the macaque (Macaca fascicularis) was employed as non-human primate model. The aim of this study was to characterize the expression of somatic as well as germ cell markers in testicular tissues and to establish macaque testicular primary cell cultures.
MATERIALS AND METHODS
Characterization of macaque testicular cell population was performed by immunohistochemical analyses for somatic cell markers (SOX9, VIM, SMA) as well as for germ cell markers (UTF1, MAGEA4, VASA). Testicular cells from adult macaque testes (n = 4) were isolated and cultured for 21 days using three stem cell culture media (SSC, PS and SM). An extended marker gene panel (SOX9, VIM, ACTA2; UTF1, FGFR3, MAGEA4, BOLL, DDX4) was then employed to assess the changes in gene expression levels and throughout the in vitro culture period. Dynamics of the spermatogonial population was further investigated by quantitative analysis of immunofluorescence-labeled MAGEA4-positive cells (n = 3).
RESULTS
RNA expression analyses of cell cultures revealed that parallel to decreasing SOX9-expressing Sertoli cells, maintenance of VIM and ACTA2-expressing somatic cells was observed. Expression levels of germ cell marker genes UTF1, FGFR3 and MAGEA4 were maintained until day 14 in SSC and SM media. Findings from MAGEA4 immunofluorescence staining corroborate mRNA expression profiling and substantiate the overall maintenance of MAGEA4-positive pre- and early meiotic germ cells until day 14.
CONCLUSIONS
Our findings demonstrate maintenance of macaque germ cell subpopulations in vitro. This study provides novel perspective and proof that macaques could be used as a research model for establishing in vitro germ cell-somatic cell cultures, to identify ideal culture conditions for long-term maintenance of primate germ cell subpopulation in vitro.
背景
从生物学和临床角度来看,建立灵长类精原细胞培养是当务之急。由于人类睾丸组织的供应有限,猕猴(Macaca fascicularis)被用作非人类灵长类动物模型。本研究的目的是描述睾丸组织中体细胞和生殖细胞标志物的表达,并建立猕猴睾丸原代细胞培养。
材料和方法
通过免疫组织化学分析,对体细胞标志物(SOX9、VIM、SMA)和生殖细胞标志物(UTF1、MAGEA4、VASA)对猕猴睾丸细胞群体进行了特征描述。从成年猕猴睾丸(n=4)中分离出睾丸细胞,并使用三种干细胞培养基(SSC、PS 和 SM)培养 21 天。然后,使用扩展的标记基因谱(SOX9、VIM、ACTA2;UTF1、FGFR3、MAGEA4、BOLL、DDX4)评估体外培养期间基因表达水平的变化。通过对免疫荧光标记的 MAGEA4 阳性细胞(n=3)进行定量分析,进一步研究精原细胞群体的动态变化。
结果
细胞培养的 RNA 表达分析显示,与 SOX9 表达的支持细胞减少平行,维持了 VIM 和 ACTA2 表达的体细胞。在 SSC 和 SM 培养基中,UTF1、FGFR3 和 MAGEA4 的生殖细胞标记基因表达水平在第 14 天之前保持不变。MAGEA4 免疫荧光染色的结果与 mRNA 表达谱分析相符,并证实了 MAGEA4 阳性的减数分裂前和早期生殖细胞在第 14 天之前总体上得到维持。
结论
我们的研究结果表明,灵长类生殖细胞亚群在体外得到维持。本研究提供了新的视角和证据,证明猕猴可作为建立体外生殖细胞-体细胞培养的研究模型,以确定体外长期维持灵长类生殖细胞亚群的理想培养条件。
Zotero 插件