Moreno-Ortiz Harold, Esteban-Perez Clara, Badran Wael, Kent-First Marijo
Reproductive Genetics and Stem Cell Laboratory, Department of Biological Sciences, Mississippi State University, Mississippi, USA.
J Vis Exp. 2009 Oct 22(32):1635. doi: 10.3791/1635.
The ability of embryonic germinal cells (EG) to differentiate into primordial germinal cells (PGCs) and later into gametes during early developmental stages is a perfect model to address our hypothesis about cancer and infertility. This protocol shows how to isolate primordial germinal cells from developing gonads in 10.5-11.5 days post coitum (dpc) mouse embryos. Developing gonadal ridges from mouse embryos (C57BL6J) were dissociated by mechanical disruption with collagenase, then plated in a mouse embryo fibroblast feeder layer (MEF-CF1) that was previously mitotically inactivated with mitomycin C in the presence of knockout media and supplemented with Leukemia Inhibitor Factor (LIF), basic Fibroblast Growth Factor (bFGF), and Stem Cell Factor (SCF). Using these optimized methods for PCG identification, isolation, and establishment of culture conditions permits long term cultures of EG cells for more than 40 days. The embryonic germinal cell lines showed embryonic phenotype and expression of common used markers of the pluripotent state. Isolation and derivation of germinal cells in culture provide a tool to understand their development in vitro and offer the opportunity to monitor cumulative damage at genetic and epigenetic levels after exposure to oxidative stress.
胚胎生殖细胞(EG)在早期发育阶段分化为原始生殖细胞(PGC)并随后分化为配子的能力,是验证我们关于癌症与不育症假说的理想模型。本实验方案展示了如何从交配后10.5 - 11.5天(dpc)的小鼠胚胎发育中的性腺中分离原始生殖细胞。将来自小鼠胚胎(C57BL6J)的发育中的性腺嵴用胶原酶进行机械破碎解离,然后接种到先前用丝裂霉素C进行有丝分裂灭活的小鼠胚胎成纤维细胞饲养层(MEF - CF1)上,该饲养层处于敲除培养基中,并补充白血病抑制因子(LIF)、碱性成纤维细胞生长因子(bFGF)和干细胞因子(SCF)。使用这些优化的原始生殖细胞鉴定、分离及培养条件建立方法,可使EG细胞长期培养超过40天。胚胎生殖细胞系表现出胚胎表型以及多能状态常用标志物的表达。培养中生殖细胞的分离和衍生为了解其体外发育提供了一种工具,并有机会监测暴露于氧化应激后在遗传和表观遗传水平上的累积损伤。
