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The Effect of Estrogen Compounds on Human Embryoid Bodies

机译:雌激素化合物对人胚状体的影响

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摘要

Human embryonic stem cells are derived from the inner cell mass of preimplantation embryo at the blastocyst stage and their differentiation occurs through an intermediate step involving the formation of embryoid bodies (EBs), which are aggregates of embryonic stem cells. The EBs seem to be a powerful tool for investigating the development of embryos, as they can mimic the initial stages of embryonic development. In this study, we aimed to investigate the effect of estrogen compounds on the proliferation and differentiation of short-term and long-term cultured EBs in vitro. For this study, 10-day-old (short-term cultured) and 30-day-old (long-term cultured) EBs were subjected to estradiol (E2), estriol (E3), selective estrogen receptor modulator (raloxifene [RLX]), bisphenol A, and 1,3,5-tris(4-hydroxyphenyl)-4-propyl-1H-pyrazole for 7 days. To confirm the effects of estrogen treatment, ICI-182780 was added to the respective EBs for additional 7 days following estrogen treatment. Quantitative reverse transcription–polymerase chain reaction was performed to analyze the relative expression of differentiation marker genes representing the 3 germ layers. The expression of 7 marker genes, which included α-fetoprotein, hepatocyte nuclear factor (HNF)-3β, HNF-4α (endoderm), brachyury, cardiac actin ([cACT]; mesoderm), nestin (ectoderm), and Oct-4 (undifferentiated), was measured. Significantly, lower expression of HNF-4α in both short-term and long-term cultured EBs was observed after treatment of estrogen compounds compared to control. The expression of HNF-3β in short-term cultured EBs has been positively affected by E2, E3, and RLX. Regarding cACT, higher expression was observed after treatment of E2 (10−7 mol/L) and E3 (10−9 mol/L) in short-term cultured EBs, but opposite effects were demonstrated in long-term cultured EBs. The lower expressions of HNF-4α by E2 and RLX were negated by ICI-182780 treatment, although these findings were not statistically significant in E3-treated group. These findings suggest that estrogen compounds have effects on endodermal and mesodermal differentiation of human EBs.
机译:人胚胎干细胞来源于胚泡期的植入前胚胎的内部细胞团,它们的分化通过一个涉及胚状体(EBs)形成的中间步骤发生,该胚状体是胚胎干细胞的聚集体。 EBs可能是研究胚胎发育的强大工具,因为它们可以模仿胚胎发育的初始阶段。在这项研究中,我们旨在调查雌激素化合物对体外培养的短期和长期EB的增殖和分化的影响。在本研究中,对10天龄(短期培养)和30天龄(长期培养)的EB进行了雌二醇(E2),雌三醇(E3),选择性雌激素受体调节剂(雷洛昔芬[RLX] ),双酚A和1,3,5-三(4-羟苯基)-4-丙基-1H-吡唑共7天。为了确认雌激素治疗的效果,在雌激素治疗后将ICI-182780添加到各自的EB中另外7天。进行了定量逆转录-聚合酶链反应以分析代表3个胚层的分化标记基因的相对表达。 7种标志物基因的表达,包括α-甲胎蛋白,肝细胞核因子(HNF)-3β,HNF-4α(内胚层),短毛尿,心脏肌动蛋白([cACT];中胚层),巢蛋白(外胚层)和Oct-4 (未区分),进行了测量。显着地,与对照相比,在处理雌激素化合物后,在短期和长期培养的EB中均观察到HNF-4α的较低表达。 H2-3在短期培养的EB中的表达已受到E2,E3和RLX的积极影响。关于cACT,在短期培养的EB中,E2(10 -7 mol / L)和E3(10 −9 mol / L)处理后观察到更高的表达,但是在长期培养的EB中显示出相反的效果。通过ICI-182780治疗,E2和RLX可降低HNF-4α的表达,尽管这些发现在E3治疗组中无统计学意义。这些发现表明,雌激素化合物对人EB的内胚层和中胚层分化有影响。

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