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Egg cylinder development during in vitro extended embryo culture predicts the post transfer developmental potential of mouse blastocysts

机译:在体外扩展胚胎培养过程中的蛋缸发育预测小鼠胚泡后转移后的转移发育潜力

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Purpose To establish parameters during mouse extended embryo culture that accurately predict fetal developmental potential of a blastocyst without performing embryo transfer. Methods Embryos of three varying qualities were produced: poor quality embryos produced from in vitro matured oocytes (IVM), intermediate quality embryos produced from in vivo matured oocytes followed by in vitro fertilization and embryo culture (IVF); high quality embryos developed in vivo (VIVO). Embryonic day (E) 3.5 embryos from each group with similar morphologies were used for surgical embryo transfer to assess implantation and fetal developmental potential, in addition to placing these embryos into extended culture until E 8.5 to examine outgrowth area, egg cylinder volume, epiblast cell number, and outgrowth morphologies by immunofluorescence and 3D confocal microscopy. Results The proportional differences in epiblast cell number are strikingly similar to fetal development following embryo transfer, suggesting that this parameter may be indicative of the potential of an embryo to successfully develop into a fetus. Conclusion Extended embryo culture provides more accurate information regarding developmental potential than blastocyst morphological assessment. Specifically, epiblast cell number is an accurate and valuable predictor of fetal developmental potential. This work sets the stage for routine evaluation of embryo quality past the time embryos would normally be transferred. The ability to determine post implantation potential without embryo transfer may greatly improve efforts to culture higher quality embryos in vitro for human IVF, as well as reducing animal use and eliminating confounding maternal factors associated with embryo transfer experiments in research.
机译:目的在小鼠扩展胚胎培养过程中建立参数,以准确地预测胚泡的胎儿发育潜力而不进行胚胎转移。方法制备三种不同品质的胚胎:由体外成熟的卵母细胞(IVM)产生的质量差,中间质量胚胎,从体内成熟的卵母细胞中产生,然后体外施肥和胚胎培养物(IVF);体内(体内)开发的高品质胚胎。来自每组的胚胎天(e)3.5胚胎具有相似的形态学用于手术胚胎转移,以评估植入和胎儿发育潜力,除了将这些胚胎放入延长的培养物之前,直到E 8.5检查产卵区域,蛋缸体积,外壳容量免疫荧光和3D共聚焦显微镜的数量和外泌盐形态。结果胚胎转移后胎儿细胞数的比例差异与胎儿发育相似,表明该参数可以指示胚胎成功发展成胎儿的潜力。结论扩展胚胎培养提供了比胚泡形态评估的发育潜力更准确的信息。具体地,胎儿细胞数是胎儿发育潜力的准确性和有价值的预测因子。这项工作设定了常规评估胚胎质量的阶段,过去通常会转移时间胚胎。确定没有胚胎转移的植入后电位的能力可能大大提高培养人IVF体外更高质量的胚胎的努力,以及减少动物使用,消除与研究中胚胎转移实验相关的混淆母体因素。

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