基于小鼠着床前胚胎第三次卵裂和压实次数的子宫内囊胚发育和着床潜力预测

Jihyun Kim, S. Kim, J. Jun
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引用次数: 13

摘要

着床前胚胎发育过程中的细胞质分裂和细胞分裂是一个精心安排的时空程序。胚胎着床前的卵裂、压实和囊胚形成对成功着床和妊娠至关重要。它们的改变与染色体失衡和发育能力丧失有关。在这项研究中,我们通过延时监测来评估卵裂和压实时间作为体外植入前和植入周发育以及子宫植入潜力的预测因子。收集小鼠2细胞胚胎,于交配后1.5天(dpc),单独培养至离体期(OG) (7.5 dpc)。发育阶段分为3细胞期、4细胞期、8细胞期、桑葚胚期、囊胚期和OG期。通过受体工作特性曲线分析确定囊胚发育成功的截止时间。当2- 4细胞阶段的第三次裂解时间为9 h, 2-细胞阶段的压实时间为40 h时,囊胚和OG的发育率分别显著提高(P < 0.0001)。胚胎按上述截止时间分组,于分娩后3.5天移植至对侧子宫角。三裂胚早期(2-细胞到4细胞≤9 h)和压实胚早期(2-细胞到桑葚胚≤40 h)在5.5 dpc时的着床率显著高于延迟胚(P < 0.05)。因此,在人类体外受精-胚胎移植计划中,从2细胞阶段到4细胞阶段的第三次卵裂时间和从2细胞阶段到桑葚胚阶段的压实时间可能是预测发育潜力的有用形态动力学参数,包括成功着床和怀孕。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Prediction of blastocyst development and implantation potential in utero based on the third cleavage and compaction times in mouse pre-implantation embryos
Cytokinesis and cell division during pre-implantation embryonic development occur as an orchestrated spatiotemporal program. Cleavage, compaction, and blastulation in pre-implantation embryos are essential for successful implantation and pregnancy. Their alteration is associated with chromosomal imbalance and loss of developmental competence. In this study, we evaluated the time of cleavage and compaction as predictors for in vitro pre- and peri-implantation development and in utero implantation potential by time-lapse monitoring. Mouse 2-cell embryos were collected on 1.5 days post coitum (dpc) and were individually cultured to the outgrowth (OG) stage (7.5 dpc). Developmental stages were classified as 3-cell, 4-cell, 8-cell, morula, blastocyst, and OG. Cut-off times for successful blastocyst development were determined by receiver operating characteristic curve analysis. When cut-off times were set as 9 h for the third cleavage from the 2- to 4-cell stage, and 40 h for compaction from the 2-cell to morula stage, blastocyst and OG development rates, respectively, were significantly higher (P < 0.0001). Embryos were grouped according to the above cut-off time and transferred to the contralateral uterine horn on 3.5 dpc. Implantation rates in utero on 5.5 dpc were significantly higher in early third cleaved (≤ 9 h from 2- to 4-cell) and early compacted embryos (≤ 40 h from 2-cell to morula) than those in delayed embryos (P < 0.05). Therefore, the time of the third cleavage from 2- to the 4-cell stage and compaction from 2-cell to morula stage may be a useful morphokinetic parameter for predicting developmental potential, including successful implantation and pregnancy in human in vitro fertilization-embryo transfer programs.
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