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首页> 外文期刊>The Journal of Reproduction and Development >Time-lapse monitoring reveals that vitrification increases the frequency of contraction during the pre-hatching stage in mouse embryos
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Time-lapse monitoring reveals that vitrification increases the frequency of contraction during the pre-hatching stage in mouse embryos

机译:延时监控显示,玻璃化增加了小鼠胚胎在孵化前阶段的收缩频率

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Contraction during the blastocyst stage is observed during embryonic development of various mammals, including humans, but the physiological role of this process is not well understood. Using time-lapse monitoring (TLM), we studied the influence of vitrification and contractions on embryonic development in mice. Mouse embryos were cultured at the 2-cell stage. At the 8-cell stage, embryos were randomly divided into a fresh group (FG) and vitrified group (VG) and observed for up to 144 h. Strong contractions (i.e., contractions causing a decrease in volume of more than 20% and expansion of the perivitelline space) occurred significantly more often in unhatched embryos than hatching embryos in both groups. Regarding hatching embryos, contractions in the pre-hatching stage were significantly more frequent in the VG than the FG. Furthermore, mRNA expression levels of genes related to contractions were determined at three time points, the 8-cell stage, early blastocyst stage, and 20 h after blastocoel formation, with quantitative reverse transcription-polymerase chain reaction. There was no significant difference in Hspa1a expression between the FG and VG, but Hspa1a overexpression was observed just after thawing and tended to decrease gradually thereafter in some blastocysts. Furthermore, in the VG, Atp1a1 tended to show higher expression in the strong contraction group than in the weak contraction group. Overall, vitrification is an excellent method for cryopreservation but could increase contractions in the pre-hatching stage and may increase energy demands of the embryo. Observation of contraction by TLM may improve the evaluation of embryo quality.
机译:在包括人类在内的各种哺乳动物的胚胎发育过程中都观察到了胚泡期的收缩,但是这一过程的生理学作用尚不十分清楚。使用延时监控(TLM),我们研究了玻璃化和收缩对小鼠胚胎发育的影响。在2-细胞阶段培养小鼠胚胎。在8细胞阶段,将胚胎随机分为新鲜组(FG)和玻璃化组(VG),并观察长达144小时。在两组中,未孵化的胚胎发生强收缩的现象(即收缩导致体积减少超过20%并增加周玻璃体空间的收缩)的发生率明显高于孵化的胚胎。关于孵化胚胎,在孵化前阶段,VG中的收缩频率明显高于FG。此外,通过定量逆转录-聚合酶链反应,在8个细胞阶段,胚泡早期和囊胚形成后20小时三个时间点测定与收缩相关的基因的mRNA表达水平。 FG和VG之间的Hspa1a表达没有显着差异,但是刚解冻后就观察到Hspa1a过表达,并且在某些胚泡中倾向于逐渐降低。此外,在VG中,强收缩组中的Atp1a1倾向于比弱收缩组中的表达更高。总体而言,玻璃化是冷冻保存的极好方法,但可能会在孵化前增加收缩,并可能增加胚胎的能量需求。通过TLM观察收缩可以改善对胚胎质量的评估。

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