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延迟囊胚形成或延长一天培养会增加猪囊胚中的细胞凋亡。

Delayed blastocyst formation or an extra day culture increases apoptosis in pig blastocysts.

作者信息

Lin Tao, Lee Jae Eun, Oqani Reza K, Kim So Yeon, Cho Eun Seok, Jeong Yong Dae, Baek Jun Jong, Jin Dong Il

机构信息

Department of Animal Science & Biotechnology, Research Center for Transgenic Cloned Pigs, Chungnam National University, Daejeon 34134, Republic of Korea.

Department of Animal Resource Development, National Institute of Animal Science, Cheonan, 31001, Republic of Korea.

出版信息

Anim Reprod Sci. 2017 Oct;185:128-139. doi: 10.1016/j.anireprosci.2017.08.012. Epub 2017 Aug 18.

Abstract

In the present study, the timing was examined of blastocyst collection/formation or of how the duration of post-blastulation culture affected the quality and developmental competence of in vitro-produced pig parthenogenetic embryos. The earliest apoptotic signals were observed at the morula stage while the earliest cytoplasmic fragmentation was observed before the 4- to 8-cell stage of embryo development. Nuclear condensation was detected in morulae and blastocysts, but not all condensed nuclei were positive for the apoptotic signal (TUNEL staining). The mean blastocyst diameter increased with delayed blastocyst collection or extended post-blastulation culture, but decreased with delayed blastocyst formation. Delayed blastocyst collection/formation or an additional day of post-blastulation culture increased the frequencies of apoptosis, condensed nuclei, and low quality blastocysts (those showing a nuclear destruction that negated counting of the nuclei); increased the expression of the pro-apoptotic BAX gene; and reduced the ratio of ICM (inner cell mass) cells to TE (trophectoderm) cells. In addition, delayed blastocyst formation decreased POU5F1 gene expression. These results suggest that a delay in blastocyst collection/formation or an additional day of culture could increase the incidence of apoptosis, decrease the ICM:TE cell ratio, and influence the gene expression and diameter of blastocysts derived from in vitro-produced pig embryos. These findings provide a useful reference for improving the quality of in vitro-produced embryos.

摘要

在本研究中,对囊胚采集/形成的时间,或囊胚形成后培养时间对体外生产的猪孤雌生殖胚胎的质量和发育能力的影响进行了研究。最早的凋亡信号在桑葚胚阶段被观察到,而最早的细胞质碎片化在胚胎发育的4至8细胞阶段之前被观察到。在桑葚胚和囊胚中检测到核浓缩,但并非所有浓缩核的凋亡信号(TUNEL染色)均为阳性。囊胚的平均直径随着囊胚采集延迟或囊胚形成后培养时间延长而增加,但随着囊胚形成延迟而减小。囊胚采集/形成延迟或囊胚形成后再培养一天会增加凋亡、核浓缩和低质量囊胚(那些显示核破坏以至于无法计数核的囊胚)的频率;增加促凋亡BAX基因的表达;并降低内细胞团(ICM)细胞与滋养外胚层(TE)细胞的比例。此外,囊胚形成延迟会降低POU5F1基因的表达。这些结果表明,囊胚采集/形成延迟或额外培养一天会增加凋亡发生率,降低ICM:TE细胞比例,并影响体外生产的猪胚胎来源囊胚的基因表达和直径。这些发现为提高体外生产胚胎的质量提供了有用的参考。

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