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采用简化的去卵丘和核移植方法产生的玻璃化克隆囊胚所出生的仔猪。

Piglets born from vitrified cloned blastocysts produced with a simplified method of delipation and nuclear transfer.

作者信息

Du Yutao, Li Juan, Kragh Peter M, Zhang Yunhai, Schmidt Mette, Bøgh Ingrid B, Zhang Xiuqing, Purup Stig, Kuwayama M, Jørgensen Arne L, Pedersen Anette M, Villemoes Klaus, Yang Huanming, Bolund Lars, Vajta Gábor

机构信息

Population Genetics and Embryology, Institute of Genetics and Biotechnology, University of Aarhus, Tjele, Denmark.

出版信息

Cloning Stem Cells. 2007 Winter;9(4):469-76. doi: 10.1089/clo.2007.0037.

Abstract

Successful cryopreservation of porcine embryos offers a promising perspective in the fields of agriculture, animal science, and human medical research. The objective of the present work was to establish a system facilitating the cryopreservation of porcine embryos produced by somatic cell nuclear transfer (SCNT). Several key techniques including micromanipulator-based enucleation, noninvasive delipation, zona-free fusion, and activation were combined with high efficiency. After a partial zona digestion and high-speed centrifugation, 89.8+/-2.1% (mean+/-SEM) of enucleated oocytes were successfully delipated. Delipated cytoplasts were incubated for an additional 0.5 or 2 h before fusion with somatic cells. After activation and 6 days of in vitro culture, no significant difference in the rate of blastocysts per reconstructed embryo was observed between the two groups (33.1+/-1.8% and 26.0+/-4.3% for 0.5 and 2 h recovery time, respectively). Cryopreservation of the blastocysts was performed with a Cryotop device and factory-prepared vitrification and warming solutions. One hundred fifty-five vitrified SCNT embryos were transferred surgically into two recipient sows to test their developmental capacity in vivo. One recipient became pregnant and delivered six piglets. In conclusion, our simplified delipation and SCNT procedure resulted in viable piglets after vitrification and embryo transfer at the blastocyst stage.

摘要

猪胚胎的成功冷冻保存为农业、动物科学和人类医学研究领域提供了一个有前景的方向。本研究的目的是建立一个有助于冷冻保存通过体细胞核移植(SCNT)产生的猪胚胎的系统。包括基于显微操作去核、无创去卵丘、无透明带融合和激活在内的几种关键技术高效结合。经过部分透明带消化和高速离心后,89.8±2.1%(平均值±标准误)的去核卵母细胞成功去卵丘。去卵丘的细胞质体在与体细胞融合前再孵育0.5或2小时。激活并体外培养6天后,两组之间每个重构胚胎的囊胚率无显著差异(恢复时间为0.5小时和2小时时分别为33.1±1.8%和26.0±4.3%)。使用Cryotop装置以及工厂制备的玻璃化和复温溶液对囊胚进行冷冻保存。将155个玻璃化的SCNT胚胎通过手术移植到两头受体母猪体内,以测试它们在体内的发育能力。一头受体母猪怀孕并产下6头仔猪。总之,我们简化的去卵丘和SCNT程序在囊胚期玻璃化和胚胎移植后产生了存活的仔猪。

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