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Cloned calves derived from somatic cell nuclear transfer embryos cultured in chemically defined medium or modified synthetic oviduct fluid

机译:在化学成分确定的培养基或改良的合成输卵管液中培养的体细胞核移植胚胎的克隆小牛

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摘要

Somatic cell nuclear transfer (SCNT) is considered to be a critical tool for propagating valuable animals. To determine the productivity calves resulting from embryos derived with different culture media, enucleated oocytes matured in vitro were reconstructed with fetal fibroblasts, fused, and activated. The cloned embryos were cultured in modified synthetic oviduct fluid (mSOF) or a chemically defined medium (CDM) and developmental competence was monitored. After 7 days of culturing, the blastocysts were transferred into the uterine horn of estrus-synchronized recipients. SCNT embryos that were cultured in mSOF or CDM developed to the blastocysts stages at similar rates (26.6% vs. 22.5%, respectively). A total of 67 preimplantational stage embryos were transferred into 34 recipients and six cloned calves were born by caesarean section, or assisted or natural delivery. Survival of transferred blastocysts to live cloned calves in the mSOF and the CDM was 18.5% (to recipients), 9.6% (to blastocysts) and 42.9% (to recipients), 20.0% (to blastocysts), respectively. DNA analysis showed that all cloned calves were genetically identical to the donor cells. These results demonstrate that SCNT embryos cultured in CDM showed higher viability as judged by survival of the calves that came to term compared to blastocysts derived from mSOF cultures.
机译:体细胞核移植(SCNT)被认为是繁殖珍贵动物的关键工具。为了确定由不同培养基衍生的胚胎产生的小牛犊,用胎儿成纤维细胞重建,融合并激活了体外成熟的去核卵母细胞。在改良的合成输卵管液(mSOF)或化学成分确定的培养基(CDM)中培养克隆的胚胎,并监测其发育能力。培养7天后,将胚泡转移到发情同步受体的子宫角中。在mSOF或CDM中培养的SCNT胚胎以相似的速率发展到胚泡阶段(分别为26.6%和22.5%)。将总共​​67个植入前阶段的胚胎转移到34个接受者中,并通过剖腹产或辅助或自然分娩方式出生了6个克隆的小牛。在mSOF和CDM中,转移的胚泡存活的克隆小牛的存活率分别为18.5%(对受体),9.6%(对胚泡)和42.9%(对受体),20.0%(对胚泡)。 DNA分析表明,所有克隆的小牛在基因上都与供体细胞相同。这些结果表明,与来自mSOF培养物的胚泡相比,在CDM中培养的SCNT胚胎表现出更高的生存能力,这一点由即将出生的小牛的存活率来判断。

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