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牛体外成熟/体外受精胚胎的核移植与电融合:培养基和电融合参数的影响

Nuclear transfer and electrofusion in bovine in vitro-matured/in vitro-fertilized embryos: effect of media and electrical fusion parameters.

作者信息

Van Stekelenburg-Hamers A E, Van Inzen W G, Van Achterberg T A, Kruip T A, de Laat S W, Weima S M

机构信息

Hubrecht Laboratory, Netherlands Institute for Developmental Biology, Utrecht.

出版信息

Mol Reprod Dev. 1993 Nov;36(3):307-12. doi: 10.1002/mrd.1080360304.

Abstract

In this study, micromanipulation and electrofusion conditions for the cloning of in vitro-produced bovine embryos (here after termed IVM/IVF embryos) derived from in vitro-matured (IVM) and in vitro-fertilized (IVF) oocytes were established. The effect of DC field strength on the fusion rate was tested in a model system using pronuclear stage embryos in which a cytoplasmic vesicle was removed and reinserted. Efficient fusion (80%) was obtained by applying a pulse of 1.75 kV/cm for 40 microseconds. In vitro development of manipulated pronuclear stage embryos was as efficient as that of unmanipulated control embryos. Different fusion media were compared in the cloning procedure, using IVM oocytes as recipients and blastomeres from day 6 IVM/IVF donor embryos. Zimmermann cell fusion medium reduced the lysis of nuclear transfer embryos compared to F300 (5% vs. 25%). The effects of drugs disrupting the microfilaments and microtubuli were determined. Neither the addition of cytochalasin B (CCB) for 1 hr in the postfusion medium nor incubation of donor blastomeres with nocodazole had a significant effect on the fusion or cleavage rate of the nuclear transfer embryos. Additional experiments demonstrated that there was no difference in developmental potential between nuclear transfer embryos allowed to develop in vitro or in vivo and that the embryos gave a 15% pregnancy rate in recipient cattle.

摘要

在本研究中,确立了用于克隆源自体外成熟(IVM)和体外受精(IVF)卵母细胞的体外生产牛胚胎(以下称为IVM/IVF胚胎)的显微操作和电融合条件。在一个模型系统中,使用去除并重新插入细胞质囊泡的原核期胚胎,测试了直流电场强度对融合率的影响。通过施加1.75 kV/cm的脉冲40微秒,获得了高效融合(80%)。经操作的原核期胚胎的体外发育与未操作的对照胚胎一样高效。在克隆过程中,以IVM卵母细胞为受体,以第6天的IVM/IVF供体胚胎的卵裂球为材料,比较了不同的融合培养基。与F300相比,齐默尔曼细胞融合培养基降低了核移植胚胎的裂解率(5%对25%)。测定了破坏微丝和微管的药物的作用。在融合后培养基中添加细胞松弛素B(CCB)1小时或用诺考达唑处理供体卵裂球,对核移植胚胎的融合率或裂解率均无显著影响。额外的实验表明,体外或体内发育的核移植胚胎的发育潜力没有差异,并且这些胚胎在受体母牛中的妊娠率为15%。

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