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改良的手工克隆骆驼方法的发展。

Development of a modified method of handmade cloning in dromedary camel.

机构信息

Department of Embryology, Camel Advanced Reproductive Technologies Centre, Government of Dubai, Dubai, United Arab Emirates.

出版信息

PLoS One. 2019 Apr 17;14(4):e0213737. doi: 10.1371/journal.pone.0213737. eCollection 2019.

Abstract

In this study, a modified method of handmade cloning (m-HMC), which had been originally developed in sheep, was used for somatic cell nuclear transfer (SCNT) in the dromedary camel. The unique feature of m-HMC over current SCNT methods lies in the use of a simple device (a finely drawn micropipette made of Pasteur pipette) for chemically-assisted enucleation of oocytes under a stereomicroscope with improved efficiency and ease of operation. Using this system, the throughput of cloned embryo reconstitution was increased over 2-fold compared to the control SCNT method (c-NT). Stepwise measurement of reactive oxygen species (ROS) revealed that method, steps, and duration of SCNT all influenced oxidative activity of oocytes, but their impact were not similar. Specifically, UV-assisted oocyte enucleation was identified as the major source of ROS production, which explained significantly higher total ROS of reconstituted embryos in c-NT compared to m-HMC. Fusion efficiency (95.3±3.3 vs. 75.4±7.6%) and total efficiency of blastocyst development (22.5±3.0 vs. 14.1±4.3%) were significantly higher in m-HMC compared to c-NT, respectively, and blastocysts of transferable quality were obtained in similar rates (41.9±8.2 vs. 48.0±15.2%, respectively). Significance differences were observed in total cell number (155.3±13.6 vs. 123.6±19.5) and trophectoderm (145±9.5 vs. 114.3±15.2), but not inner cell mass (10.3±4.1 vs. 9.3±5.3) counts between blastocysts developed in c-NT compared to m-HMC, respectively. However, expression of key developmental genes (POU5F1, KLF4, SOX2, MYC, and CDX2) was comparable between blastocysts of both groups. The introduced m-HMC method might be a viable approach for efficient production of dromedary camel clones for research and commercial utilization.

摘要

在这项研究中,我们使用了一种改良的手工克隆方法(m-HMC),该方法最初是在绵羊中开发的,用于骆驼的体细胞核移植(SCNT)。m-HMC 与当前的 SCNT 方法的独特之处在于,它使用了一种简单的设备(由巴氏吸管制成的精细拉制的微吸管),在体视显微镜下进行化学辅助的卵母细胞去核,从而提高了效率和操作简便性。使用该系统,与对照 SCNT 方法(c-NT)相比,克隆胚胎重构的通量增加了两倍以上。逐步测量活性氧(ROS)表明,方法、步骤和 SCNT 的持续时间都影响卵母细胞的氧化活性,但它们的影响并不相似。具体而言,紫外线辅助的卵母细胞去核被确定为 ROS 产生的主要来源,这解释了 c-NT 中重构胚胎的总 ROS 明显高于 m-HMC。m-HMC 的融合效率(95.3±3.3%比 75.4±7.6%)和囊胚发育的总效率(22.5±3.0%比 14.1±4.3%)均显著高于 c-NT,并且获得了具有可转移质量的囊胚,其比例分别为 41.9±8.2%和 48.0±15.2%。在 c-NT 与 m-HMC 之间,总细胞数(155.3±13.6 比 123.6±19.5)和滋养层(145±9.5 比 114.3±15.2)均存在显著差异,但内细胞团(10.3±4.1 比 9.3±5.3)计数无差异。然而,两组囊胚中的关键发育基因(POU5F1、KLF4、SOX2、MYC 和 CDX2)的表达相当。引入的 m-HMC 方法可能是一种有效的方法,可用于高效生产用于研究和商业用途的骆驼克隆。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/db90/6469772/f5f492db4aa5/pone.0213737.g001.jpg

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