Nucleus reprogramming/remodeling through selective enucleation (SE) of immature oocytes and zygotes: a nucleolus point of view

H. Fulka, P. Loi, L. Palazzese, Michal Benc, J. Fulka
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Abstract

It is now approximately 25 years since the sheep Dolly, the first cloned mammal where the somatic cell nucleus from an adult donor was used for transfer, was born. So far, somatic cell nucleus transfer, where G1-phase nuclei are transferred into cytoplasts obtained by enucleation of mature metaphase II (MII) oocytes followed by the activation of the reconstructed cells, is the most efficient approach to reprogram/remodel the differentiated nucleus. In general, in an enucleated oocyte (cytoplast), the nuclear envelope (NE, membrane) of an injected somatic cell nucleus breaks down and chromosomes condense. This condensation phase is followed, after subsequent activation, by chromatin decondensation and formation of a pseudo-pronucleus (i) whose morphology should resemble the natural postfertilization pronuclei (PNs). Thus, the volume of the transferred nuclei increases considerably by incorporating the content released from the germinal vesicles (GVs). In parallel, the transferred nucleus genes must be reset and function similarly as the relevant genes in normal embryo reprogramming. This, among others, covers the relevant epigenetic modifications and the appropriate organization of chromatin in pseudo-pronuclei. While reprogramming in SCNT is often discussed, the remodeling of transferred nuclei is much less studied, particularly in the context of the developmental potential of SCNT embryos. It is now evident that correct reprogramming mirrors appropriate remodeling. At the same time, it is widely accepted that the process of rebuilding the nucleus following SCNT is instrumental to the overall success of this procedure. Thus, in our contribution, we will mostly focus on the remodeling of transferred nuclei. In particular, we discuss the oocyte organelles that are essential for the development of SCNT embryos.
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通过未成熟卵母细胞和受精卵的选择性去核(SE)进行细胞核重编程/重塑:核仁的观点
绵羊多利诞生至今已近25年。多利是世界上第一只克隆哺乳动物,利用成年捐赠者的体细胞细胞核进行移植。到目前为止,将g1期细胞核转移到成熟中期II (MII)卵母细胞去核获得的细胞质中,然后激活重建的细胞,是对分化细胞核进行重编程/重塑的最有效方法。一般来说,在去核卵母细胞(细胞质)中,注射的体细胞细胞核的核膜(NE,膜)破裂,染色体浓缩。在随后的激活后,染色质去浓缩并形成假原核(i),其形态应类似于自然受精后原核(PNs)。因此,通过纳入生发囊泡(GVs)释放的内容物,转移核的体积大大增加。同时,转移的细胞核基因必须被重置,其功能与正常胚胎重编程中的相关基因相似。这,除其他外,涵盖了相关的表观遗传修饰和伪原核中染色质的适当组织。虽然SCNT中的重编程经常被讨论,但对转移核的重塑的研究却少得多,特别是在SCNT胚胎发育潜力的背景下。现在很明显,正确的重编程反映了适当的重塑。与此同时,人们普遍认为SCNT后重建细胞核的过程对该手术的整体成功至关重要。因此,在我们的贡献中,我们将主要关注转移核的重塑。我们特别讨论了对SCNT胚胎发育至关重要的卵母细胞细胞器。
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