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首页> 外文期刊>The Journal of Reproduction and Development >Contributions of UBE2C and UBE2S to meiotic progression of porcine oocytes
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Contributions of UBE2C and UBE2S to meiotic progression of porcine oocytes

机译:UBE2C和UBE2S对猪卵母细胞的减少进展的贡献

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Vertebrate oocytes arrested at the first meiotic prophase must proceed to the second meiotic metaphase (MII) before fertilization. This meiotic process requires the precise control of protein degradation. Part of the protein degradation in oocytes is controlled by members of the ubiquitin-conjugating enzyme family, UBE2C and UBE2S, which are known to participate in mono-ubiquitination and poly-ubiquitination, respectively. Although UBE2 enzymes have been well studied in mitosis, their contribution to mammalian oocyte meiosis is relatively unknown and has been studied only in mice. Here, we investigated the contribution of UBE2C and UBE2S to porcine oocyte maturation using an RNA injection method. Overexpression of UBE2S prevented MIT arrest of oocytes and led to the formation of a pronucleus (PN) at 48 h of culture. This effect was also observed for prolonged cultures of UBE2C-overexpressing oocytes, suggesting the effectiveness of poly-ubiquitination in the rapid escape from M-phase in porcine oocytes. Although the inhibition of either UBE2C or UBE2S by antisense RNA (asRNA) injection had no effect on oocyte maturation, asRNA-injected oocytes showed inhibited PN formation after parthenogenetic activation. These results indicated that ubiquitination of certain factors by UBE2S and UBE2C plays a role in the escape from MIT arrest in porcine oocytes. Further investigations to identify the factors and how mono- and/or poly-ubiquitination contributes to protein degradation could provide a better understanding of UBE2 roles in oocyte maturation.
机译:在第一个减数分裂预言中被捕的脊椎动物卵母细胞必须在受精之前进行到第二个减数分子中期(MII)。这种减数过程需要精确控制蛋白质降解。卵母细胞中的一部分蛋白质降解由泛素缀合的酶系列,UBE2C和UBE2S的成员控制,众所周知,众所周知,分别参与单泛素化和聚泛素化。虽然UBE2酶在有丝分裂中进行了很好的研究,但它们对哺乳动物卵母细胞的贡献是相对未知的,并且仅在小鼠中进行了研究。在这里,我们调查了使用RNA注入方法对UBE2C和UBE2S对猪卵母细胞成熟的贡献。 UBE2S的过度表达预防卵母细胞的麻痹,并导致培养48小时的原子核(PN)。对于UBE2C过表达卵母细胞的长期培养,也观察到这种效果,表明在猪卵母细胞中快速逃逸的多毒液的有效性。虽然通过反义RNA(ASRNA)注射对UBE2C或UBE2S的抑制对卵母细胞成熟没有影响,但ASRNA注入的卵母细胞显示在单性发生后抑制PN形成。这些结果表明,UBE2S和UBE2C的某些因素泛滥在猪卵母细胞中逃脱的逃脱中的作用。进一步调查识别因素和单胞和/或多毒性如何有助于蛋白质降解可以更好地了解卵母细胞成熟中的UBE2作用。

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