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Pre-mRNA processing includes N-6 methylation of adenosine residues that are retained in mRNA exons and the fallacy of 'RNA epigenetics'

机译:前mRNA处理包括保留在mRNA外显子和“RNA表观遗传学”的谬误中保留的腺苷残基的N-6甲基化

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摘要

By using a cell fraction technique that separates chromatin-associated nascent RNA, newly completed nucleoplasmic mRNA and cytoplasmic mRNA, we have shown in a previous study that residues in exons are methylated (m(6)A) in nascent pre-mRNA and remain methylated in the same exonic residues in nucleoplasmic and cytoplasmic mRNA. Thus, there is no evidence of a substantial degree of demethylation in mRNA exons that would correspond to so-called "epigenetic" demethylation. The turnover rate of mRNA molecules is faster, depending on m(6)A content in HeLa cell mRNA, suggesting that specification of mRNA stability may be the major role of m(6)A exon modification. In mouse embryonic stem cells (mESCs) lacking Mettl3, the major mRNA methylase, the cells continue to grow, making the same mRNAs with unchanged splicing profiles in the absence (90%) of m(6)A in mRNA, suggesting no common obligatory role of m(6)A in splicing. All these data argue strongly against a commonly used "reversible dynamic methylation/demethylation" of mRNA, calling into question the concept of "RNA epigenetics" that parallels the well-established role of dynamic DNA epigenetics.
机译:通过使用分离染色质的新生RNA的细胞级分技术,新完成的骨基mRNA和细胞质mRNA,我们在先前的研究中显示,外显子中的残留物在新生前预-mRNA中甲基化(M(6)A)并保持甲基化在骨髓和细胞质mRNA中的相同外部残留物中。因此,没有证据表明MRNA外显子的脱甲酰化,其对应于所谓的“表观遗传”去甲基化。根据M(6)MRA细胞mRNA中的含量,mRNA分子的周转率更快,表明mRNA稳定性的规格可能是M(6)外显子改性的主要作用。在小鼠胚胎干细胞(MESCS)缺乏METT13,主要mRNA甲基酶,细胞继续生长,使得在mRNA中的M(6)A A的缺失(& 90%)中具有不变的剪接曲线的MRNA相同的MRNA,表明没有M(6)A拼接的常见义务作用。所有这些数据都强烈地反对mRNA的常用的“可逆动态甲基化/去甲基化”,调用质疑“RNA表观遗传学”的概念,使动态DNA表观遗传学的良好作用。

著录项

  • 来源
    《RNA》 |2018年第3期|共6页
  • 作者单位

    Rockefeller Univ Lab Mol Neurooncol New York NY 10065 USA;

    Rockefeller Univ Lab Mol Neurooncol New York NY 10065 USA;

    Rockefeller Univ Mol Cell Biol Lab New York NY 10065 USA;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 生物化学;
  • 关键词

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