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PUF proteins: RNA binding, protein interactions, and RNA regulation.

机译:PUF蛋白质:RNA结合,蛋白质相互作用和RNA调节。

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摘要

In eukaryotic cells, protein expression from mRNAs is highly controlled, often through regulatory elements in the mRNA 3' untranslated regions (3'UTRs). Regulatory proteins bind these sites and control mRNA stability, translation and localization. The PUF family of 3' UTR binding proteins modulates mRNA expression in a wide variety of eukaryotic species. They do so either by enhancing turnover or repressing translation, and act combinatorially with other regulatory proteins. PUF proteins function in a variety of developmental processes: embryonic development, stem cell maintenance, germline differentiation, and neuronal development.; I show that two Caenorhabditis elegans PUF proteins, FBF and PUF-8, differ in RNA-binding specificity. FBF activity requires the presence of a single 'extra' nucleotide in the middle of an eight-nucleotide site, whereas PUF-8 requires its absence. I also show FBF-1 and its close relative, FBF-2 (collectively called FBF), bind with similar affinity to multiple RNA sites. I discover that the binding affinity of FBF for these sites can be increased when bound to CPB-1.; The yeast PUF protein, Puf5p/Mpt5p, negatively regulates expression of the HO gene by binding to the 3' UTR of HO mRNA. Here I report that another PUF protein, Puf4p, also binds to and regulates expression of the same mRNA. Puf4p represses expression of an mRNA reporter that contains a HO 3' UTR. A third RNA binding protein, Ngr1p, also binds the same 3'UTR and represses expression of the mRNA. I propose that these three proteins - Mpt5p, Ngr1p, and Puf4p - work together to regulate HO mRNA in yeast.; Mpt5p physically interacts with Pop2p, which is a component of the Ccr4p/Pop2p/Not deadenylase complex, and Pop2p is required for PUF repression activity. Reconstituted deadenylation in vitro using purified components demonstrated that the PUF-Pop2p mechanism was conserved in yeast, worms and humans. I suggest that the PUF-Pop2p interaction underlies regulated deadenylation, repression, and mRNA decay by PUF proteins.
机译:在真核细胞中,通常通过mRNA 3'非翻译区(3'UTR)中的调控元件来高度控制mRNA的蛋白表达。调节蛋白结合这些位点并控制mRNA的稳定性,翻译和定位。 3'UTR结合蛋白的PUF家族可调节各种真核生物中的mRNA表达。它们通过提高周转率或抑制翻译来实现,并与其他调节蛋白共同发挥作用。 PUF蛋白在多种发育过程中起作用:胚胎发育,干细胞维持,种系分化和神经元发育。我显示两种秀丽隐杆线虫PUF蛋白,即FBF和PUF-8,在RNA结合特异性方面有所不同。 FBF活性要求在8个核苷酸位点的中间存在一个“额外”核苷酸,而PUF-8则需要其不存在。我还显示了FBF-1及其近亲FBF-2(统称为FBF)以相似的亲和力结合到多个RNA位点。我发现当与CPB-1结合时,可以提高FBF对这些位点的结合亲和力。酵母PUF蛋白Puf5p / Mpt5p通过与HO mRNA的3'UTR结合来负调控HO基因的表达。在这里,我报道了另一种PUF蛋白Puf4p也与同一mRNA结合并调节其表达。 Puf4p抑制含有HO 3'UTR的mRNA报告基因的表达。第三种RNA结合蛋白Ngr1p也结合相同的3'UTR并抑制mRNA的表达。我建议这三种蛋白-Mpt5p,Ngr1p和Puf4p-共同调节酵母中的HO mRNA。 Mpt5p与Pop2p物理相互作用,Pop2p是Ccr4p / Pop2p / Not Deadenylase复合物的组成部分,Pop2p是PUF抑制活性所必需的。使用纯化的成分在体外重建的腺苷酸化表明,PUF-Pop2p机制在酵母,蠕虫和人类中是保守的。我建议,PUF-Pop2p相互作用是PUF蛋白调节的腺苷酸化,阻遏和mRNA衰变的基础。

著录项

  • 作者

    Hook, Brad A.;

  • 作者单位

    The University of Wisconsin - Madison.;

  • 授予单位 The University of Wisconsin - Madison.;
  • 学科 Chemistry Biochemistry.
  • 学位 Ph.D.
  • 年度 2006
  • 页码 251 p.
  • 总页数 251
  • 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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