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The enhancer of decapping proteins, Edc1p and Edc2p, bind RNA and stimulate the activity of the decapping enzyme.

机译：开盖蛋白的增强子Edc1p和Edc2p与RNA结合并刺激开盖酶的活性。

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摘要

A major pathway of eukaryotic mRNA turnover initiates with deadenylation, which allows a decapping reaction leading to 5'-3' exonucleolytic degradation. A key control point in this pathway is the decapping of the mRNA. Two proteins, Edc1 and Edc2, were genetically identified previously as enhancers of the decapping reaction. In this work, we demonstrate that Edc1p and Edc2p are RNA-binding proteins. In addition, recombinant Edc1p or Edc2p stimulates mRNA decapping in cell-free extracts or with purified decapping enzyme. These results suggest that Edc1p and Edc2p activate decapping directly by binding to the mRNA substrate and enhancing the activity of the decapping enzyme. Interestingly, edc1Delta strains show defects in utilization of glycerol as a carbon source and misregulation of several mRNAs in response to carbon-source changes. This identifies a critical role for decapping and Edc1p in alterations of gene expression in response to carbon-source changes.

机译：真核mRNA更新的主要途径以腺苷酸化开始，其允许去盖反应，导致5'-3'外切核酸降解。该途径中的关键控制点是mRNA的脱盖。以前在基因上鉴定了两种蛋白质，Edc1和Edc2，作为脱盖反应的增强子。在这项工作中，我们证明Edc1p和Edc2p是RNA结合蛋白。此外，重组的Edc1p或Edc2p可以刺激无细胞提取物中或纯化的脱盖酶对mRNA的脱盖。这些结果表明Edc1p和Edc2p通过与mRNA底物结合并增强去盖酶的活性直接激活去盖作用。有趣的是，edc1Delta菌株在利用甘油作为碳源以及响应碳源变化而调节数个mRNA时显示出缺陷。这确定了去盖和Edc1p在响应碳源变化的基因表达改变中的关键作用。

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《RNA》 |2003年第2期|共13页
作者
Schwartz D; Decker CJ; Parker R;
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正文语种 eng
中图分类核酸;
关键词
Endoribonucleases; RNA; Saccharomyces cerevisiae Proteins; 内切核糖核酸酶类;

机译：Endoribonucleases;RNA;Saccharomyces cerevisiae Proteins;内切核糖核酸酶类;

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1. The enhancer of decapping proteins, Edc1p and Edc2p, bind RNA and stimulate the activity of the decapping enzyme. [J] . Schwartz D, Decker CJ, Parker R RNA . 2003,第2期

机译：开盖蛋白的增强子Edc1p和Edc2p与RNA结合并刺激开盖酶的活性。
2. Evolutionary conservation supports ancient origin for Nudt16, a nuclear-localized, RNA-binding, RNA-decapping enzyme. [J] . Taylor Melissa J., Peculis Brenda A. Nucleic Acids Research . 2008,第18期

机译：进化保护支持了Nudt16的古老起源，Nudt16是一种核定位，RNA结合，RNA脱盖的酶。
3. Enzymatically stable 5' mRNA cap analogs: synthesis and binding studies with human DcpS decapping enzyme. [J] . Kalek M, Jemielity J, Darzynkiewicz ZM, Bioorganic and Medicinal Chemistry . 2006,第9期

机译：酶稳定的5'mRNA帽类似物：人DcpS脱盖酶的合成和结合研究。
4. A deep neural network approach using distributed representations of RNA sequence and structure for identifying binding site of RNA-binding proteins [C] . Lei Deng, Youzhi Liu, Yechuan Shi, IEEE International Conference on Bioinformatics and Biomedicine . 2019

机译：使用RNA序列和结构的分布式表示的深层神经网络方法，用于识别RNA结合蛋白的结合位点
5. Coactivator regulation of active site chemistry in the mRNA decapping enzyme Dcp2. [D] . Aglietti, Robin A. 2014

机译：mRNA脱盖酶Dcp2中活性位化学的共激活因子调节。
6. The enhancer of decapping proteins Edc1p and Edc2p bind RNA and stimulate the activity of the decapping enzyme [O] . DAVID SCHWARTZ, CAROLYN J. DECKER, ROY PARKER 2003

机译：解封蛋白的增强子Edc1p和Edc2p与RNA结合并刺激解封酶的活性
7. The enhancer of decapping proteins, Edc1p and Edc2p, bind RNA and stimulate the activity of the decapping enzyme [O] . SCHWARTZ, DAVID, DECKER, CAROLYN J., PARKER, ROY 2003

机译：解封蛋白的增强子Edc1p和Edc2p与RNA结合并刺激解封酶的活性

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