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Intron removal requires proofreading of U2AF/3 ' splice site recognition by DEK

机译:去除内含子需要DEK对U2AF / 3'剪接位点进行校对

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摘要

Discrimination between splice sites and similar, nonsplice sequences is essential for correct intron removal and messenger RNA formation in eukaryotes. The 65- and 35-kD subunits of the splicing factor U2AF, U2AF(65) and U2AF(35), recognize, respectively, the pyrimidine-rich tract and the conserved terminal AG present at metazoan 3' splice sites. We report that DEK, a chromatin- and RNA-associated protein mutated or overexpressed in certain cancers, enforces 3' splice site discrimination by U2AF. DEK phosphorylated at serines 19 and 32 associates with U2AF(35), facilitates the U2AF(35)-AG interaction and prevents binding of U2AF(65) to pyrimidine tracts not followed by AG. DEK and its phosphorylation are required for intron removal, but not for splicing complex assembly, which indicates that proofreading of early 3' splice site recognition influences catalytic activation of the spliceosome.
机译:剪接位点和类似的非剪接序列之间的区别对于正确去除内含子和真核生物中信使RNA的形成至关重要。剪接因子U2AF,U2AF(65)和U2AF(35)的65-kD亚基和35-kD亚基分别识别存在于后生动物3'剪接位点的嘧啶富集区和保守末端AG。我们报告说,DEK,在某些癌症中突变或过度表达的与染色质和RNA相关的蛋白质,通过U2AF强制3'剪接位点识别。丝氨酸19和32磷酸化的DEK与U2AF(35)缔合,促进U2AF(35)-AG相互作用,并防止U2AF(65)结合到未由AG参与的嘧啶区。内含子的去除需要DEK及其磷酸化,但剪接复杂的装配体则不需要,这表明早期3'剪接位点识别的校对会影响剪接体的催化活化。

著录项

  • 来源
    《Science》 |2006年第5782期|p. 1961-1965|共5页
  • 作者单位

    Ctr Regulacio Genom, Barcelona 08003, Spain;

    Inst Catalana Rec & Estudis Avancats, Barcelona 08003, Spain;

    Univ Pompeu Fabra, Barcelona 08003, Spain;

    European Mol Biol Lab, D-69117 Heidelberg, Germany;

  • 收录信息 美国《科学引文索引》(SCI);美国《工程索引》(EI);美国《生物学医学文摘》(MEDLINE);美国《化学文摘》(CA);
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 自然科学总论;
  • 关键词

    PROTEIN; U2AF(35); AG;

    机译:蛋白质;U2AF(35);AG;
  • 入库时间 2022-08-18 02:56:20

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