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Structure and functional implications of a complex containing a segment of U6 RNA bound by a domain of Prp24

机译:包含由Prp24域结合的U6 RNA片段的复合物的结构和功能含义

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摘要

U6 RNA plays a critical role in pre-mRNA splicing. Assembly of U6 into the spliceosome requires a significant structural rearrangement and base-pairing with U4 RNA. In the yeast Saccharomyces cerevisiae, this process requires the essential splicing factor Prp24. We present the characterization and structure of a complex containing one of Prp24's four RNA recognition motif (RRM) domains, RRM2, and a fragment of U6 RNA. NMR methods were used to identify the preferred U6 binding sequence of RRM2 (5′-GAGA-3′), measure the affinity of the interaction, and solve the structure of RRM2 bound to the hexaribonucleotide AGAGAU. Interdomain contacts observed between RRM2 and RRM3 in a crystal structure of the free protein are not detectable in solution. A structural model of RRM1 and RRM2 bound to a longer segment of U6 RNA is presented, and a partial mechanism for Prp24's annealing activity is proposed.
机译:U6 RNA在mRNA前剪接中起关键作用。 U6组装到剪接体中需要重大的结构重排和与U4 RNA的碱基配对。在酵母酿酒酵母中,该过程需要必需的剪接因子Prp24。我们介绍了包含Prp24的四个RNA识别基序(RRM)域,RRM2和U6 RNA片段之一的复合物的表征和结构。 NMR方法用于鉴定RRM2(5'-GAGA-3')的优选U6结合序列,测量相互作用的亲和力,并解决与六核糖核苷酸AGAGAU结合的RRM2的结构。在溶液中无法检测到游离蛋白晶体结构中RRM2和RRM3之间的域间接触。提出了与U6 RNA较长片段结合的RRM1和RRM2的结构模型,并提出了Prp24退火活性的部分机理。

著录项

  • 来源
    《RNA》 |2010年第4期|792-804|共13页
  • 作者单位

    Department of Biochemistry, University of Wisconsin–Madison, Madison, Wisconsin 53706, USA;

    Department of Biochemistry, University of Wisconsin–Madison, Madison, Wisconsin 53706, USA;

    Department of Biomolecular Chemistry, University of Wisconsin–Madison, Madison, Wisconsin 53706, USA;

    Department of Biochemistry, University of Wisconsin–Madison, Madison, Wisconsin 53706, USA;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    U6 snRNA; Prp24; RRM; ribonucleoprotein; NMR; RNA;

    机译:U6 snRNA;Prp24;RRM;核糖核蛋白;NMR;RNA;

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