• Title of article

    CapSeq and CIP-TAP Identify Pol II Start Sites and Reveal Capped Small RNAs as C. elegans piRNA Precursors

  • Author/Authors

    Weifeng Gu، نويسنده , , Heng-Chi Lee، نويسنده , , Daniel Chaves، نويسنده , , Elaine M. Youngman، نويسنده , , Gregory J. Pazour، نويسنده , , Darryl Conte Jr.، نويسنده , , Craig C. Mello، نويسنده ,

  • Issue Information
    هفته نامه با شماره پیاپی سال 2012
  • Pages
    13
  • From page
    1488
  • To page
    1500
  • Abstract
    Piwi-interacting (pi) RNAs are germline-expressed small RNAs linked to epigenetic programming. C. elegans piRNAs are thought to be transcribed as independent gene-like loci. To test this idea and to identify potential transcription start (TS) sites for piRNA precursors, we developed CapSeq, an efficient enzymatic method for 5′ anchored RNA profiling. Using CapSeq, we identify candidate TS sites, defined by 70–90 nt sequence tags, for >50% of annotated Pol II loci. Surprisingly, however, these CapSeq tags failed to identify the overwhelming majority of piRNA loci. Instead, we show that the likely piRNA precursors are ∼26 nt capped small (cs) RNAs that initiate precisely 2 nt upstream of mature piRNAs and that piRNA processing or stability requires a U at the csRNA +3 position. Finally, we identify a heretofore unrecognized class of piRNAs processed from csRNAs that are expressed at promoters genome wide, nearly doubling the number of piRNAs available for genome surveillance.
  • Journal title
    CELL
  • Serial Year
    2012
  • Journal title
    CELL
  • Record number

    1021500