Genome-wide detection and analysis of hippocampus core promoters using DeepCAGE

  1. Eivind Valen1,
  2. Giovanni Pascarella2,
  3. Alistair Chalk3,
  4. Norihiro Maeda4,
  5. Miki Kojima4,
  6. Chika Kawazu4,
  7. Mitsuyoshi Murata4,
  8. Hiromi Mishiyori4,
  9. Dejan Lazarevich2,
  10. Dario Motti2,
  11. Troels Torben Marstrand1,
  12. Man-Hung Eric Tang1,
  13. Xiaobei Zhao1,
  14. Anders Krogh5,
  15. Ole Winther5,
  16. Takahiro Arakawa4,
  17. Jun Kawai4,
  18. Christine Wells3,
  19. Carsten Daub4,
  20. Matthias Harbers6,
  21. Yoshihide Hayashizaki4,
  22. Stefano Gustincich2,
  23. Albin Sandelin1, and
  24. Piero Carninci4,7
  1. 1 University of Copenhagen;
  2. 2 International School for Advanced Studies (SISSA);
  3. 3 Griffith University;
  4. 4 RIKEN;
  5. 5 University of Coopenhagen;
  6. 6 Dnaform

Abstract

Finding and characterizing mRNAs, their transcription start sites (TSS) and their associated promoters is a major focus in post-genome biology. Mammalian cells have at least 5-10 magnitudes more TSS than previously believed, and deeper sequencing is necessary to detect all active promoters in a given tissue. Here, we present a new method for high throughput sequencing of 5' cDNA tags, DeepCAGE: merging the Cap Analysis of Gene Expression method with ultra-high throughput sequence technology. We apply DeepCAGE to characterize 1.4 million sequenced TSS from mouse hippocampus and reveal a wealth of novel core promoters which are preferentially used in hippocampus: this is the most comprehensive promoter dataset for any tissue to date. Using this data, we present evidence indicating a key role for the Arnt2 transcription factor in hippocampus gene regulation. DeepCAGE can also detect promoters used only in a small subset of cells within the complex tissue.

Footnotes

    • Received August 8, 2008.
    • Accepted December 3, 2008.

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  1. Published in Advance December 11, 2008, doi: 10.1101/gr.084541.108 Genome Res. gr.084541.108 Copyright © 2008, Cold Spring Harbor Laboratory Press

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