Discovery of functional noncoding elements by digital analysis of chromatin structure

  1. Peter J. Sabo*,
  2. Michael Hawrylycz*,
  3. James C. Wallace*,
  4. Richard Humbert*,
  5. Man Yu,
  6. Anthony Shafer*,
  7. Janelle Kawamoto*,
  8. Robert Hall*,
  9. Joshua Mack*,
  10. Michael O. Dorschner*,
  11. Michael McArthur*, and
  12. John A. Stamatoyannopoulos*,
  1. *Department of Molecular Biology, Regulome, 2211 Elliott Avenue, Suite 600, Seattle, WA 98121; and Division of Medical Genetics, University of Washington, 1705 NE Pacific Street, Seattle, WA 98195

  1. Communicated by Stanley M. Gartler, University of Washington, Seattle, WA, October 6, 2004 (received for review August 10, 2004)

Abstract

We developed a quantitative methodology, digital analysis of chromatin structure (DACS), for high-throughput, automated mapping of DNase I-hypersensitive sites and associated cis-regulatory sequences in the human and other complex genomes. We used 19/20-bp genomic DNA tags to localize individual DNase I cutting events in nuclear chromatin and produced ≈257,000 tags from erythroid cells. Tags were mapped to the human genome, and a quantitative algorithm was applied to discriminate statistically significant clusters of independent DNase I cutting events. We show that such clusters identify both known regulatory sequences and previously unrecognized functional elements across the genome. We used in silico simulation to demonstrate that DACS is capable of efficient and accurate localization of the majority of DNase I-hypersensitive sites in the human genome without requiring an independent validation step. A unique feature of DACS is that it permits unbiased evaluation of the chromatin state of regulatory sequences from widely separated genomic loci. We found surprisingly large differences in the accessibility of distant regulatory sequences, suggesting the existence of a hierarchy of nuclear organization that escapes detection by conventional chromatin assays.

Footnotes

  • To whom correspondence should be addressed. E-mail: jstam{at}regulome.com.

  • Author contributions: P.J.S., M.M., and J.A.S. designed research; P.J.S., M.H., M.Y., A.S., J.K., R. Hall, J.M., M.O.D., and M.M. performed research; M.H., J.C.W. and R. Humbert contributed new reagents/analytic tools; P.J.S., M.H., J.C.W., R. Humbert, M.M., and J.A.S. analyzed data; and P.J.S., M.H., and J.A.S. wrote the paper.

  • Abbreviations: DACS, digital analysis of chromatin structure; HS, hypersensitive site; HSqPCR, hypersensitivity quantitative PCR; n-cluster, n-tag cluster; PPV, positive predictive value; TSS, transcriptional start site.

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  1. Published online before print November 18, 2004, doi: 10.1073/pnas.0407387101 PNAS November 30, 2004 vol. 101 no. 48 16837-16842
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