PLoS ONE (Nov 2010)

Efficient double fragmentation ChIP-seq provides nucleotide resolution protein-DNA binding profiles.

  • Michal Mokry,
  • Pantelis Hatzis,
  • Ewart de Bruijn,
  • Jan Koster,
  • Rogier Versteeg,
  • Jurian Schuijers,
  • Marc van de Wetering,
  • Victor Guryev,
  • Hans Clevers,
  • Edwin Cuppen

DOI
https://doi.org/10.1371/journal.pone.0015092
Journal volume & issue
Vol. 5, no. 11
p. e15092

Abstract

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Immunoprecipitated crosslinked protein-DNA fragments typically range in size from several hundred to several thousand base pairs, with a significant part of chromatin being much longer than the optimal length for next-generation sequencing (NGS) procedures. Because these larger fragments may be non-random and represent relevant biology that may otherwise be missed, but also because they represent a significant fraction of the immunoprecipitated material, we designed a double-fragmentation ChIP-seq procedure. After conventional crosslinking and immunoprecipitation, chromatin is de-crosslinked and sheared a second time to concentrate fragments in the optimal size range for NGS. Besides the benefits of increased chromatin yields, the procedure also eliminates a laborious size-selection step. We show that the double-fragmentation ChIP-seq approach allows for the generation of biologically relevant genome-wide protein-DNA binding profiles from sub-nanogram amounts of TCF7L2/TCF4, TBP and H3K4me3 immunoprecipitated material. Although optimized for the AB/SOLiD platform, the same approach may be applied to other platforms.