4.8 Article

Helical coherence of DNA in crystals and solution

Journal

NUCLEIC ACIDS RESEARCH
Volume 36, Issue 17, Pages 5540-5551

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/nar/gkn514

Keywords

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Funding

  1. Alexander von Humboldt foundation
  2. Engineering and Physical Sciences Research Council [GR/S31068/01]
  3. Royal Society
  4. Liverhulme Trust
  5. Intramural Research Program
  6. National Institute of Child Health and Human Development
  7. National Institutes of Health
  8. Engineering and Physical Sciences Research Council [GR/S31068/01] Funding Source: researchfish

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The twist, rise, slide, shift, tilt and roll between adjoining base pairs in DNA depend on the identity of the bases. The resulting dependence of the double helix conformation on the nucleotide sequence is important for DNA recognition by proteins, packaging and maintenance of genetic material, and other interactions involving DNA. This dependence, however, is obscured by poorly understood variations in the stacking geometry of the same adjoining base pairs within different sequence contexts. In this article, we approach the problem of sequence-dependent DNA conformation by statistical analysis of X-ray and NMR structures of DNA oligomers. We evaluate the corresponding helical coherence length-a cumulative parameter quantifying sequence-dependent deviations from the ideal double helix geometry. We find, e. g. that the solution structure of synthetic oligomers is characterized by 100-200A coherence length, which is similar to -150 angstrom coherence length of natural, salmon-sperm DNA. Packing of oligomers in crystals dramatically alters their helical coherence. The coherence length increases to 800-1200 angstrom, consistent with its theoretically predicted role in interactions between DNA at close separations.

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