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Origins of DNA-binding specificity: Role of protein contacts with the DNA backbone

  • Joel F. Schildbach
  • , A. Wali Karzai
  • , Brigitte E. Raumann
  • , Robert T. Sauer
  • Johns Hopkins University
  • Massachusetts Institute of Technology
  • University of California at San Francisco

Research output: Contribution to journalArticlepeer-review

57 Scopus citations

Abstract

A central question in protein-DNA recognition is the origin of the specificity that permits binding to the correct site in the presence of excess, nonspecific DNA. In the P22 Arc repressor, the Phe-10 side chain is part of the hydrophobic core of the free protein but rotates out to pack against the sugar-phosphate backbone of the DNA in the repressor-operator complex. Characterization of a library of position 10 variants reveals that Phe is the only residue that results in fully active Arc. One class of mutants folds stably but binds operator with reduced affinity; another class is unstable. FV10, one member of the first class, binds operator DNA and nonoperator DNA almost equally well. The affinity differences between FV10 and wild type indicate that each Phe-10 side chain contributes 1.5-2.0 kcal to operator binding but less than 0.5 kcal/mol to nonoperator binding, demonstrating that contacts between Phe-10 and the operator DNA backbone contribute to binding specificity. This appears to be a direct contribution as the crystal structure of the FV10 dimer is similar to wild type and the Phe-10-DNA backbone interactions are the only contacts perturbed in the cocrystal structure of the FV10-operator complex.

Original languageEnglish
Pages (from-to)811-817
Number of pages7
JournalProceedings of the National Academy of Sciences of the United States of America
Volume96
Issue number3
DOIs
StatePublished - Feb 2 1999

Keywords

  • Arc repressor
  • Mutants
  • Operator DNA
  • Phosphate contacts
  • Protein core

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