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Stretching DNA to quantify nonspecific protein binding.

Abstract
Nonspecific binding of regulatory proteins to DNA can be an important mechanism for target search and storage. This seems to be the case for the lambda repressor protein (CI), which maintains lysogeny after infection of E. coli. CI binds specifically at two distant regions along the viral genome and induces the formation of a repressive DNA loop. However, single-molecule imaging as well as thermodynamic and kinetic measurements of CI-mediated looping show that CI also binds to DNA nonspecifically and that this mode of binding may play an important role in maintaining lysogeny. This paper presents a robust phenomenological approach using a recently developed method based on the partition function, which allows calculation of the number of proteins bound nonspecific to DNA from measurements of the DNA extension as a function of applied force. This approach was used to analyze several cycles of extension and relaxation of λ DNA performed at several CI concentrations to measure the dissociation constant for nonspecific binding of CI (~100 nM), and to obtain a measurement of the induced DNA compaction (~10%) by CI.
AuthorsSachin Goyal, Chandler Fountain, David Dunlap, Fereydoon Family, Laura Finzi
JournalPhysical review. E, Statistical, nonlinear, and soft matter physics (Phys Rev E Stat Nonlin Soft Matter Phys) Vol. 86 Issue 1 Pt 1 Pg. 011905 (Jul 2012) ISSN: 1550-2376 [Electronic] United States
PMID23005450 (Publication Type: Journal Article, Research Support, N.I.H., Extramural)
Chemical References
  • DNA-Binding Proteins
  • DNA
Topics
  • Computer Simulation
  • DNA (chemistry, ultrastructure)
  • DNA-Binding Proteins (chemistry, ultrastructure)
  • Micromanipulation (methods)
  • Models, Chemical
  • Molecular Probe Techniques
  • Protein Binding
  • Protein Interaction Mapping (methods)

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