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Biophys J, January 2002, p. 93-98, Vol. 82, No. 1
and§
*Beckman Institute for Advanced Science and Technology and
Departments of Biochemistry, Physics, and
§Chemistry, University of Illinois, Urbana, Illinois 61801 USA
The fundamental processes by which proteins recognize and
bind to nucleic acids are critical to understanding cellular function. To explore the factors involved in protein-DNA recognition, we used
hydrostatic pressure to perturb the binding of the BamHI endonuclease to cognate DNA, both in experiment and in molecular dynamic simulations. A new technique of high-pressure gel mobility shift analysis was used to test the effects of elevated hydrostatic pressure on the binding of BamHI to its cognate
recognition sequence. Upon application of a pressure of 500 bar, the
equilibrium dissociation constant of BamHI binding to
the cognate site was found to increase nearly 10-fold. A challenge has
been to link this type of pure thermodynamic measurement to functional
events occurring at the molecular level. Thus, we used molecular
dynamic simulations at both ambient and elevated pressures to reveal
details of the direct and water-mediated interactions between
BamHI and cognate DNA, which allow explanation of the
effects of pressure on site-specific protein-DNA binding and complex stability.
Biophys J, January 2002, p. 93-98, Vol. 82, No. 1
© 2002 by the Biophysical Society 0006-3495/02/01/93/06 $2.00
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