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(Received for publication, March 18, 1996, and in revised form, May 24, 1996)
From the Institut de Pharmacologie et de Biologie Structurale,
CNRS, 205, route de Narbonne, 31077 Toulouse, France
Preferential binding to single- or
double-stranded nucleic acids is important for the activity of many
proteins that process RNA and DNA. We have investigated the mechanism
of strandedness discrimination with peptides derived from the putative
DNA-binding domain of the RecA protein, a bacterial recombinase that
modulates its affinity for single-stranded DNA by means of ATP binding
and hydrolysis. Contributions of electrostatic and non-electrostatic
interactions to binding of these peptides with polynucleotides were
evaluated by fluorescence spectroscopy as a function of salt
concentration and peptide charge. Binding of these peptides to single-
and double-stranded nucleic acids was dominated by non-electrostatic
interactions. Small electrostatic contributions selectively enhanced
peptide complexation with single-stranded nucleic acids. Similar
results were observed in control experiments carried out with
tripeptides containing charged and aromatic amino acid residues. It was
possible to modify the strandedness preference of
peptide-polynucleotide complexes by changing electrostatic
contributions to the binding free energy. These observations suggest a
mechanism whereby some proteins that interact with DNA or RNA might
determine and regulate their relative affinity for single- and
double-stranded nucleic acids.
Volume 271, Number 33,
Issue of August 16, 1996
pp. 19675-19679
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
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