1. Displacement of Mn2+ from RNA by K+, Mg2+, Neomycin B, and an Arginine-Rich Peptide: Indirect Detection of Nucleic Acid/Ligand Interactions Using Phosphorus Relaxation Enhancement
- Author
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Michael Sturgess, Christopher T. Badger, Fredric L. Freedman, Jack S. Summers, and John Shimko
- Subjects
Stereochemistry ,Metal ions in aqueous solution ,Molecular Sequence Data ,Fluorescence Polarization ,Peptide ,Arginine ,Biochemistry ,Catalysis ,Colloid and Surface Chemistry ,Cations ,Molecule ,Magnesium ,Amino Acid Sequence ,Nuclear Magnetic Resonance, Biomolecular ,chemistry.chemical_classification ,Manganese ,Base Sequence ,Chemistry ,Cationic polymerization ,RNA ,General Chemistry ,Ligand (biochemistry) ,Small molecule ,Kinetics ,Metals ,Potassium ,Nucleic acid ,Nucleic Acid Conformation ,Peptides ,Framycetin - Abstract
We have developed a novel method to study the interactions of nucleic acids with cationic species. The method, called phosphorus relaxation enhancement (PhoRE), uses (1)H-detected (31)P NMR of exogenous probe ions to monitor changes in the equilibrium between free Mn(2+) and Mn(2+) bound to the RNA. To demonstrate the technique, we describe the interactions of four RNA molecules with metal ions (K(+) and Mg(2+)), a small molecule drug (neomycin b), and a cationic peptide (RSG1.2). In each case, cationic ligand binding caused Mn(2+) to be displaced from the RNA. Free Mn(2+) was determined from its effect on the T(2) NMR relaxation rate of either phosphite (HPO(3)(2-)) or methyl phosphite (MeOPH, CH(3)OP(H)O(2-)). Using this method, the effects of [RNA] as low as 1 microM could be measured in 20 min of accumulation using a low field (200 MHz) instrument without pulsed field gradients. Cation association behavior was sequence and [RNA] dependent. At low [K(+)], Mn(2+) association with each of the RNAs decreased with increasing [K(+)] until approximately 40 mM, where saturation was reached. While saturating K(+) displaced all the bound Mn(2+) from a 31-nucleotide poly-uridine (U(31)), Mn(2+) remained bound to each of three hairpin-forming sequences (A-site, RRE1, and RRE2), even at 150 mM K(+). Bound Mn(2+) was displaced from each of the hairpins by Mg(2+), allowing determination of Mg(2+) dissociation constants (K(d,Mg)) ranging from 50 to 500 microM, depending on the RNA sequence and [K(+)]. Both neomycin b and RSG1.2 displaced Mn(2+) upon binding the hairpins. At [RNA] approximately 3 microM, RRE1 bound a single equivalent of RSG1.2, whereas neither RRE2 nor A-site bound the peptide. These behaviors were confirmed by fluorescence polarization using TAMRA-labeled peptide. At 2.7 microM RNA, the A-site hairpin bound a single neomycin b molecule. The selectivity of RSG1.2 binding was greatly diminished at higher [RNA]. Similarly, each hairpin bound multiple equivalents of neomycin at the higher [RNA]. These results demonstrate the utility of the PhoRE method for characterizing metal binding behaviors of nucleic acids and for studying RNA/ligand interactions.
- Published
- 2002
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