Issue 22, 2009

Cation localization and movement within DNA thrombin binding aptamer in solution

Abstract

The thrombin binding aptamer, 15-mer oligonucleotide d[G2T2G2TGTG2T2G2], was folded into the well known antiparallel unimolecular G-quadruplex in the presence of 15NH4+ ions. Although the formed G-quadruplex is thermodynamically less stable than in the presence of K+ ions, the loop conformations and folding topology are the same. On the other hand, titration of Na+ ions into an aqueous solution of TBA resulted in the formation of one major and several minor species of G-quadruplexes. Solution-state NMR was used to localize 15NH4+ ions between the two G-quartets within the core of the structure, and to determine the equilibrium binding constant, which equals 190 M−1. No other potential cation binding sites were resolved on the time-scale of NMR spectrometer. Exchange of 15NH4+ ions between the inner binding site and bulk solution is characterized by the exchange rate constant of 1.0 s−1 at 15 °C. T4 and T13 form a noncanonical base pair, which greatly affects access of bulk ions into the cation binding site in the G-quadruplex core. G2 and G11 exhibit out of plane bending towards the two TT loops away from the bound 15NH4+ ions, which in turn exposes them to more efficient chemical exchange processes with bulk ions and water.

Graphical abstract: Cation localization and movement within DNA thrombin binding aptamer in solution

Supplementary files

Article information

Article type
Paper
Submitted
21 Jul 2009
Accepted
18 Aug 2009
First published
21 Sep 2009

Org. Biomol. Chem., 2009,7, 4677-4684

Cation localization and movement within DNA thrombin binding aptamer in solution

M. Trajkovski, P. Šket and J. Plavec, Org. Biomol. Chem., 2009, 7, 4677 DOI: 10.1039/B914783G

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