Frontal Analysis in Microchip CE: a Simple and Accurate Method for Determination of Protein-DNA Dissociation Constant

Overview

Journal Electrophoresis

Specialty Chemistry

Date 2007 Feb 23

PMID 17315151

Citations 4

Authors

Maojun Gong

Kenneth R Wehmeyer

Patrick A Limbach

William R Heineman

Affiliations

Soon will be listed here.

Abstract

Equilibrium constants, such as the dissociation constant (K(d)), are a key measurement of noncovalent interactions that are of importance for the proper functioning of molecules in living systems. Frontal analysis (FA) is a simple and accurate CE method for the determination of K(d). Microchip CE coupled with LIF detection was used to determine K(d) of protein-DNA interactions using the FA method. A model system of IgE and the IgE-binding aptamer was selected to demonstrate the capability of FA in microchip CE. Because the fluorescence emission was dependent on the dye migration velocity, the velocity of the free aptamer was adjusted to be the same as that of the aptamer-IgE complex by setting up individual separation voltage configurations for the free and bound aptamers. The ratio of the free and bound aptamers in the equilibrium mixture was directly measured from the heights of their plateaus detected at 1.0 cm from the intersection of the microchip, and no internal standard was needed. The K(d) of the IgE-aptamer pair was determined as 6 +/- 2 nM which is consistent with the reported results (8 nM).

Citing Articles

Aptamers against Immunoglobulins: Design, Selection and Bioanalytical Applications.

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Methods for measuring aptamer-protein equilibria: a review.

Jing M, Bowser M Anal Chim Acta. 2011; 686(1-2):9-18.

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Measurement of dissociation rate of biomolecular complexes using CE.

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Protein-aptamer binding studies using microchip affinity capillary electrophoresis.

Gong M, Nikcevic I, Wehmeyer K, Limbach P, Heineman W Electrophoresis. 2008; 29(7):1415-22.

PMID: 18324729 PMC: 3529586. DOI: 10.1002/elps.200700777.

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