Affiliation:
1. State Key Laboratory of Marine Environmental Science College of Ocean and Earth Sciences Xiamen University Xiamen Fujian 361102 China
2. Department of Chemistry Waterloo Institute for Nanotechnology University of Waterloo 200 University Avenue West Waterloo Ontario N2 L 3G1 Canada
Abstract
AbstractWhile many dye binding aptamers have been reported, most of them were for light‐up aptamers that can significantly enhance the quantum yield of fluorophores. Sulforhodamine B (SRhB) was used as a target previously to select both DNA and RNA aptamers, and the DNA aptamer was a G‐quadruplex that can bind to a number of rhodamine analogs. In addition, the previous selections were performed by immobilizing the target molecules. In this work, the library immobilization method was used to respectively select aptamers for SRhB and fluorescein. The SRhB aptamer has a non‐G‐quadruplex structure with a Kd of 1.0 μM measured from isothermal titration calorimetry. Upon titration of the aptamer, the fluorescence of SRhB increased 2.5‐fold, and this aptamer does not require Mg2+ for binding. Rhodamine B has even tighter binding suggesting binding through the xanthene moiety of the dyes. No binding was detected for fluorescein. For the fluorescein selection, a dominant aptamer sequence with a Kd of 147 μM was obtained. This study provides two new aptamers for two important fluorophores that can be used to study aptamer‐based separation, dye detection and catalysis. Comparison of these aptamers also provides insights into the effect of functional groups on aptamer binding.
Funder
Natural Sciences and Engineering Research Council of Canada
China Scholarship Council
Subject
General Chemistry,Catalysis,Organic Chemistry