| Article ID | Journal | Published Year | Pages | File Type |
|---|---|---|---|---|
| 1243625 | Talanta | 2014 | 6 Pages |
•A novel “turn-on” fluorescent probe (Cu2+–nuclear fast red) was shown for detecting guanine.•The interaction of NFR, Cu2+ and guanine was discussed.•The proposed method exhibits a high sensitivity and selectivity for guanine.•The present spectrofluoremetric method can be applied successfully to determine guanine in real samples.
A novel fluorescence method for the determination of guanine was developed based on the fluorescence enhancement of Cu2+–nuclear fast red complex in the presence of guanine in Tris–HCl buffer. The complex of Cu2+ with nuclear fast red resulted in a dramatic quenching of the fluorescence intensity. Nuclear fast red were dissociated from the complex with the addition of guanine due to the strong interaction between guanine and Cu2+, which caused the fluorescence enhancement. The enhanced fluorescence intensity was well proportional to the concentration of guanine in the range of 4.96×10−8–1.09×10−6 mol/L with the limit of detection 1.9×10−8 mol/L. The method has been applied successfully to the determination of guanine in serum and DNA samples, and the recoveries were from 96.0% to 104.8%.
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