A colorimetric and fluorometric dual-mode carbon dots probe derived from phenanthroline precursor for the selective detection of Fe2+ and Fe3.

Abstract

Iron's metabolism is heavily involved in the regulation of redox balance for cell functions, however, the simultaneous monitoring of Fe2+/3+ concentration is still a great challenge due to their transitional nature in biological systems. A novel type of carbon dots (CDs) was synthesized by solvothermal treatment with 5-amino-1,10-phenanthroline (Aphen) and salicylic acid as precursors, and the resulting targeted CDs (T-CDs) were used to simultaneously detect Fe2+ and Fe3+. Comprehensive experimental characterizations revealed that the strong binding affinity of Aphen moiety to Fe2+ leads to the formation of rigid T-CDs aggregates, which causes a substantial enhancement of fluorescence intensity, whereas Fe3+ could cause the fluorescence quenching of T-CDs due to the oxidation-reduction induced electron transfer. These different fluorescence responses allow T-CDs to sensitively differentiate Fe2+ from Fe3+, and give the limit of detection (LOD) of 1.78 and 2.78μM for Fe2+ and Fe3+, respectively. Furthermore, the Aphen dominated structure endows the T-CDs with a colorimetric response to Fe2+ with a LOD of 0.13μM, which is very different from Fe3+. Thus, the dynamic changes of Fe2+ and Fe3+ in solution can be accurately monitored by T-CDs within the total iron concentration of 50μM, which is probably the most sensitive dual-mode probe reported so far. In addition, this probe is successfully applied to detect the Fe2+/3+ concentration in cells, demonstrating a huge application potential in the sensing of the dynamic equilibrium of these important transition metals during the cell metabolism or stimulated process. The dynamic changes of Fe2+ and Fe3+ in solution can be accurately monitored by carbon dots based on the colorimetric and fluorometric dual-mode.