Abstract
Alkaline phosphatase (ALP) has been known to participate in the multiple pathways of cell metabolism. Here, a ratiometric fluorescent probe was designed for determination of ALP activity based on Ce-Tb@GMP. The Ce-Tb@GMP nanoparticles were prepared via the self-assembly of guanosine monophosphate (GMP) with terbium and cerium ions (Ce3+, Tb3+). The Ce-Tb@GMP nanoparticles own two luminescent centers, Tb and Ce, respectively. In presence of ALP, the phosphate ester in GMP was hydrolyzed and the structure of Ce-Tb@GMP was destroyed. Moreover, the coordination effect of Ce3+, Tb3+ and ligand GMP was significantly declined and the energy transfer efficiency from Ce3+, GMP to Tb3+ was reduced. Therefore, the fluorescence emission of Tb3+ and Ce3+ was quenched and the fluorescence intensity ratio (F552/F384) gradually decreased. This probe displayed low limit detection 0.12 mU/mL under the concentration range of 0.2–60 mU/mL. Meanwhile, the method accomplished the detection of ALP in a diluted serum sample of 5%. This strategy will make a construction for the application of fluorescent probes in bioanalytical sciences.
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More From: Journal of Photochemistry and Photobiology A: Chemistry
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