A new concept to construct photoresponsive nanozyme through the in situ deposition of electron transporting material (ETM) on BiOBr nanoplates was proposed. That was, the spontaneous coordination of ferricyanide ions (i.e., [Fe(CN)6]3-) onto the surface of BiOBr formed electron transporting material (ETM), which efficiently prevented electron-hole recombination and led to efficient enzyme mimicking activity under light stimuli. Moreover, the formation of the photoresponsive nanozyme was regulated by pyrophosphate ions (PPi) due to the competitive coordination of PPi with [Fe(CN)6]3- onto the surface of BiOBr. This phenomenon allowed the construction of an engineerable photoresponsive nanozyme that was coupled with the rolling circle amplification (RCA) reaction to elucidate a novel bioassay for chloramphenicol (CAP, taken as a model analyte). The developed bioassay manifested the merits of label-free, immobilization-free and with efficiently amplified signal. Quantitative analysis of CAP in a wide linear range from 0.05 to 100 nM with the detection limit of 0.015 nM was realized, which endowed the methodology with sufficiently high sensitivity. It is expected to be a powerful signal probe in bioanalytical field by virtue of its switchable and fascinating visible-light-induced enzyme mimicking activity.
Keywords: BiOBr nanoplates; Electron transporting material; Homogeneous bioassay; In situ formation; Photoresponsive nanozyme.
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