A non-aggregation colorimetric assay for thrombin based on catalytic properties of silver nanoparticles

•An AgNP-based non-aggregation colorimetric aptasensor was first developed.•The colorimetric principle was based on AgNP-catalyzed reductive degradation of RhB.•This assay combined magnetic separation with nanocatalytic amplification.•The detection limit of thrombin was as low as 0.2nM with excellen...

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Veröffentlicht in:Analytica chimica acta 2014-01, Vol.807, p.120-125
Hauptverfasser: Li, Jie, Li, Wei, Qiang, Weibing, Wang, Xi, Li, Hui, Xu, Danke
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Sprache:eng
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Zusammenfassung:•An AgNP-based non-aggregation colorimetric aptasensor was first developed.•The colorimetric principle was based on AgNP-catalyzed reductive degradation of RhB.•This assay combined magnetic separation with nanocatalytic amplification.•The detection limit of thrombin was as low as 0.2nM with excellent specificity. In this paper, we developed a simple and rapid colorimetric assay for protein detection based on the reduction of dye molecules catalyzed by silver nanoparticles (AgNPs). Aptamer-modified magnetic particles and aptamer-functionalized AgNPs were employed as capture and detection probes, respectively. Introduction of thrombin as target protein could form a sandwich-type complex involving catalytically active AgNPs, whose catalytic activity was monitored on the catalytic reduction of rhodamine B (RhB) by sodium borohydride (NaBH4). The amount of immobilized AgNPs on the complex increased along with the increase of the thrombin concentration, thus the detection of thrombin was achieved via recording the decrease in absorbance corresponding to RhB. This method has adopted several advantages from the key factors involved, i.e., the sandwich binding of affinity aptamers contributed to the increased specificity; magnetic particles could result in rapid capture and separation processes; the conjugation of AgNPs would lead to a clear visual detection. It allows for the detection limit of thrombin down to picomolar level by the naked eye, with remarkable selectivity over other proteins. Moreover, it is possible to apply this method to the other targets with two binding sites as well.
ISSN:0003-2670
1873-4324
DOI:10.1016/j.aca.2013.11.011