A method for the enzymatic determination of atropine has been developed, which is based on a sequence of reactions involving (1) the hydrolysis of atropine to give tropine; (2) the enzymatic oxidation of tropine with NAD (catalysed by tropinone reductase); and (3) an indicator reaction, in which the NADH previously formed reduces the dye iodonitrotetrazolium chloride (INT) to a reddish species, the reaction catalysed by diaphorase. The method was first developed in solution (linear response range from 2.4âÃâ10(-6) M to 1.0âÃâ10(-4) M). It was then implemented in cellulose platforms to develop a rapid test where the determination is made by measuring the RGB coordinates of the platforms using a smartphone-based device. The device is based on the integrating sphere concept and contains a light source to avoid external illumination effects. The smartphone is controlled by an app that allows a calibration line to be generated and the atropine concentration to be quantified; moreover, since the app normalizes the CCD response of the smartphone, the results and calibrations obtained with different smartphones are similar and can be shared. Using the G coordinate, the results were shown to have a linear response with the concentration of atropine ranging from 1.2âÃâ10(-5) M to 3.0âÃâ10(-4) M with an RSD of 1.4% (nâ=â5). The method has been applied to the determination of atropine in baby food and buckwheat samples with good results.
Colorimetric enzymatic rapid test for the determination of atropine in baby food using a smartphone.
利用智能手机进行比色酶法快速检测婴儿食品中阿托品的含量
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作者:DomÃnguez M, Moraru D, Lasso S, Sanz-Vicente I, de Marcos S, Galbán J
| 期刊: | Analytical and Bioanalytical Chemistry | 影响因子: | 3.800 |
| 时间: | 2024 | 起止号: | 2024 Dec;416(30):7317-7323 |
| doi: | 10.1007/s00216-024-05401-x | 研究方向: | 免疫/内分泌 |
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