Department of Chemistry, University of Turin, Via Giuria, 5, I-10125, Turin, Italy.
Department of General and Inorganic Chemistry, Chemistry Institute, Saratov State University, Astrakhanskaya 83, 410012, Saratov, Russia.
Mikrochim Acta. 2018 Jan 10;185(2):94. doi: 10.1007/s00604-017-2642-0.
A lateral flow immunoassay (LFIA) was developed for the determination of fumonisin mycotoxins. The fluorescence of CdSe/ZnS quantum dots (QDs), observed at excitation/emission wavelengths of 365/525 nm, is suppressed by the addition of silver nanoparticles (SNPs) or gold nanoparticles (GNPs) because SNPs overlap the excitation bands of the QDs, and GNPs overlap the emission bands. The fluorescence of the QDs is recovered upon addition of fumonisins, allowing for the sensitive detection in "positive mode" of the target mycotoxin by monitoring the changes of the QDs fluorescence intensity. The SNPs are found to be the most effective quenchers, while the use of GNPs allows for an efficient recovery of fluorescence and can be employed in the LFIA. The method was successfully applied to the fluorometric determination of fumonisins in spiked maize flour samples. The visual detection limit is at the ng·mL level. This is four times lower compared to the colorimetric LFIA based on the use of the conventional gold NPs. Graphical abstract Schematic of the fluorescence quenching lateral flow immunoassay that uses fluorescent quantum dots (QD) and metal nanoparticles (NP) as the quencher: the binding of NP-labelled antibody to the antigen (purple triangle) modulates QD luminescence at the Test line, allowing for 'positive mode' detection of fumonisins. The NP accumulation at Control line assures validity of the test.
侧向流动免疫分析(LFIA)用于测定伏马菌素真菌毒素。CdSe/ZnS 量子点(QDs)的荧光在 365/525nm 的激发/发射波长下被观察到,由于 SNPs 重叠了 QDs 的激发带,而 GNPs 重叠了发射带,因此加入银纳米粒子(SNPs)或金纳米粒子(GNPs)会抑制其荧光。加入伏马菌素后,QDs 的荧光会恢复,从而允许通过监测 QDs 荧光强度的变化,以“正模式”灵敏地检测目标真菌毒素。发现 SNPs 是最有效的猝灭剂,而使用 GNPs 可以有效地恢复荧光,并可用于 LFIA。该方法成功应用于玉米粉样品中添加伏马菌素的荧光测定。目视检测限为 ng·mL 水平。与基于常规金 NPs 的比色 LFIA 相比,这降低了四倍。
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