Homogeneous quenching immunoassay for fumonisin B1 based on gold nanoparticles and an epitope-mimicking yellow fluorescent protein

Peltomaa, Riikka Johanna; Amaro Torres, Francisco; Carrasco, Sergio; Orellana Moraleda, Guillermo; Benito Peña, María Elena; Moreno Bondi, María Cruz

Homogeneous quenching immunoassay for fumonisin B1 based on gold nanoparticles and an epitope-mimicking yellow fluorescent protein

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Official URL

https://doi.org/10.1021/acsnano.8b06094

Publication date

2018

Authors

Peltomaa, Riikka Johanna

Amaro Torres, Francisco

Carrasco, Sergio

Orellana Moraleda, Guillermo

Benito Peña, María Elena

Moreno Bondi, María Cruz

Publisher

American Chemical Society

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URI

https://hdl.handle.net/20.500.14352/93316

Citation

Riikka Peltomaa, Francisco Amaro-Torres, Sergio Carrasco, Guillermo Orellana, Elena Benito-Peña, and María C. Moreno-Bondi ACS Nano 2018 12 (11), 11333-11342 DOI: 10.1021/acsnano.8b06094

Abstract

Homogeneous immunoassays represent an attractive alternative to traditional heterogeneous assays due to their simplicity, sensitivity, and speed. On the basis of a previously identified epitope-mimicking peptide, or mimotope, we developed a homogeneous fluorescence quenching immunoassay based on gold nanoparticles (AuNPs) and a recombinant epitope-mimicking fusion protein for the detection of mycotoxin fumonisin B1 (FB1). The fumonisin mimotope was cloned as a fusion protein with a yellow fluorescent protein that could be used directly as the tracer for FB1 detection without the need of labeling or a secondary antibody. Furthermore, owing to the fluorescence quenching ability of AuNPs, a homogeneous immunoassay could be performed in a single step without washing steps to separate the unbound tracer. The homogeneous quenching assay showed negligible matrix effects in 5% wheat extract and high sensitivity for FB1 detection, with a dynamic range from 7.3 to 22.6 ng/mL, a detection limit of 1.1 ng/mL, and IC50 value of 12.9 ng/mL, which was significantly lower than the IC50 value of the previously reported assay using the synthetic counterpart of the same mimotope in a microarray format. The homogeneous assay was demonstrated to be specific for fumonisins B1 and B2, as no significant cross-reactivity with other mycotoxins was observed, and acceptable recoveries (86% for FB1 2000 μg/kg and 103% for FB1 4000 μg/kg), with relative standard deviation less than 6.5%, were reported from spiked wheat samples, proving that the method could provide a valuable tool for simple analysis of mycotoxin-contaminated food samples.