Multititration: The New Method for Implementing Ultrasensitive and Quantitative Multiplexed In-Field Immunoassays Despite Cross-Reactivity?

Fanny Mousseau; Cécile Féraudet Tarisse; Stéphanie Simon; Thierry Gacoin; Antigoni Alexandrou; Cédric Ismael Bouzigues

doi:10.1021/acs.analchem.3c01846

Multititration: The New Method for Implementing Ultrasensitive and Quantitative Multiplexed In-Field Immunoassays Despite Cross-Reactivity?

Anal Chem. 2023 Sep 12;95(36):13509-13518. doi: 10.1021/acs.analchem.3c01846. Epub 2023 Aug 28.

Authors

Fanny Mousseau¹, Cécile Féraudet Tarisse², Stéphanie Simon², Thierry Gacoin³, Antigoni Alexandrou¹, Cédric Ismael Bouzigues¹

Affiliations

¹ Laboratoire d'Optique et Biosciences, Ecole Polytechnique, Institut Polytechnique de Paris, CNRS, INSERM, Route de Saclay, 91128 Palaiseau, France.
² Département Médicaments et Technologies pour la Santé (DMTS), Université Paris-Saclay, CEA, INRAE, 91191 Gif-sur-Yvette, France.
³ Laboratoire de Physique de la Matière Condensée, Ecole Polytechnique, Institut Polytechnique de Paris, CNRS, Route de Saclay, 91128 Palaiseau, France.

PMID: 37639578
DOI: 10.1021/acs.analchem.3c01846

Abstract

The accurate in-field titration of multiple pathogens is essential to efficiently describe and monitor environmental or biological contamination, isolate, act, and treat adequately. This underscores the requirement of portable, fast, quantitative, and multiplexed detection technologies, which, however, have not been properly developed so far, notably because it has been hindered by the phenomenon of cross-reactivity. In this work, we proposed a new analytical method based on the imaging through a portable device of lanthanide-based nanoparticles (YVO₄:Eu) for spatially multiplexed detection, relying on a multiparameter analysis, i.e., a simultaneous analysis of all of the luminescence signals through the comparison to a calibration surface built in the presence of multiple analytes of interest. We then demonstrated the possibility to simultaneously quantify by multiplexed lateral flow assay (xLFA) the three enterotoxins SEG, SEH, and SEI in unknown mixtures, over two concentration decades (from a dozen of pg·mL^-1 to few ng·mL^-1). Assays were performed in less than an hour (25 min of strip migration followed by 30 min of drying at room temperature), the time during which the presence of the operator was not required for more than 5 min, in order to dip the strip and have it imaged by the reader. The concepts of nominal concentration recovery, coefficient of variation (CV), limit of blank (LOB), and limit of detection (LOD) were discussed in detail in the context of multiplexed assays. With our new definitions, quantitative results demonstrated a high recovery of the nominal concentrations (115%), reliability (CV = 20%), and sensitivity (LOBs of 3, 27, and 6 pg·mL^-1 for SEG, SEH, and SEI respectively, and LODs of 6, 48, and 11 pg·mL^-1 for SEG, SEH, and SEI, respectively). Based on this method, we observed an increase in sensitivity of 100 compared to the other multiplexed LFA labeled with gold particles and we approached the sensitivity of the simplex enzyme-linked immunosorbent assay (ELISA) performed with the same capture and detection antibodies. To conclude, our results, which are applicable to virtually any kind of multiplexed test, pave the way to the next generation of in-field analytical immunoassays by providing fast, quantitative, and highly sensitive multiplexed detection of biomarkers or pathogens.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Antibodies*
Biological Assay*
Calibration
Cross Reactions
Reproducibility of Results

Substances

Antibodies