2024
Comparison of single and double pulse laser-induced breakdown spectroscopy for the detection of biomolecules tagged with photon-upconversion nanoparticles
FARKA, Zdeněk, Karolína VYTISKOVÁ, Ekaterina MAKHNEVA, Eva ZIKMUNDOVÁ, Daniel HOLUB et. al.Základní údaje
Originální název
Comparison of single and double pulse laser-induced breakdown spectroscopy for the detection of biomolecules tagged with photon-upconversion nanoparticles
Autoři
FARKA, Zdeněk (203 Česká republika, garant, domácí), Karolína VYTISKOVÁ (203 Česká republika), Ekaterina MAKHNEVA (643 Rusko, domácí), Eva ZIKMUNDOVÁ (203 Česká republika), Daniel HOLUB, Jakub BUDAY, David PROCHAZKA, Karel NOVOTNÝ (203 Česká republika, domácí), Petr SKLÁDAL (203 Česká republika, domácí), Pavel POŘÍZKA (203 Česká republika) a Jozef KAISER (203 Česká republika)
Vydání
Analytica Chimica Acta, Elsevier, 2024, 0003-2670
Další údaje
Jazyk
angličtina
Typ výsledku
Článek v odborném periodiku
Obor
10406 Analytical chemistry
Stát vydavatele
Nizozemské království
Utajení
není předmětem státního či obchodního tajemství
Odkazy
Impakt faktor
Impact factor: 6.200 v roce 2022
Organizační jednotka
Přírodovědecká fakulta
UT WoS
001209691500001
Klíčová slova anglicky
Laser-induced breakdown spectroscopy; Double pulse; Tag-LIBS; Photon-upconversion nanoparticle; Immunoassay; Human serum albumin
Štítky
Příznaky
Mezinárodní význam, Recenzováno
Změněno: 10. 5. 2024 12:47, Mgr. Marie Šípková, DiS.
Anotace
V originále
Laser-induced breakdown spectroscopy (LIBS) is a well-recognized analytical technique used for elemental analysis. This method is gaining considerable attention also in biological applications thanks to its ability for spatial mapping and elemental imaging. The implementation of LIBS in the biomedical field is based on the detection of metals or other elements that either naturally occur in the samples or are present artificially. The artificial implementation of nanoparticle labels (Tag-LIBS) enables the use of LIBS as a readout technique for immunochemical assays. However, one of the biggest challenges for LIBS to meet immunoassay readout standards is its sensitivity. This paper focuses on the improvement of LIBS sensitivity for the readout of nanoparticle-based immunoassays. First, the LIBS setup was optimized on photon-upconversion nanoparticle (UCNP) droplets deposited on the microtiter plate wells. Two collection optics systems were compared, with single pulse (SP) and collinear double pulse (DP) LIBS arrangements. By deploying the second laser pulse, the sensitivity was improved up to 30 times. The optimized SP and DP setups were then employed for the indirect detection of human serum albumin based on immunoassay with UCNP-based labels. Compared to our previous LIBS study, the detection limit was enhanced by two orders of magnitude, from 10 ng mL−1 to 0.29 ng mL−1. In addition, two other immunochemical methods were used for reference, based on the readout of upconversion luminescence of UCNPs and absorbance measurement with enzyme labels. Finally, the selectivity of the assay was tested and the practical potential of Tag-LIBS was demonstrated by the successful analysis of urine samples. In this work, we improved the sensitivity of the Tag-LIBS method by combining new labels based on UCNPs with the improved collection optics and collinear DP configuration. In the instrumental setup optimization, the DP LIBS showed better sensitivity and signal-to-noise ratio than SP. The optimizations allowed the LIBS readout to surpass the sensitivity of enzyme immunoassay, approaching the qualities of upconversion luminescence readout, which is nowadays a state-of-the-art readout technique.
Návaznosti
| EF18_053/0016952, projekt VaV |
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| GA22-27580S, projekt VaV |
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