Amplification-Free Attomolar Detection of Short Nucleic Acids with Upconversion Luminescence: Eliminating Nonspecific Binding by Hybridization Complex Transfer - UTU Tutkimustietojärjestelmä

A1 Vertaisarvioitu alkuperäisartikkeli tieteellisessä lehdessä

Amplification-Free Attomolar Detection of Short Nucleic Acids with Upconversion Luminescence: Eliminating Nonspecific Binding by Hybridization Complex Transfer

Tekijät: Máčala, Jakub; Kuusinen, Saara; Lahtinen, Satu; Gorris, Hans H.; Skládal, Petr; Farka, Zdeněk; Soukka, Tero

Kustantaja: American Chemical Society (ACS)

Kustannuspaikka: WASHINGTON

Julkaisuvuosi: 2025

Journal: Analytical Chemistry

Tietokannassa oleva lehden nimi: Analytical Chemistry

Lehden akronyymi: ANAL CHEM

Vuosikerta: 97

Numero: 3

Aloitussivu: 1775

Lopetussivu: 1782

Sivujen määrä: 8

ISSN: 0003-2700

eISSN: 1520-6882

DOI: https://doi.org/10.1021/acs.analchem.4c05401

Verkko-osoite: https://doi.org/10.1021/acs.analchem.4c05401

Rinnakkaistallenteen osoite: https://research.utu.fi/converis/portal/detail/Publication/484550287

Tiivistelmä

The anti-Stokes emission of photon upconversion nanoparticles (UCNPs) facilitates their use as labels for ultrasensitive detection in biological samples as infrared excitation does not induce autofluorescence at visible wavelengths. The detection of extremely low-abundance analytes, however, remains challenging as it is impossible to completely avoid nonspecific binding of label conjugates. To overcome this limitation, we developed a novel hybridization complex transfer technique using UCNP labels to detect short nucleic acids directly without target amplification. The assay involves capturing the target-label complexes on an initial solid phase, then using releasing oligonucleotides to specifically elute only the target-UCNP complexes and recapturing them on another solid phase. The nonspecifically adsorbed labels remain on the first solid phase, enabling background-free, ultrasensitive detection. When magnetic microparticles were used as the first solid phase in a sample volume of 120 mu L, the assay achieved a limit of detection (LOD) of 310 aM, a 27-fold improvement over the reference assay without transfer. Moreover, the additional target-specific steps introduced in the complex transfer procedure improved the sequence specificity of the complex transfer assay compared with the reference assay. The suitability for clinical analysis was confirmed using spiked plasma samples, resulting in an LOD of 190 aM. By increasing the sample volume to 600 mu L and using magnetic preconcentration, the LOD was improved to 46 aM. These results highlight the importance of background elimination in achieving ultralow LODs for the analysis of low-abundance biomarkers.

Ladattava julkaisu

This is an electronic reprint of the original article.
This reprint may differ from the original in pagination and typographic detail. Please cite the original version.

máčala-et-al-2025-amplification-free-attomolar-detection-of-short-nucleic-acids-with-upconversion-luminescence.pdf

Julkaisussa olevat rahoitustiedot:
The work was supported by grant GA22-27580S from the Czech Science Foundation.