том 96 издание 29 страницы 12093-12101

Ultrasensitive Dual ELONA/SERS–RPA Multiplex Diagnosis of Antimicrobial Resistance

Тип публикацииJournal Article
Дата публикации2024-07-08
SCImago Q1
Tоп 10% SCImago
WOS Q1
БС1
SJR1.358
CiteScore11.6
Impact factor6.7
ISSN00032700, 15206882, 21542686
Краткое описание
Antimicrobial resistance (AMR) is a significant global health threat concern, necessitating healthcare practitioners to accurately prescribe the most effective antimicrobial agents with correct doses to combat resistant infections. This is necessary to improve the therapeutic outcomes for patients and prevent further increase in AMR. Consequently, there is an urgent need to implement rapid and sensitive clinical diagnostic methods to identify resistant pathogenic strains and monitor the efficacy of antimicrobials. In this study, we report a novel proof-of-concept magnetic scaffold-recombinase polymerase amplification (RPA) technique, coupled with an enzyme-linked oligonucleotide assay (ELONA) and surface-enhanced Raman scattering (SERS) detection, aimed at selectively amplifying and detecting the DNA signature of three resistant carbapenemase genes, VIM, KPC, and IMP. To achieve this, streptavidin-coated magnetic beads were functionalized with biotin-modified forward primers. RPA was conducted on the surface of the beads, resulting in an immobilized duplex amplicon featuring a single overhang tail specific to each gene. These tails were subsequently hybridized with recognition HRP probes conjugated to a complementary single-stranded oligonucleotide and detected colorimetrically. Additionally, they underwent hybridization with similar selective SERS probes and were measured using a handheld Raman spectrometer. The resulting quantification limits were at subpicomolar level for both assays, allowing the potential for early diagnosis. Moreover, we demonstrated the platform capability to conduct a multiplex RPA–SERS detection of the three genes in a single tube. Compared to similar approaches like PCR, RPA offers advantages of speed, affordability, and isothermal operation at 37 °C, eliminating the need for a thermal cycler. The whole assay was completed within <2 h. Therefore, this novel magnetic scaffold ELONA/SERS–RPA platform, for DNA detection, demonstrated excellent capability for the rapid monitoring of AMR in point-of-care applications, in terms of sensitivity, portability, and speed of analysis.
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ГОСТ |
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Hassanain W. A. et al. Ultrasensitive Dual ELONA/SERS–RPA Multiplex Diagnosis of Antimicrobial Resistance // Analytical Chemistry. 2024. Vol. 96. No. 29. pp. 12093-12101.
ГОСТ со всеми авторами (до 50) Скопировать
Hassanain W. A., Johnson C. L., Faulds K., Keegan N., Graham D. Ultrasensitive Dual ELONA/SERS–RPA Multiplex Diagnosis of Antimicrobial Resistance // Analytical Chemistry. 2024. Vol. 96. No. 29. pp. 12093-12101.
RIS |
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TY - JOUR
DO - 10.1021/acs.analchem.4c02165
UR - https://pubs.acs.org/doi/10.1021/acs.analchem.4c02165
TI - Ultrasensitive Dual ELONA/SERS–RPA Multiplex Diagnosis of Antimicrobial Resistance
T2 - Analytical Chemistry
AU - Hassanain, Waleed A.
AU - Johnson, C L
AU - Faulds, Karen
AU - Keegan, Neil
AU - Graham, Duncan
PY - 2024
DA - 2024/07/08
PB - American Chemical Society (ACS)
SP - 12093-12101
IS - 29
VL - 96
PMID - 38975860
SN - 0003-2700
SN - 1520-6882
SN - 2154-2686
ER -
BibTex |
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BibTex (до 50 авторов) Скопировать
@article{2024_Hassanain,
author = {Waleed A. Hassanain and C L Johnson and Karen Faulds and Neil Keegan and Duncan Graham},
title = {Ultrasensitive Dual ELONA/SERS–RPA Multiplex Diagnosis of Antimicrobial Resistance},
journal = {Analytical Chemistry},
year = {2024},
volume = {96},
publisher = {American Chemical Society (ACS)},
month = {jul},
url = {https://pubs.acs.org/doi/10.1021/acs.analchem.4c02165},
number = {29},
pages = {12093--12101},
doi = {10.1021/acs.analchem.4c02165}
}
MLA
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Hassanain, Waleed A., et al. “Ultrasensitive Dual ELONA/SERS–RPA Multiplex Diagnosis of Antimicrobial Resistance.” Analytical Chemistry, vol. 96, no. 29, Jul. 2024, pp. 12093-12101. https://pubs.acs.org/doi/10.1021/acs.analchem.4c02165.
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