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Retroreflection-based sandwich type affinity sensing of isothermal gene amplification products for foodborne pathogen detection
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dc.contributor.authorLee, Danbi-
dc.contributor.authorKim, Eunsuk-
dc.contributor.authorLee, Kyung Won-
dc.contributor.authorKim, Ka Ram-
dc.contributor.authorChun, Hyeong Jin-
dc.contributor.authorYoon, Hyunjin-
dc.contributor.authorYoon, Hyun C.-
dc.date.issued2022-02-07-
dc.identifier.urihttps://dspace.ajou.ac.kr/dev/handle/2018.oak/32512-
dc.description.abstractLoop-mediated isothermal amplification (LAMP) is an outstanding method for molecular diagnostics, as the rapid, specific, and sensitive amplification of target genes is possible. However, it is necessary to measure fluorescence in the quantitative analysis of LAMP products, so a sophisticated optical setup is required. This study tried to develop a novel sensing method that can quantify target analytes with simple equipment, such as nonspectroscopic white light and a CMOS camera. To achieve this, a retroreflective Janus particle (RJP) as a probe and specially designed loop primers, fluorescein isothiocyanate (FITC)- and biotin-modified loop primers, were introduced into the LAMP system. By performing LAMP in the presence of designed primers, double-stranded amplicons possessing FITC and biotin labels at each end are generated in proportion to the quantity of the target pathogen. Using the anti-FITC antibody-modified sensing surface and streptavidin-conjugated RJP probes, the amplicons can be captured in sandwich-configuration and detected under nonspectroscopic conditions composed of white light and a camera. To confirm the feasibility of the sensing system, the invA gene of Salmonella was selected as the target. It was possible to quantitatively analyze the Salmonella concentration from 0 to 106 colony-forming units, sufficiently covering the required detection range. In addition, quantitative analyses of pathogens in contaminated food sources, including milk and chicken meat, were successfully conducted with a limit of detection of 10 CFU. This journal is-
dc.description.sponsorshipThis work was supported by the Creative Materials Discovery Program (NRF-2019M3D1A1078943) and research grants (NRF-2019R1A6A1A11051471 and NRF-2021R1A2C3004180) funded by the National Research Foundation of Korea. H. C. Y also acknowledges the support from the Technology Innovation Program (20004103) by MOTIE, Korea.-
dc.language.isoeng-
dc.publisherRoyal Society of Chemistry-
dc.subject.meshAmplicons-
dc.subject.meshAmplification products-
dc.subject.meshFluorescein isothiocyanate-
dc.subject.meshGene amplification-
dc.subject.meshJanus particles-
dc.subject.meshLoop mediated isothermal amplifications-
dc.subject.meshLoop-mediated isothermal amplifications-
dc.subject.meshRetro reflection-
dc.subject.meshSandwich types-
dc.subject.meshWhite light-
dc.subject.meshAnimals-
dc.subject.meshDNA Primers-
dc.subject.meshGene Amplification-
dc.subject.meshMilk-
dc.subject.meshNucleic Acid Amplification Techniques-
dc.subject.meshSalmonella-
dc.subject.meshSensitivity and Specificity-
dc.titleRetroreflection-based sandwich type affinity sensing of isothermal gene amplification products for foodborne pathogen detection-
dc.typeArticle-
dc.citation.endPage460-
dc.citation.startPage450-
dc.citation.titleAnalyst-
dc.citation.volume147-
dc.identifier.bibliographicCitationAnalyst, Vol.147, pp.450-460-
dc.identifier.doi10.1039/d1an01543e-
dc.identifier.pmid34985468-
dc.identifier.scopusid2-s2.0-85123968946-
dc.identifier.urlhttp://pubs.rsc.org/en/journals/journal/an-
dc.description.isoafalse-
dc.subject.subareaAnalytical Chemistry-
dc.subject.subareaBiochemistry-
dc.subject.subareaEnvironmental Chemistry-
dc.subject.subareaSpectroscopy-
dc.subject.subareaElectrochemistry-
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