Simple Screening of Listeria monocytogenes Based on a Fluorescence Assay via a Laminated Lab-On-Paper Chip

Monitoring food safety is essential for protecting the health and safety of consumers. Conventional methods used are time consuming and laborious, requiring anywhere from three to seven days to obtain results. Thus, better monitoring methods are required. In this study, a laminated lab-on-paper chip...

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Main Authors: Kankanit Pisamayarom, Annop Suriyasomboon, Piyasak Chaumpluk
Format: Article
Language:English
Published: MDPI AG 2017-11-01
Series:Biosensors
Subjects:
Online Access:https://www.mdpi.com/2079-6374/7/4/56
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spelling doaj-d5972f7d61554fe9a3fe7fe21cefbf9b2020-11-24T21:24:57ZengMDPI AGBiosensors2079-63742017-11-01745610.3390/bios7040056bios7040056Simple Screening of Listeria monocytogenes Based on a Fluorescence Assay via a Laminated Lab-On-Paper ChipKankanit Pisamayarom0Annop Suriyasomboon1Piyasak Chaumpluk2Laboratory of Plant Transgenic Technology and Biosensor, Department of Botany, Faculty of Science, Chulalongkorn University, Bangkok 10330, ThailandDepartment of Animal Husbandry, Faculty of Veterinary Science, Chulalongkorn University, Bangkok 10330, ThailandLaboratory of Plant Transgenic Technology and Biosensor, Department of Botany, Faculty of Science, Chulalongkorn University, Bangkok 10330, ThailandMonitoring food safety is essential for protecting the health and safety of consumers. Conventional methods used are time consuming and laborious, requiring anywhere from three to seven days to obtain results. Thus, better monitoring methods are required. In this study, a laminated lab-on-paper chip was developed, and its use for the screening of ready-to-eat seafood was demonstrated. The assay on a chip was based on loop-mediated isothermal DNA amplification (LAMP) of the hly gene of Listeria monocytogenes and fluorescence signal detection via SYBR GoldTM. Overall assay processes were completed in 4.5 h., (including 3.5 h. incubation for the bacteria enrichment, direct DNA amplification with no DNA extraction, and signal detection), without relying on standard laboratory facilities. Only positive samples induced fluorescence signals on chip upon illumination with UV light (λ = 460). The method has a limit of detection of 100 copies of L. monocytogenes DNA per 50 g of sample. No cross-reactivity was observed in samples contaminated with other bacteria. On-site monitoring of the seafood products using this chip revealed that one of 30 products from low sanitation vendors (3.33%) were contaminated, and these agreed with the results of PCR. The results demonstrated a benefit of this chip assay for practical on-site monitoring.https://www.mdpi.com/2079-6374/7/4/56Lab-on-paper chipListeria monocytogenesDetectionLAMPhly genefrozen seafood
collection DOAJ
language English
format Article
sources DOAJ
author Kankanit Pisamayarom
Annop Suriyasomboon
Piyasak Chaumpluk
spellingShingle Kankanit Pisamayarom
Annop Suriyasomboon
Piyasak Chaumpluk
Simple Screening of Listeria monocytogenes Based on a Fluorescence Assay via a Laminated Lab-On-Paper Chip
Biosensors
Lab-on-paper chip
Listeria monocytogenes
Detection
LAMP
hly gene
frozen seafood
author_facet Kankanit Pisamayarom
Annop Suriyasomboon
Piyasak Chaumpluk
author_sort Kankanit Pisamayarom
title Simple Screening of Listeria monocytogenes Based on a Fluorescence Assay via a Laminated Lab-On-Paper Chip
title_short Simple Screening of Listeria monocytogenes Based on a Fluorescence Assay via a Laminated Lab-On-Paper Chip
title_full Simple Screening of Listeria monocytogenes Based on a Fluorescence Assay via a Laminated Lab-On-Paper Chip
title_fullStr Simple Screening of Listeria monocytogenes Based on a Fluorescence Assay via a Laminated Lab-On-Paper Chip
title_full_unstemmed Simple Screening of Listeria monocytogenes Based on a Fluorescence Assay via a Laminated Lab-On-Paper Chip
title_sort simple screening of listeria monocytogenes based on a fluorescence assay via a laminated lab-on-paper chip
publisher MDPI AG
series Biosensors
issn 2079-6374
publishDate 2017-11-01
description Monitoring food safety is essential for protecting the health and safety of consumers. Conventional methods used are time consuming and laborious, requiring anywhere from three to seven days to obtain results. Thus, better monitoring methods are required. In this study, a laminated lab-on-paper chip was developed, and its use for the screening of ready-to-eat seafood was demonstrated. The assay on a chip was based on loop-mediated isothermal DNA amplification (LAMP) of the hly gene of Listeria monocytogenes and fluorescence signal detection via SYBR GoldTM. Overall assay processes were completed in 4.5 h., (including 3.5 h. incubation for the bacteria enrichment, direct DNA amplification with no DNA extraction, and signal detection), without relying on standard laboratory facilities. Only positive samples induced fluorescence signals on chip upon illumination with UV light (λ = 460). The method has a limit of detection of 100 copies of L. monocytogenes DNA per 50 g of sample. No cross-reactivity was observed in samples contaminated with other bacteria. On-site monitoring of the seafood products using this chip revealed that one of 30 products from low sanitation vendors (3.33%) were contaminated, and these agreed with the results of PCR. The results demonstrated a benefit of this chip assay for practical on-site monitoring.
topic Lab-on-paper chip
Listeria monocytogenes
Detection
LAMP
hly gene
frozen seafood
url https://www.mdpi.com/2079-6374/7/4/56
work_keys_str_mv AT kankanitpisamayarom simplescreeningoflisteriamonocytogenesbasedonafluorescenceassayviaalaminatedlabonpaperchip
AT annopsuriyasomboon simplescreeningoflisteriamonocytogenesbasedonafluorescenceassayviaalaminatedlabonpaperchip
AT piyasakchaumpluk simplescreeningoflisteriamonocytogenesbasedonafluorescenceassayviaalaminatedlabonpaperchip
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