2017
DOI: 10.1039/c7ay01750b
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A one-step rapid screening test ofListeria monocytogenesin food samples using a real-time loop-mediated isothermal amplification turbidity assay

Abstract: A rapid and specific, hly-based, loop-mediated isothermal amplification (LAMP) was applied for the detection of Listeria monocytogenes in food and food products, using a real-time turbidimeter platform (LAMP-turbidity). The principle behind this method relies on an increase in a DNA yield, which correlates with the production of magnesium pyrophosphate, and the results can be determined via an amplification curve within 1 h. The specificity test revealed that L. monocytogenes (DMST 17303) was observed from 34.… Show more

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Cited by 25 publications
(15 citation statements)
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References 24 publications
(23 reference statements)
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“…The LAMP reaction is detected by measuring the fluorescent intensity of the indicated reagents (Fischbach et al, 2015 ) or the turbidity of the DNA polymerization by-products (magnesium pyrophosphate; Mori et al, 2001 ; Jayawardena et al, 2007 ). These methods are capable of obtaining real time signals, from which the amount of the DNA template can be quantified (Liu et al, 2017 ; Wachiralurpan et al, 2017b ). The visual detection of turbidity by the naked eye was achieved when a fluorescent dye such as SYBR green was added to the solution after the LAMP reaction (Mashooq et al, 2016 ).…”
Section: Introductionmentioning
confidence: 99%
“…The LAMP reaction is detected by measuring the fluorescent intensity of the indicated reagents (Fischbach et al, 2015 ) or the turbidity of the DNA polymerization by-products (magnesium pyrophosphate; Mori et al, 2001 ; Jayawardena et al, 2007 ). These methods are capable of obtaining real time signals, from which the amount of the DNA template can be quantified (Liu et al, 2017 ; Wachiralurpan et al, 2017b ). The visual detection of turbidity by the naked eye was achieved when a fluorescent dye such as SYBR green was added to the solution after the LAMP reaction (Mashooq et al, 2016 ).…”
Section: Introductionmentioning
confidence: 99%
“…To assess this hypothesis, we tested five different initial concentrations of L. monocytogenes DMST 17303 gDNA samples. Figure 4 shows the results: when injecting a LAMP mixture containing approximately 0.8 ng of L. monocytogenes gDNA, starting amplification led to a signal onset after 27 min It is worth noting that this clearly showcases an added advantage of the QCM-based assay: turbidity measurements at 650 nm showed a signal only after 46 min [ 21 ]. Switching to measuring on the QCM in situ hence improves sensitivity by decreasing the measuring time.…”
Section: Resultsmentioning
confidence: 99%
“…Modified QCM were placed in a custom-made PDMS cell for measurements. The temperature was kept at 60 °C by a thermostat (Thermo Haake ® DC30, Gebrüder HAAKE GmbH, Karlsruhe, Germany), which turned out the optimal temperature for LAMP amplification [ 21 ] when developing a colorimetric test for a different gene of L. monocytogenes . This cell was then connected to a custom-made oscillator circuit to operate the device.…”
Section: Methodsmentioning
confidence: 99%
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“…Traditional microbiological and biochemical assays for the detection of Listeria monocytogenes rely on preliminary culture, followed by biochemical and serological identification, taking at least 3 days. More recently, traditional methods are gradually being replaced by those that are more convenient and simple, such as immunological (Zhang, He, Liu, Peng, & Li, 2014), molecular biological (Wachiralurpan, 2017; Yan Wang, 2018), or electrochemical biosensor method techniques (Suh et al, 2018; Yang, Zhou, Zhu, & Xing, 2017). Among the many detection methods, the design of ECL biosensors, including solution‐state and solid‐state ECL systems has recently become an active research focus.…”
Section: Introductionmentioning
confidence: 99%