2017
DOI: 10.1371/journal.pone.0169011
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Colorimetric tests for diagnosis of filarial infection and vector surveillance using non-instrumented nucleic acid loop-mediated isothermal amplification (NINA-LAMP)

Abstract: Accurate detection of filarial parasites in humans is essential for the implementation and evaluation of mass drug administration programs to control onchocerciasis and lymphatic filariasis. Determining the infection levels in vector populations is also important for assessing transmission, deciding when drug treatments may be terminated and for monitoring recrudescence. Immunological methods to detect infection in humans are available, however, cross-reactivity issues have been reported. Nucleic acid-based mo… Show more

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Cited by 92 publications
(98 citation statements)
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“…Furthermore, although the stranddisplacing polymerase has reverse transcriptase activity, a reverse transcriptase can be included to improve sensitivity within the reaction when detecting an RNA target (RT-LAMP), such as the SARS-CoV-2 RNA. LAMP assays have a variety of readouts due to the large amount of DNA generated, including fluorescence using an intercalating DNA dye, turbidity, or by a drop in the pH if the reaction is minimally buffered 1,3,4 . This change in pH, sufficient to cause a pH indicator dye to visibly change color, is the most applicable method for a point-of-care LAMP-based diagnostic.…”
Section: Introduction/backgroundmentioning
confidence: 99%
“…Furthermore, although the stranddisplacing polymerase has reverse transcriptase activity, a reverse transcriptase can be included to improve sensitivity within the reaction when detecting an RNA target (RT-LAMP), such as the SARS-CoV-2 RNA. LAMP assays have a variety of readouts due to the large amount of DNA generated, including fluorescence using an intercalating DNA dye, turbidity, or by a drop in the pH if the reaction is minimally buffered 1,3,4 . This change in pH, sufficient to cause a pH indicator dye to visibly change color, is the most applicable method for a point-of-care LAMP-based diagnostic.…”
Section: Introduction/backgroundmentioning
confidence: 99%
“…In PCR, thermal cycling is required to denature the template, anneal primers and extend the amplicon. LAMP employs Bst DNA polymerase, which provides both strand displacement and target ampli cation at a single temperature in a simple heat block or water bath at 60-65 °C [25] or other portable device with a stable heat source [57]. In addition, LAMP tests have been reported to be signi cantly cheaper than PCR [58].…”
Section: Discussionmentioning
confidence: 99%
“…LAMP assays can also be run in multiplex format and this could be exploited for the identification of several mosquito species in one reaction or for the combination of mosquito identification and detection of pathogens carried by them. LAMP assays for the detection of pathogens in insect vectors have already been described (Aonuma et al, 2010;Poole et al, 2017). Analyses of such multiplex LAMP assays can easily be achieved by lateral flow dipstick tests (Yongkiettrakul et al, 2017).…”
Section: Discussionmentioning
confidence: 99%