Rapid detection of Galba truncatula in water sources on pasture-land using loop-mediated isothermal amplification for control of trematode infections

Chelsea N Davis; Fiona Tyson; David Cutress; Emma Davies; Dewi Llyr Jones; Peter M Brophy; Alex Prescott; Michael T Rose; Manod Williams; Hefin Wyn Williams; Rhys Aled Jones

doi:10.1186/s13071-020-04371-0

Rapid detection of Galba truncatula in water sources on pasture-land using loop-mediated isothermal amplification for control of trematode infections

Parasit Vectors. 2020 Sep 30;13(1):496. doi: 10.1186/s13071-020-04371-0.

Authors

Affiliations

¹ Institute of Biological, Environmental and Rural Sciences, Aberystwyth University, Aberystwyth, UK.
² Coleg Cambria, Llysfasi, Ruthin Road, Ruthin, Denbighshire, UK.
³ Tasmanian Institute of Agriculture, University of Tasmania, Sandy Bay, TAS, Australia.
⁴ Institute of Biological, Environmental and Rural Sciences, Aberystwyth University, Aberystwyth, UK. raj22@aber.ac.uk.

Abstract

Background: Fascioliasis caused by the trematodes Fasciola hepatica and F. gigantica, is a global neglected zoonotic disease estimated to cost the livestock industry over €2.5 billion annually. Farm management measures and sustainable use of anthelmintics can, in principle, effectively control trematode infection in livestock and reduce the rate of developing anthelmintic resistance. Previously, we designed an environmental DNA (eDNA) assay to identify a common trematode intermediate host, the freshwater snail Galba truncatula, in water sources to measure specific trematode infection risk areas on pasture-land. To improve this procedure, we now report a loop-mediated isothermal amplification (LAMP) assay to identify G. truncatula eDNA.

Methods: A LAMP assay was designed and optimised (e.g. temperature, time duration and primer concentration) to identify G. truncatula DNA. The ability of the LAMP assay to target G. truncatula DNA was identified, and LAMP assay limit of detection was investigated in comparison to conventional PCR. In the field, 48 water samples were collected from stream, ditch and water pool habitats in four locations at two Aberystwyth University farms over a seven week period to investigate the applicability of the LAMP assay for use on eDNA samples, in comparison to conventional PCR.

Results: The LAMP assay delivered detectable results in 30 min at 63 °C. The assay discriminated between G. truncatula DNA and non-target DNA, presenting a level of DNA detection comparable to conventional PCR. No significant difference was found between the ability of the LAMP and PCR assay to identify G. truncatula eDNA in water samples. Kappa coefficient analysis revealed a moderate level of agreement between LAMP and PCR assays.

Conclusions: This study demonstrated that the LAMP assay can detect G. truncatula eDNA in a simple and rapid manner. The LAMP assay may become a valuable tool to determine optimum pasture management for trematode parasite control.

Keywords: Calicophoron daubneyi; Environmental DNA; Farm management; Fasciola hepatica; Fluke; Galba truncatula; Loop-mediated isothermal amplification; Trematode.

Publication types

Evaluation Study

MeSH terms

Animals
DNA, Environmental / genetics*
Ecosystem
Fasciola hepatica / genetics
Fasciola hepatica / physiology
Fascioliasis / parasitology
Fascioliasis / prevention & control
Fascioliasis / transmission
Fascioliasis / veterinary*
Fresh Water / parasitology*
Livestock / parasitology
Molecular Diagnostic Techniques / methods*
Nucleic Acid Amplification Techniques / methods*
Snails / genetics*
Snails / parasitology

Substances

DNA, Environmental

Supplementary concepts

LAMP assay