A novel snapback primer probe assay for the detection and discrimination of sympatric Haemonchus species using DNA melting analysis

Rudolf Pichler; Katja Silbermayr; Kathiravan Periasamy

doi:10.1016/j.vetpar.2017.02.012

A novel snapback primer probe assay for the detection and discrimination of sympatric Haemonchus species using DNA melting analysis

Vet Parasitol. 2017 Apr 15:237:94-103. doi: 10.1016/j.vetpar.2017.02.012. Epub 2017 Feb 20.

Authors

Rudolf Pichler¹, Katja Silbermayr², Kathiravan Periasamy³

Affiliations

¹ Animal Production and Health Laboratory, Joint FAO/IAEA Division of Nuclear Techniques in Food and Agriculture, International Atomic Energy Agency, Vienna, Austria. Electronic address: Rudolf.Pichler@iaea.org.
² Animal Production and Health Laboratory, Joint FAO/IAEA Division of Nuclear Techniques in Food and Agriculture, International Atomic Energy Agency, Vienna, Austria; Institute of Parasitology, Department of Pathobiology, University of Veterinary Medicine, Vienna, Austria. Electronic address: katja.silbermayr@gmail.com.
³ Animal Production and Health Laboratory, Joint FAO/IAEA Division of Nuclear Techniques in Food and Agriculture, International Atomic Energy Agency, Vienna, Austria. Electronic address: K.Periasamy@iaea.org.

PMID: 28242041
DOI: 10.1016/j.vetpar.2017.02.012

Abstract

Different sympatric species of Haemonchus parasites infecting ruminants and camels can be distinguished morphologically, but involves tedious microscopic examinations, measurements and several other limitations. Information on internal transcribed spacer-2 (ITS-2) sequence provides confirmatory differentiation of sympatric Haemonchus species. The present study introduces a novel, snapback primer probe based, real time PCR assay for the differentiation of three sympatric Haemonchus species, H. contortus (Hco), H. placei (Hpl) and H. longistipes (Hlo). The assay was designed to amplify a region of 130bp within the ITS-2 gene that included three diagnostic mutational sites capable of discriminating Hco, Hpl and Hlo. Following melt curve analysis, species-specific diagnostic melt peaks were obtained for Hco, Hpl and Hlo with a mean melting temperature of 56.6±0.3°C, 64.4±0.1°C and 54.4±0.1°C respectively. The test for analytical sensitivity revealed the ability of the assay to detect up to 5 copies per reaction. To evaluate the discriminating power of the assay, 174 samples from adult worms and 3rd stage larvae belonging to different Haemonchus species and various other nematode species including Cooperia curticei, Trichostrongylus axei, Trichostrongylus colubriformis, and Teladorsagia circumcincta were tested. Additionally, DNA extracted from 25 fecal egg samples was also tested and the specificity of the assay was verified by sequencing the ITS-2 gene of all the Haemonchus positive and non-Haemonchus samples. The assay worked accurately with 100% specificity in at least three real time PCR platforms. The assay is an effective alternative to the sequencing approach and is expected to be helpful for the screening of individual adult and larval Haemonchus parasites. However, caution needs to be applied while interpreting the results from fecal egg samples due to varying levels of sympatric co-infections from different Haemonchus species. The present study is the first report on the application of snapback primer probe methodology for the differentiation of nematode parasites.

Keywords: Haemonchus; Hairpin loop; Limit of detection; Melting curve analysis; Snapback primer probe; qPCR.

MeSH terms

Animals
Coinfection / veterinary
DNA Primers / genetics
DNA, Helminth / genetics
Feces / parasitology
Female
Haemonchiasis / parasitology
Haemonchiasis / veterinary*
Haemonchus / genetics
Haemonchus / isolation & purification*
Limit of Detection
Nematoda / genetics
Nematoda / isolation & purification*
Ovum
Species Specificity
Sympatry

Substances

DNA Primers
DNA, Helminth