Isolation and detection of Fasciola hepatica DNA in Lymnaea viatrix from formalin-fixed and paraffin-embedded tissues through multiplex-PCR.

Vet Parasitol

Laboratório de Helmintoses Intestinais-Centro de Pesquisas René Rachou da Fundação Oswaldo Cruz, Av. Augusto de Lima 1715, Belo Horizonte, MG, Brazil.

Published: April 2008

AI Article Synopsis

  • The study aimed to detect Fasciola hepatica infections in Lymnaea viatrix using histological analysis, but differentiating between trematode forms can be challenging due to their similarities and other helminth interference.
  • A new method for extracting DNA from formalin-fixed, paraffin-embedded tissues involved deparaffinization and proteinase K digestion, followed by multiplex-PCR for amplification.
  • The results demonstrated that this technique was highly sensitive and specific, allowing for the detection of F. hepatica DNA even in samples where larval stages weren't visible, which can aid in fascioliasis epidemiology research.

Article Abstract

Detection of Fasciola hepatica infection in Lymnaea viatrix through analysis of histological cuts is based upon morphological characters of the parasite during the intra-mollusk phase of parasitism. At this stage, trematode forms are very similar and, thus, very difficult to differentiate. Specific detection may also be impaired by the presence of other helminthes in the mollusk. Histological samples are usually fixed in formalin, embedded in paraffin, sectioned and HE stained. In the current study, a method for the extraction of DNA from formalin-fixed, paraffin-embedded tissues was standardized by means of deparaffinizing with xylol and digesting with proteinase K. Extracted DNA was amplified in a multiplex-PCR, by using simultaneous primers in a single reaction under high stringency conditions. Results showed specific amplification of DNA from the trematode and the snails. The technique was sensitive enough to detect F. hepatica infections in L. viatrix, in histological sections in which the presence of larval stages could not be observed through brightfield microscopy. The profiles generated were: stair bands referring to F. hepatica DNAmt amplification; a band of 1200 bp referring to L. viatrix ITS and another of 1300 bp referring to F. hepatica ITS and other trematodes. Multiplex-PCR has shown to be a fast, safe, highly sensitive and specific method, which is able to amplify DNA from fixed tissues, despite a low DNA quantity and its degradation caused by fixation processes. Such methodology may be useful in studies on fascioliasis epidemiology, enabling the use of material from histological collections.

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http://dx.doi.org/10.1016/j.vetpar.2007.12.019DOI Listing

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