| Literature DB >> 26414906 |
Fabiano Antonio Cadioli1, Otavio Luiz Fidelis Junior2, Paulo Henrique Sampaio2, Giuliana Nascimento dos Santos3, Marcos Rogério André2, Kayo José Garcia de Almeida Castilho3, Rosangela Zacarias Machado2.
Abstract
Trypanosoma vivax affects cattle herds in Africa and Americas and has been spreading rapidly in Brazil, through introduction of animals with subclinical infections and without apparent parasitemia, which makes its diagnosis challenging. PCR and LAMP are effective in detecting the presence of T. vivax DNA in situations of low parasitemia. LAMP is simpler and faster technique than PCR, and can be performed in the field, with limited resources. In this study, the capacities of conventional PCR and LAMP for detecting T. vivax in bovine blood samples classified as aparasitemic were evaluated. The capacity of conventional PCR (56.25%) for detecting positive samples was lower than that of LAMP (93.73%). This may influence the choice of screening tests for cattle herds infected with T. vivax.Entities:
Keywords: ELISA; Loop-mediated isothermal amplification; Polymerase chain reaction; Trypanosomiasis
Mesh:
Year: 2015 PMID: 26414906 DOI: 10.1016/j.vetpar.2015.09.001
Source DB: PubMed Journal: Vet Parasitol ISSN: 0304-4017 Impact factor: 2.738