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Journal of Clinical Microbiology, 10 1995, 2665-2669, Vol 33, No. 10
C d'Oliveira, M van der Weide, MA Habela, P Jacquiet and F Jongejan
We report the detection of Theileria annulata, the causative agent of
tropical theileriosis, by PCR in blood samples obtained from carrier
cattle. The assay employs primers specific for the gene encoding the 30-
kDa major merozoite surface antigen of T. annulata. A 721-bp fragment was
amplified from blood samples taken monthly from calves experimentally
infected with one of four different stocks of T. annulata originating in
either Mauritania, Portugal, Spain, or Turkey. At the end of the
experiment, five animals carried the infection for 12 months and two
animals remained infected for 15 months. DNAs from six other Theileria
species, T. parva, T. mutans, T. sergenti, T. buffeli, T. velifera, and T.
taurotragi, were not amplified. Moreover, DNAs from four other
hemoparasites (Anaplasma centrale, Anaplasma marginale, Babesia bovis, and
Babesia bigemina) were also not amplified. As a control, primers derived
from the small subunit rRNA gene of Theileria spp. amplified a 1.1-kb DNA
fragment from all Theileria species examined but not from the other four
hemoparasites. As few as two to three parasites per microliter of infected
blood in a 50-microliters sample volume were detected by Southern or
microplate hybridization with a T. annulata-specific cDNA probe. In
addition, 92 field samples obtained from cattle in Spain were tested; 22%
were positive in blood smears, 40% were positive by immunofluorescent
antibody test, and 75% were positive for T. annulata by PCR. The method
provides a useful diagnostic tool for detecting T. annulata carrier cattle.
Copyright © 1995 by the American Society for Microbiology. All rights reserved.
Detection of Theileria annulata in blood samples of carrier cattle by PCR
Department of Parasitology and Tropical Veterinary Medicine, Faculty of Veterinary Medicine, Utrecht University, The Netherlands.
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