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Fig. 2 | Parasites & Vectors

Fig. 2

From: Serological and molecular diagnostic surveys combined with examining hematological profiles suggests increased levels of infection and hematological response of cattle to babesiosis infections compared to native buffaloes in Egypt

Fig. 2

Agarose gel electrophoresis separation of PCR products of the B. bovis PCR detection methods: Two replica comparisons of the relative sensitivity of the nested PCR and semi-nested PCR methods for the detection of B. bovis DNA using genomic DNA extracted from in vitro cultured parasites from the B. bovis T3B strain (A) and from experimentally infected bovine (Mo7 strain) (B). a. The two PCR methods used were based on the B. bovis rap-1 (U) and on the rra (L) genes. The amounts of DNA amplified were 5 ng (lanes 1,8); 5×10−1 ng (lanes 2,9); 5×10−2 ng (lanes 3,10); 5×10−3 ng (lanes 4,11); 5×10−4 ng (lanes 5,12); 5×10−5 ng (lanes 6,13); 5×10−6 ng (lanes 7,14). Lane 15 represents PCR amplifications without adding DNA, and lane 16 represents PCR amplifications using plasmid pCR™ 2.1-TOPO B. bovis-rap-1 (U) or plasmid pCR™ 2.1-TOPO B. bovis-rra-1 (L) as positive controls. b. The two PCR methods used were based on the B. bovis rap-1 (U) and on the rra (L) genes. The amounts of DNA amplified were 5 ng (lanes 1,10); 5×10−1 ng (lanes 2,11); 5×10−2 ng (lanes 3,12); 5×10−3 ng (lanes 4,13); 5×10−4 ng (lanes 5,14); 5×10−5 ng (lanes 6,15); 5×10−6 ng (lanes 7,16); 5×10−7 ng (lanes 8,17); and 5×10−8 ng (lanes 9,18). Lane 19 represents PCR amplification without adding DNA, and lane 20 represents PCR amplifications using plasmid pCR™ 2.1-TOPO B. bovis-rap-1 (U) or plasmid pCR™ 2.1-TOPO B. bovis-rra-1 (L) as positive controls. Molecular size ladder in base pair (bp), 100 bp DNA ladder (lane m). The amplicons of interest are indicated at the left

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Parasites & Vectors

ISSN: 1756-3305

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