Detection of Babesia equi (Laveran, 1901) by nested polymerase chain reaction

We describe a nested polymerase chain reaction (PCR) for the detection of Babesia equi in equine infected erythrocytes using oligonucleotides designed on the published sequence of a B. equi merozoite antigen gene ( ema-1). A 102 bp DNA fragment is specifically amplified from B. equi but not from Bab...

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Bibliographic Details
Published in:Veterinary parasitology 2001-10, Vol.101 (1), p.9-21
Main Authors: Nicolaiewsky, T.B, Richter, M.F, Lunge, V.R, Cunha, C.W, Delagostin, O, Ikuta, N, Fonseca, A.S, da Silva, S.S, Ozaki, L.S
Format: Article
Language:English
Subjects:
Amino Acid Sequence
Animals
Antigens, Protozoan
Babesia - genetics
Babesia - isolation & purification
Babesia equi
Babesiosis - diagnosis
Babesiosis - veterinary
Base Sequence
Chronic Disease
Detection method
DNA sequence analysis
DNA, Protozoan - analysis
ema1 gene
Equine erythrocytes
Erythrocytes - parasitology
Gene Amplification
Horse Diseases - diagnosis
Horses
Membrane Proteins - genetics
Molecular Sequence Data
Molecular Weight
Nested polymerase chain reaction
PCR
Polymerase Chain Reaction - veterinary
Polymorphism, Restriction Fragment Length
Protozoan Proteins - genetics
Restriction Mapping - veterinary
RFLP
Sensitivity and Specificity
Sequence Analysis, DNA - veterinary
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Summary:We describe a nested polymerase chain reaction (PCR) for the detection of Babesia equi in equine infected erythrocytes using oligonucleotides designed on the published sequence of a B. equi merozoite antigen gene ( ema-1). A 102 bp DNA fragment is specifically amplified from B. equi but not from Babesia caballi, Babesia bovis or Babesia bigemina DNA. In a mock infection we were able to detect down to six infected cells in 10 8 equine erythrocytes or to detect the parasite in blood with an equivalent parasitemia of 0.000006%. Furthermore, gene polymorphism was found by performing a PCR-RFLP (PCR combined with restriction fragment length polymorphism) on both the 102 bp and the entire ema-1 gene DNA amplified from two B. equi isolates, Florida (USA) and Pelotas (Southern Brazil) isolates. The polymorphism was confirmed by sequencing the entire ema-1 gene from the B. equi isolate Pelotas. Our results demonstrate that the ema-1 based nested PCR is a valuable technique for routine detection of B. equi in chronically infected horses. It may be used for epidemiological and phylogenetic studies of the parasite as well as monitoring B. equi infected horses in chemotherapeutic trials.
ISSN:0304-4017
1873-2550
DOI:10.1016/S0304-4017(01)00471-X