An immunoblotting diagnostic assay for heartwater based on the immunodominant 32-kilodalton protein of Cowdria ruminantium detects false positives in field sera

Mahan, Suman M.; Tebele, N; Mukwedeya, D; Semu, S. M.; Nyathi, C.B.; Wassink, L.A.; Kelly, Patrick J.; Peter, Trevor; Barbet, Anthony F.

doi:10.1128/jcm.31.10.2729-2737.1993

Cited by 61 publications

(51 citation statements)

References 22 publications

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“…Furthermore, xenodiagnosis in mice has recently been shown to have low sensitivity and is unreliable for the detection of infection (38). More-expedient DNA probe and PCR assays based on the pCS20 and MAP 1 DNA sequences of C. ruminantium have been developed recently and have been used to detect infections in ticks and animals (1,31,37,38,42,43,52,60,62). PCR assays, which have greater sensitivity than DNA probe assays (52), may be useful tests for laboratory and field epidemiological investigations which are needed for improved understanding of heartwater epidemiology and the impact of new control measures (49).…”

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confidence: 99%

Detection of the Agent of Heartwater, Cowdria ruminantium , in Amblyomma Ticks by PCR: Validation and Application of the Assay to Field Ticks

Peter¹,

Barbet

Alleman

et al. 2000

J Clin Microbiol

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We have previously reported that the pCS20 PCR detection assay forCowdria ruminantium, the causative agent of heartwater disease of ruminants, is more sensitive than xenodiagnosis and the pCS20 DNA probe for the detection of infection in the vectorAmblyomma ticks. Here, we further assessed the reliability of the PCR assay and applied it to field ticks. The assay detected DNA of 37 isolates of C. ruminantium originating from sites throughout the distribution of heartwater and had a specificity of 98% when infected ticks were processed concurrently with uninfected ticks. The assay did not detect DNA of Ehrlichia chaffeensis, which is closely related to C. ruminantium. PCR sensitivity varied with tick infection intensity and was high (97 to 88%) with ticks bearing 107 to 104 organisms but dropped to 61 and 28%, respectively, with ticks bearing 103 and 102 organisms. The assay also detected C. ruminantium in collections of Amblyomma hebraeum andAmblyomma variegatum field ticks from 17 heartwater-endemic sites in four southern African countries. Attempts at tick transmission of infection to small ruminants failed with four of these collections. The pCS20 PCR assay is presently the most characterized and reliable test for C. ruminantium in ticks and thus is highly useful for field and laboratory epidemiological investigations of heartwater.

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confidence: 99%

Detection of the Agent of Heartwater, Cowdria ruminantium , in Amblyomma Ticks by PCR: Validation and Application of the Assay to Field Ticks

Peter¹,

Barbet

Alleman

et al. 2000

J Clin Microbiol

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“…For example, on the Caribbean islands of St. Kitts and Nevis, heartwater has never been diagnosed, but PME has been detected in A. variegatum , which may be the cause of false positives. As further demonstrated here, false‐positive reactions for E. rumanintium on the MAP‐IB ELISA in experimentally inoculated PME‐positive goats indicate that serology appears to be of limited use for diagnosing either heartwater or PME, in HW endemic and non‐endemic areas where PME may be circulating (Mahan et al., ; Simbi et al., ; Kelly et al., ). This underscores the need for a highly sensitive, rapid and specific assay that can differentiate between E. ruminantium and PME.…”

Section: Discussionmentioning

confidence: 70%

Development of a Quantitative PCR Assay for Differentiating the Agent of Heartwater Disease, Ehrlichia ruminantium , from the Panola Mountain Ehrlichia

Sayler

Loftis

Mahan

et al. 2015

Transbound Emerg Dis

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Panola Mountain Ehrlichia (PME) is an emerging Ehrlichia sp. reported in ten US states. Based on the sequence homology of all known genes, PME is closely related to Ehrlichia ruminantium (ER), the causative agent of heartwater. Heartwater is an economically important tick-borne disease of cattle, sheep and goats responsible for stock losses in sub-Saharan Africa. Unfortunately, ER was imported to the Caribbean islands in the 19th century, and the presence of this foreign animal disease in the Caribbean poses a threat to the US mainland. If introduced, a heartwater outbreak would cause massive losses of naïve livestock. The serologic assay of choice to diagnose heartwater is cross-reactive with Ehrlichia spp., including PME, as we demonstrate here, which would confound disease surveillance in the event of a heartwater outbreak. The purpose of this study was to develop a diagnostic assay capable of rapidly distinguishing between these pathogens. Using synthetic MAP-1B peptides for ER and PME, we tested the cross-reactivity of this assay using sera from infected livestock. The MAP-1B ELISA cannot distinguish between animals infected with PME and ER. Therefore, a dual-plex Taqman qPCR assay targeting the groEL gene of PME and ER was developed and validated. Primers were designed that are conserved among all known strains of ER, allowing for the amplification of strains from the Caribbean and Africa. The assay is highly sensitive (10 copies of DNA) and specific. This assay distinguishes between infection with PME and ER and will be a valuable tool in the event of heartwater outbreak on the US mainland, or for epidemiological studies involving either disease-causing organism.

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“…Antemortem tests for detecting C. ruminantium include animal subinoculation, cell culture isolation, serodiagnostic tests, DNA hybridization, and PCR. Serodiagnostic methods, such as the indirect fluorescent antibody test, immunoblotting, and enzyme-linked immunosorbent assays (ELISA), have been hampered by cross-reactions with Ehrlichia species (18,22,24). However, the use of recombinant major antigenic protein 1 (MAP1) of C. ruminantium has been recently introduced, and an indirect ELISA based on a specific fragment of this protein (fragment B, referred to herein as MAP1-B) has been developed (32).…”

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confidence: 99%

Validation of the Indirect MAP1-B Enzyme-Linked Immunosorbent Assay for Diagnosis of Experimental Cowdria ruminantium Infection in Small Ruminants

Mboloi¹,

Bekker²,

Kruitwagen

et al. 1999

Clin Diagn Lab Immunol

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The major antigenic protein 1 fragment B (MAP1-B) enzyme-linked immunosorbent assay (ELISA) for the diagnosis of Cowdria ruminantium infections was validated to determine cutoff values and evaluate its diagnostic performance with sheep and goat sera.Cowdria-infected populations consisted of 48 sheep and 44 goats, while the noninfected populations consisted of 64 sheep and 107 goats. Cutoff values were determined by two-graph receiver-operating characteristic (TG-ROC) curves. The cutoff value was set at 31 and 26.6% of the positive control reference samples for sheep and goat sera, respectively. The test’s diagnostic performance was evaluated with measurements of the area under the concentration-time curve (AUC) of the ROC curves and by the valid range proportion (VRP). The AUCs were 0.978 for sheep sera and 0.989 for goat sera. The VRP for both sheep and goat sera was approximately 1.0. The intermediate range (IR), which defines results that are neither positive nor negative, was 0 for goat sera and 2.81 for sheep sera. In an ideal test, the AUC and VRP would be 1.0 and the IR would be 0. In this study these parameters were close to those of an ideal test. It is concluded that the MAP1-B ELISA is a useful test for the diagnosis of C. ruminantiuminfection in small ruminants.

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An immunoblotting diagnostic assay for heartwater based on the immunodominant 32-kilodalton protein of Cowdria ruminantium detects false positives in field sera

Cited by 61 publications

References 22 publications

Detection of the Agent of Heartwater, Cowdria ruminantium , in Amblyomma Ticks by PCR: Validation and Application of the Assay to Field Ticks

Detection of the Agent of Heartwater, Cowdria ruminantium , in Amblyomma Ticks by PCR: Validation and Application of the Assay to Field Ticks

Development of a Quantitative PCR Assay for Differentiating the Agent of Heartwater Disease, Ehrlichia ruminantium , from the Panola Mountain Ehrlichia

Validation of the Indirect MAP1-B Enzyme-Linked Immunosorbent Assay for Diagnosis of Experimental Cowdria ruminantium Infection in Small Ruminants

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