Accuracy of urine circulating cathodic antigen (CCA) test for Schistosoma mansoni diagnosis in different settings of Côte d'Ivoire

Jean T Coulibaly; Stefanie Knopp; Nicaise A N'Guessan; Kigbafori D Silué; Thomas Fürst; Laurent K Lohourignon; Jean K Brou; Yve K N'Gbesso; Penelope Vounatsou; Eliézer K N'Goran; Jürg Utzinger

doi:10.1371/journal.pntd.0001384

Accuracy of urine circulating cathodic antigen (CCA) test for Schistosoma mansoni diagnosis in different settings of Côte d'Ivoire

PLoS Negl Trop Dis. 2011 Nov;5(11):e1384. doi: 10.1371/journal.pntd.0001384. Epub 2011 Nov 22.

Authors

Jean T Coulibaly¹, Stefanie Knopp, Nicaise A N'Guessan, Kigbafori D Silué, Thomas Fürst, Laurent K Lohourignon, Jean K Brou, Yve K N'Gbesso, Penelope Vounatsou, Eliézer K N'Goran, Jürg Utzinger

Affiliation

¹ Department of Epidemiology and Public Health, Swiss Tropical and Public Health Institute, Basel, Switzerland.

Abstract

Background: Promising results have been reported for a urine circulating cathodic antigen (CCA) test for the diagnosis of Schistosoma mansoni. We assessed the accuracy of a commercially available CCA cassette test (designated CCA-A) and an experimental formulation (CCA-B) for S. mansoni diagnosis.

Methodology: We conducted a cross-sectional survey in three settings of Côte d'Ivoire: settings A and B are endemic for S. mansoni, whereas S. haematobium co-exists in setting C. Overall, 446 children, aged 8-12 years, submitted multiple stool and urine samples. For S. mansoni diagnosis, stool samples were examined with triplicate Kato-Katz, whereas urine samples were tested with CCA-A. The first stool and urine samples were additionally subjected to an ether-concentration technique and CCA-B, respectively. Urine samples were examined for S. haematobium using a filtration method, and for microhematuria using Hemastix dipsticks.

Principal findings: Considering nine Kato-Katz as diagnostic 'gold' standard, the prevalence of S. mansoni in setting A, B and C was 32.9%, 53.1% and 91.8%, respectively. The sensitivity of triplicate Kato-Katz from the first stool and a single CCA-A test was 47.9% and 56.3% (setting A), 73.9% and 69.6% (setting B), and 94.2% and 89.6% (setting C). The respective sensitivity of a single CCA-B was 10.4%, 29.9% and 75.0%. The ether-concentration technique showed a low sensitivity for S. mansoni diagnosis (8.3-41.0%). The specificity of CCA-A was moderate (76.9-84.2%); CCA-B was high (96.7-100%). The likelihood of a CCA-A color reaction increased with higher S. mansoni fecal egg counts (odds ratio: 1.07, p<0.001). A concurrent S. haematobium infection or the presence of microhematuria did not influence the CCA-A test results for S. mansoni diagnosis.

Conclusion/significance: CCA-A showed similar sensitivity than triplicate Kato-Katz for S. mansoni diagnosis with no cross-reactivity to S. haematobium and microhematuria. The low sensitivity of CCA-B in our study area precludes its use for S. mansoni diagnosis.

Publication types

Evaluation Study
Research Support, Non-U.S. Gov't

MeSH terms

Animals
Antigens, Helminth / urine*
Child
Clinical Laboratory Techniques / methods*
Cote d'Ivoire
Cross-Sectional Studies
Feces / chemistry
Female
Glycoproteins / urine*
Helminth Proteins / urine*
Humans
Immunoassay / methods
Male
Parasitology / methods*
Prevalence
Schistosomiasis mansoni / diagnosis*
Sensitivity and Specificity
Urine / chemistry

Substances

Antigens, Helminth
CCA protein, Schistosoma mansoni
Glycoproteins
Helminth Proteins