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dc.contributor.authorSousa, Mariana Silva-
dc.contributor.authorDam, Govert J. van-
dc.contributor.authorPinheiro, Marta Cristhiany Cunha-
dc.contributor.authorDood, Claudia J. de-
dc.contributor.authorPeralta, Jose Mauro-
dc.contributor.authorPeralta, Regina Helena Saramago-
dc.contributor.authorDaher, Elizabeth de Francesco-
dc.contributor.authorCorstjens, Paul L. A. M-
dc.contributor.authorBezerra, Fernando Schemelzer Moraes-
dc.date.accessioned2020-01-31T13:14:12Z-
dc.date.available2020-01-31T13:14:12Z-
dc.date.issued2019-04-
dc.identifier.citationSOUSA, M. S. et al. Performance of an ultra-sensitive assay targeting the circulating anodic antigen (CAA) for detection of Schistosoma mansoni infection in a low endemic area in Brazil. Frontiers in Immunology, v. 10, p. 1-16, apr. 2019.pt_BR
dc.identifier.issn1664-3224 (On line)-
dc.identifier.urihttp://www.repositorio.ufc.br/handle/riufc/49781-
dc.description.abstractTechniques with high sensitivity and specificity are required for an accurate diagnosis in low-transmission settings, where the conventional parasitological methods are insensitive. We determined the accuracy of an up-converting phosphor-lateral flow circulating anodic antigen (UCP-LF CAA) assay in urine and serum for Schistosoma mansoni diagnosis in low-prevalence settings in Ceará, Brazil, before and after praziquantel treatment. Clinical samples of a total of 258 individuals were investigated by UCP-LF CAA, point-of-care—circulating cathodic antigen (POC-CCA), soluble worm antigen preparation (SWAP)-ELISA and Kato-Katz (KK); a selection of 128 stools by real-time PCR technique. Three and 6-weeks after treatment, samples were collected and evaluated by detection Schistosoma circulating antigens (CAA and CCA). The UCP-LF CAA assays detected 80 positives (31%) with urine and 82 positives (31.8%) with serum. The urine POC-CCA and serum SWAP-ELISA assays detected 30 (11.6%) and 107 (40.7%) positives, respectively. The Kato-Katz technique revealed only 4 positive stool samples (1.6%). Among the 128 individuals with complete data records, 19 cases were identified by PCR (14.8%); Sensitivities and specificities of the UCP-LF CAA assays, determined versus a combined reference standard based on CCA/KK/PCR positivity, ranged from60–68%to 68–77%, respectively. In addition only for comparative purposes, sensitivities of the different assays were determined vs. a comparative reference based on CAA/KK/PCR positivity, showing the highest sensitivity for the urine CAA assay (80%), followed by the serum CAA (70.9%), SWAP-ELISA (43.6%), PCR (34.5%), POC-CCA (29.1%), whilst triplicate Kato-Katz thick smears had a very low sensitivity (3.6%). CAA concentrations were higher in serum than in urine and were significantly correlated. There was a significant decrease in urine and serum CAA levels 3 and 6-weeks after treatment. The UCP-LF CAA assays revealed 33 and 28 S. mansoni-infected patients at the 3- and 6-week post-treatment follow-up, respectively. The UCP-LF CAA assays show high sensitivity for the diagnosis of S.mansoni in low-endemicity settings. It detects a considerably higher number of infections than microscopy, POC-CCA or PCR. Also it shows to be very useful for evaluating cure rates after treatment. Hence, the UCP-LF CAA assay is a robust and promising diagnostic approach in low-transmission settings.pt_BR
dc.language.isoenpt_BR
dc.publisherFrontiers in Immunologypt_BR
dc.subjectDiagnósticopt_BR
dc.subjectDiagnosispt_BR
dc.subjectFósforopt_BR
dc.subjectPhosphoruspt_BR
dc.subjectReação em Cadeia da Polimerasept_BR
dc.subjectPolymerase Chain Reactionpt_BR
dc.subjectSchistosoma mansonipt_BR
dc.subjectBrasilpt_BR
dc.subjectBrazilpt_BR
dc.titlePerformance of an ultra-sensitive assay targeting the circulating anodic antigen (CAA) for detection of Schistosoma mansoni Infection in a low endemic area in Brazilpt_BR
dc.typeArtigo de Periódicopt_BR
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