Sensitive Diagnosis and Post-Treatment Follow-Up of Schistosoma mansoni Infections in Asymptomatic Eritrean Refugees by Circulating Anodic Antigen Detection and Polymerase Chain Reaction

Author:

Hoekstra Pytsje T.1,Chernet Afona23,de Dood Claudia J.4,Brienen Eric A. T.1,Corstjens Paul L. A. M.4,Labhardt Niklaus D.235,Nickel Beatrice23,Wammes Linda J.6,van Dam Govert J.1,Neumayr Andreas237,van Lieshout Lisette1

Affiliation:

1. 1Department of Parasitology, Leiden University Medical Center, Leiden, The Netherlands;

2. 2Swiss Tropical and Public Health Institute, Basel, Switzerland;

3. 3University of Basel, Basel, Switzerland;

4. 4Department of Cell and Chemical Biology, Leiden University Medical Center, Leiden, The Netherlands;

5. 5Department of Infectious Diseases and Hospital Epidemiology, University Hospital Basel, Basel, Switzerland;

6. 6Department of Medical Microbiology, Leiden University Medical Center, Leiden, The Netherlands;

7. 7Department of Public Health and Tropical Medicine, College of Public Health, Medical and Veterinary Sciences, James Cook University, Queensland, Australia

Abstract

ABSTRACT. The increasing number of refugees coming from or passing through Schistosoma-endemic areas and arriving in Europe highlights the importance of screening for schistosomiasis on arrival, and focuses attention on the choice of diagnostic test. We evaluate the diagnostic performance of circulating anodic antigen (CAA) detection in 92 asymptomatic refugees from Eritrea. Results were compared with already-available stool microscopy, serology, and urine point-of-care circulating cathodic antigen (POC-CCA) data. For a full diagnostic comparison, real-time polymerase chain reaction (PCR) and the POC-CCA were included. All outcomes were compared against a composite reference standard. Urine and serum samples were subjected to the ultra-sensitive and highly specific up-converting particle lateral flow CAA test, Schistosoma spp. real-time PCR was performed on urine and stool, and the POC-CCA was used on urine using the G-score method. CAA was detected in 43% of urine and in 40% of serum samples. Urine PCR was negative in all 92 individuals, whereas 25% showed Schistosoma DNA in stool. POC-CCA was positive in 30% of individuals. The CAA test confirmed all microscopy positives, except for two cases that were also negative by all other diagnostic procedures. Post-treatment, a significant reduction in the number of positives and infection intensity was observed, in particular regarding CAA levels. Our findings confirm that microscopy, serology, and POC-CCA lack the sensitivity to detect all active Schistosoma infections. Accuracy of stool PCR was similar to microscopy, indicating that this method also lacks sensitivity. The CAA test appeared to be the most accurate method for screening active Schistosoma infections and for monitoring treatment efficacy.

Publisher

American Society of Tropical Medicine and Hygiene

Subject

Virology,Infectious Diseases,Parasitology

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