Molecular Characterization of <i>Giardia duodenalis</i> in Children and Adults Sampled in Algeria

Salem Belkessa; Daniel Thomas-Lopez; Karim Houali; Farida Ghalmi; Christen Rune Stensvold

doi:10.3390/microorganisms9010054

Microorganisms (Dec 2020)

Molecular Characterization of <i>Giardia duodenalis</i> in Children and Adults Sampled in Algeria

Salem Belkessa,
Daniel Thomas-Lopez,
Karim Houali,
Farida Ghalmi,
Christen Rune Stensvold

Affiliations

Salem Belkessa: Laboratory of Analytical Biochemistry and Biotechnology (LABAB), Department of Biochemistry and Microbiology, Faculty of Biological and Agronomic Sciences, Mouloud Mammeri University of Tizi Ouzou, Tizi Ouzou 15000, Algeria
Daniel Thomas-Lopez: Laboratory of Parasitology, Department of Bacteria, Parasites & Fungi, Infectious Disease Preparedness, Statens Serum Institut, Artillerivej 5, DK-2300 Copenhagen S, Denmark
Karim Houali: Laboratory of Analytical Biochemistry and Biotechnology (LABAB), Department of Biochemistry and Microbiology, Faculty of Biological and Agronomic Sciences, Mouloud Mammeri University of Tizi Ouzou, Tizi Ouzou 15000, Algeria
Farida Ghalmi: Higher National Veterinary School of Algiers, El Alia, Algiers 16000, Algeria
Christen Rune Stensvold: Laboratory of Parasitology, Department of Bacteria, Parasites & Fungi, Infectious Disease Preparedness, Statens Serum Institut, Artillerivej 5, DK-2300 Copenhagen S, Denmark

DOI: https://doi.org/10.3390/microorganisms9010054
Journal volume & issue: Vol. 9, no. 1
p. 54

Abstract

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The molecular epidemiology of giardiasis in Africa remains unclear. A study was carried out across four hospitals in Algeria. A total of 119 fecal samples from 55 children, 37 adults, and 27 individuals of undetermined age, all scored positive for intestinal parasites by microscopy, and were screened by real-time PCR for Giardia. Molecular characterization of Giardia was performed by assemblage-specific PCR and PCR targeting the triose phosphate isomerase gene (tpi). Of the 119 samples, 80 (67%) were Giardia-positive by real-time PCR. For 48 moderately-highly real-time PCR-positive samples, tpi genotyping assigned 22 samples to Assemblage A and 26 to Assemblage B. Contrary to Assemblage A, Assemblage B exhibited substantial genetic diversity and allelic heterozygosity. Assemblage-specific PCR proved to be specific for discriminating Assemblage A or B but not as sensitive as tpi genotyping. We confirmed that real-time PCR is more sensitive than microscopy for detecting Giardia in stool samples and that robust amplification and sequencing of the tpi gene is feasible when moderate-to-strongly real-time PCR-positive samples are used. This study is one of the few performed in Africa providing genotyping data on Giardia infections in humans. Both assemblages A and B were commonly seen and not associated with specific sociodemographic data.

Published in Microorganisms

ISSN: 2076-2607 (Online)
Publisher: MDPI AG
Country of publisher: Switzerland
LCC subjects: Science: Biology (General)
Website: https://www.mdpi.com/journal/microorganisms

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