Comparison of multiplex-PCR and antigen detection for differential diagnosis of Entamoeba histolytica

Autor:	Heloisa Werneck de Macedo, José Mauro Peralta, Magali G. M. Barreto, Regina Helena Saramago Peralta, Helena Lúcia Carneiro Santos
Rok vydání:	2007
Předmět:	Microbiology (medical) Dispar lcsh:QR1-502 Antigens Protozoan Multiplex-PCR Polymerase Chain Reaction Sensitivity and Specificity lcsh:Microbiology lcsh:Infectious and parasitic diseases law.invention Microbiology Diagnosis Differential Entamoeba Immunoenzyme Techniques Feces Entamoeba histolytica fluids and secretions law parasitic diseases Multiplex polymerase chain reaction medicine Animals Humans lcsh:RC109-216 Multiplex Amoebiasis Polymerase chain reaction Entamoebiasis biology Reproducibility of Results DNA Protozoan medicine.disease biology.organism_classification digestive system diseases Infectious Diseases amebiasis
Zdroj:	Brazilian Journal of Infectious Diseases, Volume: 11, Issue: 3, Pages: 365-370, Published: JUN 2007 Brazilian Journal of Infectious Diseases v.11 n.3 2007 Brazilian Journal of Infectious Diseases Brazilian Society of Infectious Diseases (BSID) instacron:BSID Brazilian Journal of Infectious Diseases, Vol 11, Iss 3, Pp 365-370
ISSN:	1413-8670
DOI:	10.1590/s1413-86702007000300013
Popis:	Amebiasis is an infection caused by Entamoeba histolytica. However, differentiation between E. histolytica and Entamoeba dispar, which are morphologically identical species, is essential for treatment decision, precaution of the invasive disease and public health. The purpose of the present study was to evaluate a Multiplex -PCR for detection and differentiation of E. histolytica from E. dispar from fresh stool samples in comparison with the coproantigen commercial ELISA. Microscopic examination of stools using the Coprotest method, detection of stool antigen by enzyme-linked immunosorbent assay kit and a home made Multiplex-PCR, were used for the diagnosis of amoebiasis infection. Analysis of the 127 stools samples by microscopy examination demonstrated that only 27 (21%) samples were positive for E. histolytica/E. dispar complex. Among these stool samples, 11 were positive by Multiplex-PCR, with nine presenting the diagnostic fragment characteristic of E. dispar (96 bp) and two presenting diagnostic fragment of E. histolytica (132 bp). Among negative samples detected by microscopic examination, three positive samples for E. dispar and one positive for E. histolytica by Multiplex-PCR was observed. This denotes a low sensibility of microscopic examination when a single stool sample is analyzed. Assay for detection of E. histolytica antigen was concordant with multiplex-PCR in relation to E. histolytica. Statistical analysis comparing the sensibility tests was not done because of the low number of E. histolytica cases. The results demonstrate the importance of the specific techniques use for the differentiation between E. histolytica and E. dispar.
Databáze:	OpenAIRE
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