Strongyloidiasis in humans: diagnostic efficacy of four conventional methods and real-time polymerase chain reaction

Campo-Polanco, Laura Francisca; Sarmiento, José Mauricio Hernández; Mesa, Miguel Antonio; Franco, Carlos Jaime Velásquez; López, Lucelly; Botero, Luz Elena; Builes, Lina Andrea Gutiérrez

Campo-Polanco, Laura Francisca; Sarmiento, José Mauricio Hernández; Mesa, Miguel Antonio; Franco, Carlos Jaime Velásquez; López, Lucelly; Botero, Luz Elena; Builes, Lina Andrea Gutiérrez.

Campo-Polanco, Laura Francisca; Universidad Pontificia Bolivariana. Facultad de Medicina. Grupo Biología de Sistemas. Medellín. CO
Sarmiento, José Mauricio Hernández; Universidad Pontificia Bolivariana. Facultad de Medicina. Grupo Salud Publica. Medellín. CO
Mesa, Miguel Antonio; Universidad Pontificia Bolivariana. Clínica Universitaria Bolivariana. Sección Reumatología. Medellín. CO
Franco, Carlos Jaime Velásquez; Universidad Pontificia Bolivariana. Clínica Universitaria Bolivariana. Sección Reumatología. Medellín. CO
López, Lucelly; Universidad Pontificia Bolivariana. Facultad de Medicina. Grupo Salud Publica. Medellín. CO
Botero, Luz Elena; Universidad Pontificia Bolivariana. Facultad de Medicina. Grupo Biología de Sistemas. Medellín. CO
Builes, Lina Andrea Gutiérrez; Universidad Pontificia Bolivariana. Facultad de Medicina. Grupo Biología de Sistemas. Medellín. CO

Rev. Soc. Bras. Med. Trop ; 51(4): 493-502, July-Aug. 2018. tab, graf

Article in English | LILACS | ID: biblio-957450

ABSTRACT

ABSTRACT

Abstract

INTRODUCTION:

Strongyloides stercoralis is an intestinal parasitic nematode that causes hyperinfection and/or a dissemination syndrome in hosts, which is often difficult to diagnose. This study aims to compare the diagnostic efficacy of four conventional methods used to diagnose strongyloidiasis with real-time polymerase chain reaction (qPCR) to detect S. stercoralis in fecal samples.

METHODS:

We analyzed 143 fecal samples collected from Colombian regions with varying degrees of risk for intestinal infections caused by S. stercoralis to assess the validity, performance, overall efficiency, and concordance of the qPCR using a direct stool test, modified Ritchie concentration technique, agar plate culture, and Harada-Mori technique as reference tests. RESULTS While four fecal samples were positive for S. stercoralis using conventional methods, 32 were positive via qPCR. The diagnostic sensitivity of the qPCR was 75% [95% confidence interval (CI) 20.07-100%], whereas its specificity, negative predictive value, negative likelihood ratio, and Youden's J index were 78.42% (95% CI 71.22-85.62%), 99.09% (95% CI 96.86-100%), 0.32 (95% CI 0.06-1.74), and 0.53, respectively. In addition, the estimated kappa index between the qPCR and the conventional methods was 0.12 (95% CI -0.020-0.26).

CONCLUSIONS:

The diagnostic sensitivity of qPCR to detect strongyloidiasis is analogous to that of conventional parasitology methods, with an additional advantage of being capable of identifying the parasite DNA at low sample concentrations.

Subject(s)

Humans; Animals; Male; Female; Adolescent; Adult; Young Adult; Strongyloides/genetics; Strongyloidiasis/diagnosis; RNA, Ribosomal, 18S/genetics; RNA, Protozoan/genetics; Feces/parasitology; Real-Time Polymerase Chain Reaction/methods; Strongyloides/isolation & purification; Sensitivity and Specificity; Middle Aged

Helminthology; Intestinal diseases; Molecular diagnostic techniques; Strongyloides stercoralis

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Full text: Available Index: LILACS (Americas) Main subject: Strongyloides / Strongyloidiasis / RNA, Ribosomal, 18S / RNA, Protozoan / Feces / Real-Time Polymerase Chain Reaction Type of study: Diagnostic study / Prognostic study Limits: Animals / Female / Humans / Male Language: English Journal: Rev. Soc. Bras. Med. Trop Journal subject: Tropical Medicine Year: 2018 Type: Article Affiliation country: Colombia Institution/Affiliation country: Universidad Pontificia Bolivariana/CO

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