Abstract
Strongyloidiasis is caused by the nematode Strongyloides stercoralis which has the unique ability to reproduce and complete its entire life cycle within the human host through its autoinfection cycle. Diagnosis of this infection is important because of its potential to cause fatal hyperinfection syndrome or disseminated infections in those with defective cellular immunity. Parasitological methods based on faecal microscopy and culture often fail to detect low-intensity infections. A multiplex polymerase chain reaction (PCR) assay was developed for the detection of S. stercoralis, Ascaris lumbricoides, and Enterobius vermicularis by designing primers specific for the ITS1 region of ribosomal DNA of S. stercoralis and A. lumbricoides and 18S region of rRNA of E. vermicularis. A 61-year-old patient presented with chronic gastrointestinal and respiratory symptoms and weight loss with a stool microscopy positive for helminth larvae. Stool cultures with the Harada–Mori technique yielded L3 larvae which were identified as S. stercoralis based on morphology. The multiplex PCR performed on DNA extracted from stool elicited the expected band at 129 bp on gel electrophoresis of the PCR yield providing molecular evidence of intestinal strongyloidiasis. The patient's gastrointestinal symptoms improved with a six-day course of albendazole (400 mg twice daily). Negative posttreatment stool microscopy, culture, and PCR confirmed successful clearance of infection. Molecular-based PCR assay is a promising tool to diagnose and assess the therapeutic efficacy of anthelmintics in intestinal helminthiases such as strongyloidiasis.
Highlights
Strongyloidiasis is a soil-transmitted helminthiasis (STH), caused by the nematode Strongyloides stercoralis and to a lesser extent by the zoonotic species Strongyloides fuelleborni and Strongyloides cf fuelleborni [1,2,3]
Serology-based antigen or antibody detection assays have the potential to be used in the diagnosis of strongyloidiasis and other intestinal helminthiases due to their high sensitivity [7]. ese include the enzyme-linked immunosorbent assay (ELISA) and its derived procedures such as Falcon assay screening test ELISA, dot-ELISA, luciferase immunoprecipitation system (LIPS), immunoblotting, indirect immunofluorescent antibody test (IFAT)/ direct immunofluorescent antibody test, and rapid diagnostic tests (RDTs) [23]
Despite Sri Lanka being a tropical country with favorable climatic conditions for the sustenance of the life cycle of S. stercoralis, the infection rates are very low (0–1.6%) [8,9,10] compared to neighboring countries such as India (6.6–12.2%) [6]
Summary
Strongyloidiasis is a soil-transmitted helminthiasis (STH), caused by the nematode Strongyloides stercoralis and to a lesser extent by the zoonotic species Strongyloides fuelleborni and Strongyloides cf fuelleborni [1,2,3]. In Sri Lanka, strongyloidiasis is infrequently detected in stool surveys compared to other major STH infections [8,9,10]. Serology-based antigen or antibody detection assays have the potential to be used in the diagnosis of strongyloidiasis and other intestinal helminthiases due to their high sensitivity [7]. Polymerase chain reaction- (PCR-) based applications are considered a priority area in the field of modern diagnostics It has shown a higher sensitivity than microscopy, at low intensities of infections [25]. Molecular-based diagnostics are infrequently applied in the diagnosis of intestinal helminthiases, they are considered a necessity in the STH elimination drive to detect areas with low intensities of infection [27, 28].
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