Development of a real-time PCR assay and comparison to CHROMagarTM STEC to screen for Shiga toxin-producing Escherichia coli in stool, Cape Town, South Africa

African Journal of Laboratory Medicine

 
 
Field Value
 
Title Development of a real-time PCR assay and comparison to CHROMagarTM STEC to screen for Shiga toxin-producing Escherichia coli in stool, Cape Town, South Africa
 
Creator Kalule, John B. Keddy, Karen H. Smith, Anthony Nicol, Mark P. Robberts, Lourens
 
Subject Microbiology; Assay development; Laboratory testing Shiga toxin-producing E. coli; CHROMagarTMSTEC; Assay development
Description Introduction: Shiga toxin-producing Escherichia coli (STEC) is an emerging infectious pathogen which could lead to haemolytic uremic syndrome. Even though previous studies have compared the performance of CHROMagarTMSTEC to real-time polymerase chain reaction (PCR) in Europe, no study has been done to assess its performance on African isolates.Objectives: This project aimed to validate and test an in-house-developed duplex real-time PCR and use it as a reference standard to determine the performance of CHROMagarTMSTEC on African isolates from diarrhoeic stool samples.Methods: This study evaluated STEC diagnostic technology on African isolates. An in-house-developed duplex real-time PCR assay for detection of stx1 and stx2 was validated and tested on diarrhoeic stool samples and then used as a reference standard to assess the performance of CHROMagarTMSTEC. Real-time PCR was used to screen for stx in tryptic soy broth and the suspected STEC isolates, while conventional PCR was used to detect the other virulence genes possessed by the isolates.Results: The real-time PCR limit of detection was 5.3 target copies/μL of broth. The mean melting temperature on melt-curve analysis for detection of stx1 was 58.2 °C and for stx2 was 65.3 °C. Of 226 specimens screened, real-time PCR detected stx in 14 specimens (6.2%, 95% confidence interval = 3.43% – 10.18%). The sensitivity, specificity, negative predictive value and positive predictive value of the CHROMagarTMSTEC were 33.3%, 77.4%, 95.3% and 11.3%.Conclusions: The in-house developed real-time PCR assay is a sensitive and specific option for laboratory detection of STEC as compared to CHROMagarTMSTEC in this setting.
 
Publisher AOSIS
 
Contributor National Research Foundation, ACP-RISE scholarship fund, ADB-HEST scholarship fund.
Date 2017-12-14
 
Type info:eu-repo/semantics/article info:eu-repo/semantics/publishedVersion — Experimental
Format text/html application/epub+zip text/xml application/pdf
Identifier 10.4102/ajlm.v6i1.609
 
Source African Journal of Laboratory Medicine; Vol 6, No 1 (2017); 8 pages 2225-2010 2225-2002
 
Language eng
 
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The following web links (URLs) may trigger a file download or direct you to an alternative webpage to gain access to a publication file format of the published article:

https://ajlmonline.org/index.php/ajlm/article/view/609/942 https://ajlmonline.org/index.php/ajlm/article/view/609/941 https://ajlmonline.org/index.php/ajlm/article/view/609/943 https://ajlmonline.org/index.php/ajlm/article/view/609/937
 
Coverage Cape Town, South Africa — Stool from diarrhea patients irrespective of age, gender or ethnicity
Rights Copyright (c) 2017 John B. Kalule, Karen H. Keddy, Anthony Smith, Mark P. Nicol, Lourens Robberts https://creativecommons.org/licenses/by/4.0
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