The accuracy of extended-spectrum beta-lactamase detection in Escherichia coli and Klebsiella pneumoniae in South African laboratories using the Vitek 2 Gram-negative susceptibility card AST-N255

Southern African Journal of Infectious Diseases

 
 
Field Value
 
Title The accuracy of extended-spectrum beta-lactamase detection in Escherichia coli and Klebsiella pneumoniae in South African laboratories using the Vitek 2 Gram-negative susceptibility card AST-N255
 
Creator Young, Andrea L. Nicol, Mark P. Moodley, Clinton Bamford, Colleen M.
 
Subject — Antimicrobial susceptibility testing; Extended-spectrum beta-lactamase (ESBL) Detection; Automated systems for ESBL Detection; Vitek 2 ESBL detection; Gram-negative susceptibility card AST-N255
Description Background: Phenotypic detection of extended-spectrum beta-lactamases (ESBLs) is based on the inhibition of ESBL enzymes by β-lactamase inhibitors and on the comparison of cephalosporin activity with or without a β-lactamase inhibitor. Many South African diagnostic laboratories rely on the Vitek 2 for automated susceptibility testing and for ESBL detection. However, the Gram-negative susceptibility card currently used locally (AST-N255) has been modified and its accuracy for ESBL detection is not known.Methods: We randomly selected 50 isolates of Klebsiella pneumoniae and Escherichia coli from a collection of clinical bloodstream isolates from Groote Schuur Hospital from 2015 to 2016, including ESBL-producing and non-ESBL-producing strains. We used standardised phenotypic (disc diffusion and broth microdilution) and genotypic (conventional polymerase chain reaction (PCR) for blaCTX-M, blaSHV and blaTEM) methods for detection of ESBLs. We compared ESBL detection by Vitek 2 to a composite reference standard comprising ESBL detection either by both phenotypic methods or by one phenotypic method together with genotypic detection.Results: The sensitivity of Vitek 2 system for detection of ESBLs was 33/36 or 92% (78% – 97%) for E. coli, and 40/40 or 100% (91% – 100%) for K. pneumoniae, whilst specificity was 10/10 or 100% (72% – 100%) and 9/10 or 90% (60% – 98%), respectively. This is comparable with previous studies.Conclusion: Using a composite reference standard of the phenotypic and genotypic methods employed in this study, no Vitek-categorised ESBL E. coli or K. pneumoniae was found to be a non-ESBL with the exception of possible misinterpretation with K. pneumoniae SHV-hyper-producing isolates.
 
Publisher AOSIS Publishing
 
Contributor
Date 2019-08-07
 
Type info:eu-repo/semantics/article info:eu-repo/semantics/publishedVersion — —
Format text/html application/epub+zip application/xml application/pdf
Identifier 10.4102/sajid.v34i1.114
 
Source Southern African Journal of Infectious Diseases; Vol 34, No 1 (2019); 6 pages 2313-1810 2312-0053
 
Language eng
 
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https://sajid.co.za/index.php/sajid/article/view/114/129 https://sajid.co.za/index.php/sajid/article/view/114/128 https://sajid.co.za/index.php/sajid/article/view/114/130 https://sajid.co.za/index.php/sajid/article/view/114/127
 
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Rights Copyright (c) 2019 Colleen Bamford, Andrea L. Young, Clinton Moodley, Mark Nicol https://creativecommons.org/licenses/by/4.0
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