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Evaluation of the multiplex PCR Allplex-GI assay in the detection of bacterial pathogens in diarrheic stool samples.

Authors :
Martín, Ariadna
Pérez-Ayala, Ana
Chaves, Fernando
Lora, David
Orellana, M. Ángeles
Source :
Journal of Microbiological Methods. Jan2018, Vol. 144, p33-36. 4p.
Publication Year :
2018

Abstract

Rapid and accurate detection of the pathogens that cause gastrointestinal infection is important for appropriate therapy and proper infection control. This study assesses the performance of a new molecular assay for simultaneous detection of 13 different gastrointestinal bacteria in stool specimens. Using the Allplex GI-Bacteria (AGI-BI/AGI-BII) assay, a total of 394 stool samples were tested and the results were compared with culturing on selective differential followed by identification by mass spectroscopy. Discordant results were analyzed by a different multiplex PCR method, the Fast-Track Diagnostics Bacterial gastroenteritis (FTD-BG). The routine method (RM) detected 109 (27.7%) positive samples and the Allplex-GI assay, 261 (66.2%). Analysis of discordant results revealed that the molecular assay detected 44 pathogens that were not detected by the RM, including 23 Campylobacte r spp., 11 Salmonella spp, 3 Y . enterocolitica , 2 EIEC/ Shigella spp, 2 E . coli 0157, 2 C . difficile and 1 Aeromonas spp. Five cases not detected by the molecular method were detected by the RM (3 Aeromonas spp, 1 Salmonella spp and 1 Y . enterocolitica ). For all targets, the percentages of sensitivity and specificity were > 95%, except for Aeromonas spp., which were 81% and 99% respectively. This study suggests that Allplex-GI multiplex PCR is a sensitive and specific assay that enables a rapid and accurate diagnosis of bacterial gastrointestinal infections. [ABSTRACT FROM AUTHOR]

Details

Language :
English
ISSN :
01677012
Volume :
144
Database :
Academic Search Index
Journal :
Journal of Microbiological Methods
Publication Type :
Academic Journal
Accession number :
126944560
Full Text :
https://doi.org/10.1016/j.mimet.2017.10.016