Comparative Evaluation of Luminex xTAG® Gastrointestinal Pathogen Panel and Direct-From-Stool Real-Time PCR for Detection of C. difficile Toxin tcdB in Stool Samples from a Pediatric Population

Author:

Tyrrell Hannah,Morin Sarah B. N.,Lloyd Colin D.,Parsons BrendonORCID,Stokowski Taryn,Xie Jianling,Zhuo RanORCID,Lee Bonita E.,Pang Xiao-Li,Freedman Stephen B.ORCID,Chui LindaORCID

Abstract

Detection of Clostridioides difficile toxins in patients with gastroenteritis has increasingly been accomplished through the use of enteric multiplex syndromic panels. Comparisons of the performance of these panels to both direct-from-stool (DFS) and culture-enriched stools followed by polymerase chain reaction (PCR) methods in pediatric populations are limited. Here, we compare the performance of the Luminex xTAG® Gastrointestinal Pathogen Panel (GPP) to our DFS in-house real-time PCR (DFS RT-PCR) assay for the detection of C. difficile toxin gene, tcdB, using 2641 stool specimens collected from children enrolled in the Alberta Provincial Pediatric EnTeric Infection Team (APPETITE) study in Alberta, Canada. We used culture enrichment followed by in-house RT-PCR to resolve discordant results between the two assays. We found excellent agreement (k = 0.89) between the GPP and our DFS RT-PCR assay: the positive percent agreement between the two assays was 97%, and the negative percent agreement was 99%. GPP, a multi-analyte platform can easily be implemented into a routine diagnostic laboratory for detecting enteric pathogens including C. difficile.

Funder

Alberta Provincial Pediatric EnTeric Infection TEam

Alberta Children’s Hospital Foundation Professorship in Child Health and Wellness

Alberta Health Services Residual Funds

Alberta Innovates Summer Research Studentship

Publisher

MDPI AG

Subject

Virology,Microbiology (medical),Microbiology

Reference26 articles.

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