4.7 Article

Evaluation of Molecular Serotyping Assays for Shigella flexneri Directly on Stool Samples

期刊

JOURNAL OF CLINICAL MICROBIOLOGY
卷 59, 期 2, 页码 -

出版社

AMER SOC MICROBIOLOGY
DOI: 10.1128/JCM.02455-20

关键词

PCR; Shigella flexneri; serotype; stool

资金

  1. Bill and Melinda Gates Foundation
  2. Centers for Disease Control and Prevention [75D30118C02910]
  3. NIH [K24 AI102972]

向作者/读者索取更多资源

Real-time PCR assays were evaluated for identifying major serotypes of Shigella flexneri using 0-antigen modification genes. The assays demonstrated high sensitivity and specificity compared to conventional serotyping, with efficient performance on direct stool samples as well. These PCR assays provide a novel tool for S. flexneri serotype identification.
Shigella flexneri is prevalent worldwide and is the most common Shigella species in many countries. At least 19 S. flexneri serotypes exist, and serotype information is important for epidemiologic and vaccine development purposes. We evaluated the performance of real-time PCR assays for 0-antigen modification genes to identify the major serotypes on isolates and direct stool samples. The assays were formulated into two multiplex panels: one panel included gtrll, gtrV, gtrX, oac, and wzx6 to identify S. flexneri serotypes 2a, 2b, 3a, 5a, 5b, 6, and X, and the other panel included ipaH, gtrl, gtrlc, and gtr1V to confirm Shigella detection and further identify S. flexneri serotypes 1a, 1b, 1d, 3b, 4a, 4b, 7a, and 7b. We first evaluated 283 Shigella isolates, and PCR serotyping demonstrated 97.0% (95% confidence interval, 93.0% to 99.0%) sensitivity and 99.9% (99.9% to 100%) specificity compared to conventional serotyping. The assays then were utilized on direct stool specimens. A quantitative detection algorithm was developed with a validation set of 174 Shigella culture-positive stool samples and further tested with a derivation set of 164 samples. The PCR serotyping on stool achieved 93% (89% to 96%) sensitivity and 99% (99% to 100%) specificity compared to serotyping. Most discrepancies were genotypic-phenotypic discordance, not genotypic failure. These real-time PCR assays provide an efficient and novel tool for S. flexneri serotype identification.

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