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Detection and Characterization of Mycoplasma pneumoniae during an Outbreak of Respiratory Illness at a University
Author(s) -
Jessica L. Waller,
Maureen H. Diaz,
Brianna L. Petrone,
Alvaro J. Benitez,
Bernard J. Wolff,
Laura Edison,
Melissa TobinD’Angelo,
Ashley Moore,
Audrey Martyn,
Hope Dishman,
Cherie Drenzek,
Kim Turner,
Lauri A. Hicks,
Jonas M. Winchell
Publication year - 2013
Publication title -
journal of clinical microbiology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.349
H-Index - 255
eISSN - 1070-633X
pISSN - 0095-1137
DOI - 10.1128/jcm.02810-13
Subject(s) - outbreak , mycoplasma pneumoniae , multiple loci vntr analysis , typing , virology , biology , pneumonia , microbiology and biotechnology , variable number tandem repeat , molecular epidemiology , taqman , genotype , multiplex , polymerase chain reaction , medicine , genetics , gene
An outbreak at a university in Georgia was identified after 83 cases of probable pneumonia were reported among students. Respiratory specimens were obtained from 21 students for the outbreak investigation. The TaqMan array card (TAC), a quantitative PCR (qPCR)-based multipathogen detection technology, was used to initially identify Mycoplasma pneumoniae as the causative agent in this outbreak. TAC demonstrated 100% diagnostic specificity and sensitivity compared to those of the multiplex qPCR assay for this agent. All M. pneumoniae specimens (n=12) and isolates (n=10) were found through genetic analysis to be susceptible to macrolide antibiotics. The strain diversity of M. pneumoniae associated with this outbreak setting was identified using a variety of molecular typing procedures, resulting in two P1 genotypes (types 1 [60%] and 2 [40%]) and seven different multilocus variable-number tandem-repeat analysis (MLVA) profiles. Continued molecular typing of this organism, particularly during outbreaks, may enhance the current understanding of the epidemiology of M. pneumoniae and may ultimately lead to a more effective public health response.

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