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Enhanced detection and serotyping of using multiplex polymerase chain reaction
- Source :
- Korean Journal of Pediatrics, Vol 55, Iss 11, Pp 424-429 (2012)
- Publication Year :
- 2012
- Publisher :
- Korean Pediatric Society, 2012.
-
Abstract
- PurposeMethods for quick and reliable detection of Streptococcus pneumoniae are needed for the diagnosis of pneumococcal disease and vaccine studies. This study aimed to show that sequential multiplex polymerase chain reaction (PCR) is more efficient than conventional culture in achieving S. pneumoniae-positive results.MethodsNasopharyngeal (NP) secretions were obtained from 842 pediatric patients admitted with lower respiratory infections at Severance Children's Hospital in Korea between March 2009 and June 2010. For identification and serotype determination of pneumococci from the NP secretions, the secretions were evaluated via multiplex PCR technique with 35 serotype-specific primers arranged in 8 multiplex PCR sets and conventional bacteriological culture technique.ResultsAmong the results for 793 samples that underwent both bacterial culture and PCR analysis for pneumococcal detection, 153 (19.3%) results obtained by PCR and 81 (10.2%) results obtained by conventional culture technique were positive for S. pneumoniae. The predominant serotypes observed, in order of decreasing frequency, were 19A (23%), 6A/B (16%), 19F (11%), 15B/C (5%), 15A (5%), and 11A (4%); further, 26% of the isolates were non-typeable.ConclusionAs opposed to conventional bacteriological tests, PCR analysis can accurately and rapidly identify pneumococcal serotypes.
- Subjects :
- Multiplex polymerase chain reaction
Culture
Pediatrics
RJ1-570
Subjects
Details
- Language :
- English
- ISSN :
- 17381061 and 20927258
- Volume :
- 55
- Issue :
- 11
- Database :
- Directory of Open Access Journals
- Journal :
- Korean Journal of Pediatrics
- Publication Type :
- Academic Journal
- Accession number :
- edsdoj.6f86db288a4e4ce283fb95d9c877fd01
- Document Type :
- article
- Full Text :
- https://doi.org/10.3345/kjp.2012.55.11.424