Detection of group a streptococcal pharyngitis by quantitative PCR

被引:47
|
作者
Dunne, Eileen M. [1 ]
Marshall, Julia L. [3 ]
Baker, Ciara A. [2 ]
Manning, Jayne [1 ]
Gonis, Gena [4 ]
Danchin, Margaret H. [2 ,3 ]
Smeesters, Pierre R. [2 ,5 ]
Satzke, Catherine [1 ,6 ]
Steer, Andrew C. [2 ,7 ]
机构
[1] Murdoch Childrens Res Inst, Parkville, Vic, Australia
[2] Murdoch Childrens Res Inst, Grp A Streptococcus, Parkville, Vic, Australia
[3] Univ Melbourne, Dept Paediat, Parkville, Vic 3052, Australia
[4] Royal Childrens Hosp, Dept Lab Serv, Parkville, Vic 3052, Australia
[5] Univ Libre Bruxelles, Fac Sci, Inst Biol & Med Mol, Lab Genet & Physiol Bacterienne, Gosselies, Belgium
[6] Univ Melbourne, Dept Microbiol & Immunol, Parkville, Vic 3052, Australia
[7] Univ Melbourne, Ctr Int Child Hlth, Parkville, Vic 3052, Australia
关键词
ACUTE SORE THROAT; DIAGNOSIS; PNEUMONIAE; CARRIAGE; PYOGENES; CHILDREN; BURDEN;
D O I
10.1186/1471-2334-13-312
中图分类号
R51 [传染病];
学科分类号
100401 ;
摘要
Background: Group A streptococcus (GAS) is the most common bacterial cause of sore throat. School-age children bear the highest burden of GAS pharyngitis. Accurate diagnosis is difficult: the majority of sore throats are viral in origin, culture-based identification of GAS requires 24-48 hours, and up to 15% of children are asymptomatic throat carriers of GAS. The aim of this study was to develop a quantitative polymerase chain reaction (qPCR) assay for detecting GAS pharyngitis and assess its suitability for clinical diagnosis. Methods: Pharyngeal swabs were collected from children aged 3-18 years (n = 91) and adults (n = 36) located in the Melbourne area who presented with sore throat. Six candidate PCR assays were screened using a panel of reference isolates, and two of these assays, targeting speB and spy1258, were developed into qPCR assays. The qPCR assays were compared to standard culture-based methods for their ability to detect GAS pharyngitis. GAS isolates from culture positive swabs underwent emm-typing. Clinical data were used to calculate McIsaac scores as an indicator of disease severity. Results: Twenty-four of the 127 samples (18.9%) were culture-positive for GAS, and all were in children (26%). The speB qPCR had 100% sensitivity and 100% specificity compared with gold-standard culture, whereas the spy1258 qPCR had 87% sensitivity and 100% specificity. Nine different emm types were found, of which emm 89, 3, and 28 were most common. Bacterial load as measured by qPCR correlated with culture load. There were no associations between symptom severity as indicated by McIsaac scores and GAS bacterial load. Conclusions: The speB qPCR displayed high sensitivity and specificity and may be a useful tool for GAS pharyngitis diagnosis and research.
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页数:7
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