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Implementation of vanA and vanB genes by PCR technique research interest in system (Xpert vanA/vanB CepheidR) closed in a laboratory of microbiology in managing an outbreak to Enterococcus faecium resistant glycopeptide (EfRG)
被引:5
|作者:
Dekeyser, S.
[1
]
Beclin, E.
[1
]
Descamps, D.
[2
]
机构:
[1] Ctr Hosp German & Gauthier Bethune, Unite Hyg & Lutte Infect Nosocomiales, F-62408 Bethune, France
[2] Ctr Hosp German & Gauthier Bethune, Com Lutte Infect Nosocomiales, F-62408 Bethune, France
来源:
关键词:
Real time PCR;
VanA/VanB;
Enterococcus;
Glycopeptide;
Resistance;
D O I:
10.1016/j.patbio.2010.07.013
中图分类号:
R36 [病理学];
学科分类号:
100104 ;
摘要:
Subject. - The closed system PCR for the rapid detection of vanA and vanB genes (Xpert vanA/vanB Cepheid (R)) was evaluated in our laboratory, to improve the rapidity of the response and thus the management of patients and isolation measures during two GRE outbreaks. Method. - From March to December 2009, 565 samples were analysed by PCR associated to bacterial culture initially for all samples for 2 months (n = 75), and thereafter for PCR-positive samples only. Results. - In this study, sensitivity and negative predictive values of the PCR were 100%. Specificity was evaluated in the presence and absence of outbreak: 69.3 and 76.8% respectively. The variability of false positive rates between units were lower in nonepidemic than during epidemic phase. The global false positive rate was 23.9%. Conclusion. - This easy-to-use technology provides rapid results... four samples are tested in 1 h versus 72 h for culture. Despite its reagent cost, it represents an important hospital diagnostic tool: improvement of the management of cohorting areas and patient transfer between units, adaptation of isolation measures and treatments. However, culture remains necessary to confirm any positive result obtained by PCR and for epidemiological surveillance. (C) 2010 Elsevier Masson SAS. All rights reserved.
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页码:73 / 78
页数:6
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