Effect of routine use of a multiplex PCR for detection of vanA- and vanB- mediated enterococcal resistance on accuracy, costs and earlier reporting.

نویسندگان

  • A Petrich
  • K Luinstra
  • B Page
  • S Callery
  • D Stevens
  • A Gafni
  • D Groves
  • M Chernesky
  • J B Mahony
چکیده

A multiplex PCR (MPCR) for detection of vanA-and vanB-mediated resistance to vancomycin was optimized and adapted for use in the routine microbiology laboratory. Consecutive specimens (1196) submitted for vancomycin resistant Enterococci (VRE) surveillance were processed by clinical technologists on Bile Esculin Azide Agar containing 6 mg/L vancomycin (BEAA/Vanco6) plates and 466 showing black colony growth were processed by conventional biochemical testing (CBT) and by MPCR. CBT identified 208 VRE positives. MPCR detected 205 of the CBT- positives plus an additional 10. Analysis of the discordant specimens determined that 5 CBT- negative/MPCR-positive specimens also contained Enterococci with vanC resistance, 3 CBT-positive/MPCR-negative specimens were true positives, and 5 CBT-negative/MPCR-positive specimens occurred due to technical error. The sensitivity and specificity of MPCR were 98.4% and 96.1%. MPCR identifications of VRE were achieved approximately 48 h earlier than CBT and at 60% of the costs.

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تشخیص ژن‌های vanA, vanB, vanC با روش Multiplex-PCR در ایزوله‌های انتروکوکوس فکالیس و انتروکوکوس فسیوم در بیماران بستری

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عنوان ژورنال:
  • Diagnostic microbiology and infectious disease

دوره 41 4  شماره 

صفحات  -

تاریخ انتشار 2001