Use of Molecular and Reference Susceptibility Testing Methods in a Multicenter Evaluation of MicroScan Dried Overnight Gram-Positive MIC Panels for Detection of Vancomycin and High-Level Aminoglycoside Resistances in Enterococci

Chen, Yao-Shen; Marshall, Steven A.; Winokur, Patricia L.; Coffman, Stacy L.; Wilke, Werner W.; Murray, Patrick R.; Spiegel, Carol A.; Pfaller, Michael A.; Doern, Gary V.; Jones, Ronald N.

doi:10.1128/jcm.36.10.2996-3001.1998

Cited by 21 publications

(2 citation statements)

References 34 publications

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“…Many reports are available in the literature regarding the identification of VRE using conventional microbiological methods, which require time, resources, and space − . The application of conventional polymerase chain reaction technique for detection of VRE, although an improvement over conventional microbiological or biochemical tests, lacks absolute quantitation and requires time-consuming post PCR analysis , .…”

Section: Introductionmentioning

confidence: 99%

Real Time PCR for the Rapid Detection of vanA Gene in Surface Waters and Aquatic Macrophyte by Molecular Beacon Probe

Lata

Ram

Agrawal

et al. 2009

Environ. Sci. Technol.

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Enterococci serve as an "indicator" of fecal contamination for recreational water quality. The vancomycin-resistant-enterococci (VRE) are emerging environmental contaminants in the surface waters. The aim ofthis study wasto develop a rapid and specific molecular beacon probe (MBP)-based real-time PCR assay for detection of vanA gene in surface waters and aquatic macrophyte. The limit of detection (LOD) of the MBP assay was 1 CFU/mL of VRE [r = 0.943; PCR efficiency = 99.7%] in 2-fold dilution format within 2.5 h and demonstrated high specificityfor environmental enterococci isolates exhibiting VanA phenotype (n=25). VRE were detected from downstream surface waters of the rivers impacted by point sources of pollution and recreational activities.The probe detected vanA gene in rootmat associated microbiota of E. crassipes (Mart) Solms. an aquatic nuisance weed, at eutrophic sites of the surface waters (ANOVA p < 0.001). In addition, the assay enabled detection of otherwise nondetectable vanA gene concentration in the upstream sites of two Indian rivers (Student's ttest p < 0.001). The MBP assay developed can be used for sensitive and rapid detection of VRE in surface waters and identification of nonpoint sources of pollution for implementation of preventive measures to protect human health.

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Section: Introductionmentioning

confidence: 99%

Real Time PCR for the Rapid Detection of vanA Gene in Surface Waters and Aquatic Macrophyte by Molecular Beacon Probe

Lata

Ram

Agrawal

et al. 2009

Environ. Sci. Technol.

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“…Enterococcus faecalis and E. faecium account for 80 to 90% and 10 to 15% of enterococcal infections, respectively, and other species including E. gallinarum, E. casseliflavus, E. raffinosus, E. durans, E. hirae, and E. avium, account for a majority of the remainder (14)(15)(16)(17)19). Identification systems, such as Vitek and MicroScan, have been utilized to identify only a few of the Enterococcus species, including E. faecalis, E. faecium, E. durans, and E. avium (1,4,24). Recently, MicroScan revised the gram-positive identification panel by adding Enterococcus species (E. casseliflavus, E. gallinarum, and E. raffinosus and combining E. hirae with E. durans as E. durans/hirae) to the database, reformulating biochemical tests, and including new tests.…”

mentioning

confidence: 99%

Evaluation of the Revised MicroScan Dried Overnight Gram-Positive Identification Panel To Identify Enterococcus Species

Iwen¹,

Rupp

Schreckenberger

et al. 1999

J Clin Microbiol

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The revised MicroScan Dried Overnight Gram-Positive Identification panel was evaluated for its efficacy at identifyingEnterococcus species in comparison with conventional biochemical tests. Supplemental testing of ampicillin-susceptibleEnterococcus faecium for motility and the ability to acidify methyl-α-d-glucopyranoside helped recognizeE. gallinarum and increased the accuracy of the panel for identifying Enterococcus species to 98.5%.

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An update on the emergence of glycopeptide resistance in enterococci

Gardam

Conly

1999

Curr Infect Dis Rep

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Glycopeptide resistance may be either constitutive or transferable (on plasmids or as a transposon), and four phenotypes (van A, B, C, D) have been described to date. Recent data suggest solid media screening protocols appear to be insensitive at detecting low levels of carriage, and up to 40% of colonized patients may be falsely glycopeptide-resistant enterococci (GRE) negative. Managing GRE-colonized or -infected patients using contact precautions appears to be useful in controlling clonal outbreaks, but may be of limited utility once GRE is endemic. Alternate strategies to manage GRE-colonized patients with prolonged carriage and in outpatient or home health settings include using risk-based transmission assessment to limit the logistic and psychosocial difficulties associated with the use of continuous contact precautions. The therapeutic options for treating GRE infection remain limited. Attempts to decolonize GRE-colonized patients with bacitracin appear to be of limited utility.

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Use of Molecular and Reference Susceptibility Testing Methods in a Multicenter Evaluation of MicroScan Dried Overnight Gram-Positive MIC Panels for Detection of Vancomycin and High-Level Aminoglycoside Resistances in Enterococci

Cited by 21 publications

References 34 publications

Real Time PCR for the Rapid Detection of vanA Gene in Surface Waters and Aquatic Macrophyte by Molecular Beacon Probe

Real Time PCR for the Rapid Detection of vanA Gene in Surface Waters and Aquatic Macrophyte by Molecular Beacon Probe

Evaluation of the Revised MicroScan Dried Overnight Gram-Positive Identification Panel To Identify Enterococcus Species

An update on the emergence of glycopeptide resistance in enterococci

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