Rapid Detection of
            <i>vanA</i>
            and
            <i>vanB</i>
            Genes Directly from Clinical Specimens and Enrichment Broths by Real-Time Multiplex PCR Assay

Palladino, Silvano; Kay, Ian; Flexman, James; I, Boehm; Costa, Anna Maria; Lambert, Erica J.; Christiansen, Keryn

doi:10.1128/jcm.41.6.2483-2486.2003

Cited by 81 publications

(55 citation statements)

References 12 publications

(18 reference statements)

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“…This has led to increased interest in screening of patients for colonization as well as to increased interest in methods used for a fast, sensitive, and reliable VRE detection (Vonberg et al, 2007). Rapid screening methods for VRE using direct polymerase chain reaction (PCR) from rectal swabs or stool have been described ( [Palladino et al, 2003], [Petrich et al, 1999] and [Satake et al, 1997]); some of these assays are commercially available ( [Bourdon et al, 2010], [Stamper et al, 2007], [Sloan et al, 2004] and [Usacheva et al, 2010]). These tests have been evaluated in a few studies performed, and excellent sensitivity and specificity for detecting vanA enterococci were shown, and a low specificity due to comparably high rates of supposed false-positive vanB samples appeared as a problem ( [Stamper et al, 2007] and [Sloan et al, 2004]).…”

Section: Introductionmentioning

confidence: 99%

Comparison of direct cultivation on a selective solid medium, polymerase chain reaction from an enrichment broth, and the BD GeneOhm™ VanR Assay for identification of vancomycin-resistant enterococci in screening specimens

Werner

Serr

Schütt

et al. 2011

Diagnostic Microbiology and Infectious Disease

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Section: Introductionmentioning

confidence: 99%

Comparison of direct cultivation on a selective solid medium, polymerase chain reaction from an enrichment broth, and the BD GeneOhm™ VanR Assay for identification of vancomycin-resistant enterococci in screening specimens

Werner

Serr

Schütt

et al. 2011

Diagnostic Microbiology and Infectious Disease

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“…Of these, vanA and vanB predominate and are the only two that are of epidemiologic importance due to the transmissibility of the resistance genes (2). The vanA and vanB genes are found almost exclusively in Enterococcus faecium and E. faecalis, the enterococcal species that most commonly cause disease in humans, but have been detected in other species of Enterococcus (16,32); and vanB has been detected in resident anaerobic flora of the human bowel (41a). VanA-mediated resistance is associated with inducible high-level resistance to vancomycin and teicoplanin, while vanB-mediated resistance is associated with resistance to vancomycin but retained susceptibility to teicoplanin.…”

Section: Detection Of Vre Directly From Patient Samplesmentioning

confidence: 99%

Rapid Detection of Antimicrobial-Resistant Organism Carriage: an Unmet Clinical Need

Diekema¹,

Dodgson²,

Sigurðardóttir³

et al. 2004

J Clin Microbiol

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“…Our pediatric institution has a low prevalence of VRE, and we use conventional VRE screening methods, which require up to 5 days to identify VRE-positive patients (9) and 3 days to identify VREnegative patients. Other attempts to expedite VRE detection have included the use of 24-to 36-h selective broth cultures (9) and real-time PCR assays, using either swabs or broth for the identification of vanA and vanB genes encoding vancomycin resistance determinants (9,11). Preliminary work in our laboratory indicated that direct testing of rectal swabs with the Roche LightCycler VRE detection kit using DNA from our automated extraction protocol was inhibited in 50% of the samples tested.…”

mentioning

confidence: 99%

A 24-Hour Screening Protocol for Identification of Vancomycin-Resistant Enterococcus faecium

et al. 2006

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We describe a 24-h protocol for the identification of patients who are positive for vancomycin-resistant Enterococcus faecium (VRE), using stool and rectal swab samples and VRE screening broth, automated DNA extraction, and real-time PCR for vanA and vanB genes. Compared to conventional screening methods, this protocol had a high sensitivity and specificity and a negative predictive value.Vancomycin-resistant enterococci (VRE) are antibiotic-resistant colonizers of the gastrointestinal tract that cause nosocomial outbreaks of both colonization of the gastrointestinal tract and infection at various sites (2, 4, 6, 7). Our pediatric institution has a low prevalence of VRE, and we use conventional VRE screening methods, which require up to 5 days to identify VRE-positive patients (9) and 3 days to identify VREnegative patients. Other attempts to expedite VRE detection have included the use of 24-to 36-h selective broth cultures (9) and real-time PCR assays, using either swabs or broth for the identification of vanA and vanB genes encoding vancomycin resistance determinants (9, 11). Preliminary work in our laboratory indicated that direct testing of rectal swabs with the Roche LightCycler VRE detection kit using DNA from our automated extraction protocol was inhibited in 50% of the samples tested. In light of these findings, the purpose of this study was to validate a 24-h protocol for the confirmation of VRE-negative and VRE-positive patients by the use of stool or rectal swab samples screened with a VRE-selective broth for 18 h prior to automated DNA extraction and real-time PCR.This study was initiated during an outbreak of infection with vanA-positive vancomycin-resistant Enterococcus faecium at a quaternary-care pediatric institution. A total of 1,863 samples were screened for VRE, and 34 patients were found to be colonized with vancomycin-resistant E. faecium. Twenty-six stool and 26 rectal swab samples were collected from 34 VRE culture-positive patients. We randomly chose 55 stool samples and 54 rectal swabs from patients defined as VRE contacts who were admitted to a specific floor at the same time as a VRE-positive person. Rectal swabs were transported in Amies agar gel medium with charcoal (Copan Venturi Transystem swab, Copan, Italy). Amies agar gel medium without charcoal (Copan Venturi Transystem swab, Copan, Italy) was used for VRE-positive mock samples. Stool samples were collected in 100-ml Starplex LeakBuster specimen containers (Starplex Scientific, Inc., Etobicoke, ON, Canada). Direct culture and enrichment broth cultures were carried out using the same swab. Stool samples from patients were frozen at Ϫ70°C until inoculated into the VRE-selective broth. Swabs were stored at 4°C until the next available PCR run. The positive and negative control VRE strains were Enterococcus faecalis strain ATCC 51299 and E. faecalis strain ATCC 29212, respectively.Rectal swab and stool samples were inoculated onto screening plates consisting of Difco mEnterococcus agar with 6 g/ml vancomycin (Becton Dickinson and...

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Rapid Detection of vanA and vanB Genes Directly from Clinical Specimens and Enrichment Broths by Real-Time Multiplex PCR Assay

Cited by 81 publications

References 12 publications

Comparison of direct cultivation on a selective solid medium, polymerase chain reaction from an enrichment broth, and the BD GeneOhm™ VanR Assay for identification of vancomycin-resistant enterococci in screening specimens

Comparison of direct cultivation on a selective solid medium, polymerase chain reaction from an enrichment broth, and the BD GeneOhm™ VanR Assay for identification of vancomycin-resistant enterococci in screening specimens

Rapid Detection of Antimicrobial-Resistant Organism Carriage: an Unmet Clinical Need

A 24-Hour Screening Protocol for Identification of Vancomycin-Resistant Enterococcus faecium

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