Performance of CHROMagar VRE Medium for the Detection of Airborne Vancomycin-Resistant/Sensitive<i>Enterococcus</i>Species

Hsiao, Pao-Kuei; Cheng, Chieh-Chen; Chang, Kai‐Chih; Yiin, Lih‐Ming; Hsieh, Chia‐Jung; Tseng, Chun-Chieh

doi:10.1080/02786826.2013.865833

Cited by 12 publications

(8 citation statements)

References 36 publications

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“…The Andersen 1‐STG impactor has a very similar air velocity to that of CFCs, at 23.3 m/s . However, our previous studies demonstrated that the culturable collection efficiency of the Andersen 1‐STG impactor was at least 10 times higher than that of CFCs when sampling for the same bacterial species . These results indicated that even though these air sampling velocities are similar, additional sampling stresses such as desiccation and filter elution caused by CFC sampling cause microbes to significantly lose their culturability.…”

Section: Discussionmentioning

confidence: 94%

Altered susceptibility to air sampling stress by filtration is related to colistin resistance development inAcinetobacter baumannii

Tseng

Liou

et al. 2018

Indoor Air

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The accurate quantification of antibiotic-resistant bacteria in indoor air has recently attracted increasing attention. Here, we investigated whether the susceptibility of a nosocomial infection-related microbe, Acinetobacter baumannii, to strong sampling stress caused by Nuclepore filter changes as it develops resistance to a drug called colistin. Both colistin-sensitive A. baumannii (CSAB) and colistin-resistant A. baumannii (CRAB) are generally desiccation-resistant strains that can be collected by filter sampling. However, the resistance of CRAB to the three combined stresses (aerosolization, impaction, and desiccation) caused by filter sampling was 1.8 times lower than that of CSAB (P < 0.05). The sampling stresses caused by filter sampling not only reduced the culturability of A. baumannii but also destroyed proteins to result in cellular protein leakage. CRAB released 17%-38% more extracellular protein than did CSAB when they were both subjected to desiccation stress for 240 minutes (P < 0.01). The combination of using a sampling flow rate of 20 L/min and sampling for 60 minutes with a Nuclepore filter with open-face cassettes (OFCs) is recommended for collecting airborne A. baumannii. A Nuclepore filter operated with closed-face cassettes (CFCs) significantly decreased the culturability of CRAB due to desiccation effects.

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Section: Discussionmentioning

confidence: 94%

Altered susceptibility to air sampling stress by filtration is related to colistin resistance development inAcinetobacter baumannii

Tseng

Liou

et al. 2018

Indoor Air

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“…In field applications, higher sampling flow rates are needed to detect airborne microbe species present at low concentrations. Although sampling with a Nuclepore filter sampler at 20 l/min was not optimized, it has been used to monitor airborne Mycobacterium tuberculosis (Chen and Li, ), S. aureus (Hsiao et al., ), Enterococcus (Hsiao et al., ), and viruses (Tseng et al., ) in the field. For the Nuclepore filter sampler, the lower CR and VR values compared to impingement sampling reflect the loss of microbial culturability and viability during the sampling processes.…”

Section: Resultsmentioning

confidence: 99%

“…The purpose of this study was to optimize PMA‐qPCR for detecting viable A. baumannii and subsequently to evaluate the effects of three bioaerosol sampling methods (the AGI‐30 impinger, BioSampler and Nuclepore filter sampler) on A. baumannii recovery by culture, qPCR, and PMA‐qPCR. Based on our experience, relative humidity (RH) may affect the biological efficiency of the samplers when collecting viruses and gram‐positive bacteria (Hsiao et al., , ; Tseng and Li, ). Therefore, airborne samples were taken at three different RH levels (35%, 55%, and 85% RH).…”

Section: Introductionmentioning

confidence: 99%

Detection of viable antibiotic-resistant/sensitiveAcinetobacter baumanniiin indoor air by propidium monoazide quantitative polymerase chain reaction

et al. 2014

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Acinetobacter baumannii represents a significant cause of nosocomial infections. Therefore, we combined real-time quantitative polymerase chain reaction (PCR) with the propidium monoazide (PMA-qPCR) to assess the feasibility of detecting viable, airborne A. baumannii. The biological collection efficiencies of three samplers for collecting airborne A. baumannii were evaluated by PMA-qPCR in a chamber study. After sampling, the effects of storage in collection fluid on A. baumannii were evaluated. The results showed that the culturable ratio of A. baumannii measured using the culture method was significantly correlated with the viable ratio measured using PMA-qPCR, but was not significantly correlated with the qPCR results. It was indicated that the AGI-30 impinger and the BioSampler were much more effective than the Nuclepore filter sampler for collecting airborne A. baumannii. The storage temperature was critical for aerosol samples, as the loss of viable A. baumannii was minimized when the PMA-bound DNA was stored at -20°C or if the collected cells were stored at 4°C and subsequently processed by PMA-qPCR within 1 month. The PMA-qPCR method was also to distinguish between colistin-sensitive and colistin-resistant A. baumannii, and no colistin-sensitive A. baumannii was detected by PMA-qPCR upon treatment of the BioSampler collection medium with 2 μg/ml colistin for 5 min.

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“…The challenged bacterial aerosols in this study were Acinetobacter baumannii, Enterococcus faecalis, and Staphylococcus aureus. These bacterial species are highly related to nosocomial infection and can cause airborne dispersal and transmission (Hsiao et al 2012;Hsiao et al 2014;Tseng et al 2015). The predecontamination effects of GS5 were studied and divided into two aspects.…”

Section: Introductionmentioning

confidence: 99%

Application of a quaternary ammonium agent on surgical face masks before use for pre-decontamination of nosocomial infection-related bioaerosols

Tseng

Pan

Chang

2016

Aerosol Science and Technology

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Surgical face masks are commonly used by the general public in indoor environments. However, masks could be contaminated, resulting in secondary microbial infections when they act as touchable fomites. Therefore, we evaluated the ability and durability of a covalently bound antimicrobial surfactant coated onto mask surfaces before use to reduce the bacterial burden upon exposure to aerosols. With regard to bacteria that settled onto the mask surface, this antimicrobial product provided >99.3% efficiency for all three tested bacterial species. In addition, the antimicrobial ability of the coated mask maintained efficacy at least one week after coating. For bioaerosols that came into contact with the mask (10 3 CFU/m 3), the antimicrobial agent reduced the average colony rates by 91.8%, but the rates decreased with increased bioaerosol concentrations. Moreover, regardless of whether the coated mask was processed with the bioaerosol penetration test or the National Institute for Occupational Safety and Health-certified sodium chloride aerosol test, the filtration performance of the surgical mask was not significantly altered. These results demonstrate that this antimicrobial product has a durable inhibitory activity for the reduction of bacterial burdens on masks.

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Performance of CHROMagar VRE Medium for the Detection of Airborne Vancomycin-Resistant/SensitiveEnterococcusSpecies

Cited by 12 publications

References 36 publications

Altered susceptibility to air sampling stress by filtration is related to colistin resistance development inAcinetobacter baumannii

Altered susceptibility to air sampling stress by filtration is related to colistin resistance development inAcinetobacter baumannii

Detection of viable antibiotic-resistant/sensitiveAcinetobacter baumanniiin indoor air by propidium monoazide quantitative polymerase chain reaction

Application of a quaternary ammonium agent on surgical face masks before use for pre-decontamination of nosocomial infection-related bioaerosols

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