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本文引用的文献

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Comparison of PCR assay to culture for surveillance detection of vancomycin-resistant enterococci.用于监测检测耐万古霉素肠球菌的聚合酶链反应(PCR)检测法与培养法的比较。
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Rapid detection of vanA and vanB genes directly from clinical specimens and enrichment broths by real-time multiplex PCR assay.通过实时多重聚合酶链反应检测法直接从临床标本和增菌肉汤中快速检测vanA和vanB基因。
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SHEA guideline for preventing nosocomial transmission of multidrug-resistant strains of Staphylococcus aureus and enterococcus.预防耐多药金黄色葡萄球菌和肠球菌医院内传播的SHEA指南。
Infect Control Hosp Epidemiol. 2003 May;24(5):362-86. doi: 10.1086/502213.
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Evaluation of selective and enrichment media for isolation of glycopeptide-resistant enterococci from faecal specimens.评估用于从粪便标本中分离耐糖肽肠球菌的选择性和增菌培养基。
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A PCR assay for rapid detection of vancomycin-resistant enterococci.一种用于快速检测耐万古霉素肠球菌的聚合酶链反应检测法。
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Am J Infect Control. 2001 Dec;29(6):404-21. doi: 10.1067/mic.2001.119952.
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High rate of false-negative results of the rectal swab culture method in detection of gastrointestinal colonization with vancomycin-resistant enterococci.直肠拭子培养法检测耐万古霉素肠球菌胃肠道定植时假阴性结果的发生率较高。
Clin Infect Dis. 2002 Jan 15;34(2):167-72. doi: 10.1086/338234. Epub 2001 Dec 4.
8
Detection and typing of vancomycin-resistance genes of enterococci from clinical and nosocomial surveillance specimens by multiplex PCR.采用多重聚合酶链反应对临床和医院监测标本中肠球菌的万古霉素耐药基因进行检测和分型。
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Prevalence and determinants of fecal colonization with vancomycin-resistant Enterococcus in hospitalized patients in The Netherlands.荷兰住院患者中耐万古霉素肠球菌粪便定植的患病率及影响因素
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10
Incidence and outcome of vancomycin-resistant enterococcal bacteremia following autologous peripheral blood stem cell transplantation.自体外周血干细胞移植后耐万古霉素肠球菌血症的发生率及转归
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用于从粪便样本中分离耐万古霉素肠球菌的便捷选择性鉴别肉汤培养基。

Convenient selective differential broth for isolation of vancomycin-resistant enterococcus from fecal material.

作者信息

Novicki Thomas J, Schapiro Jeffrey M, Ulness Bruce K, Sebeste Ann, Busse-Johnston Laurel, Swanson Kristine M, Swanzy Susan R, Leisenring Wendy, Limaye Ajit P

机构信息

Department of Laboratory Medicine, University of Washington, Seattle, Washington 98195-7110, USA.

出版信息

J Clin Microbiol. 2004 Apr;42(4):1637-40. doi: 10.1128/JCM.42.4.1637-1640.2004.

DOI:10.1128/JCM.42.4.1637-1640.2004
PMID:15071018
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC387614/
Abstract

Studies have shown that vancomycin broth enrichment is superior to direct plating for the detection of vancomycin-resistant enterococcus (VRE), but vancomycin selective broth is not generally commercially available. We developed an easy-to-prepare VRE selective differential broth and compared it to direct plating on bile esculin azide (BEA) agar for the isolation of VRE from fecal samples. A total of 528 consecutive rectal swabs and stools were inoculated onto BEA agar and into BEA broth with vancomycin at a concentration of 15 microg/ml (BEA VAN15 microg/ml broth). After 1 to 2 days of incubation, broths were subcultured to BEA VAN6 microg/ml agar. Bile esculin-positive colonies from the direct and broth subculture plates were evaluated for the presence of VRE by standard microbiological techniques. Addition of the broth enrichment step led to the detection of significantly more VRE isolates than did direct plating alone (28 versus 18 VRE isolates, respectively). In all, 30 VRE strains were isolated from 29 cultures, all of which were Enterococcus faecium. MICs of vancomycin ranged from 32 microg/ml (n = 2) to > 256 microg/ml (n = 28). Twenty-two VRE isolates were available for further testing: sixteen exhibited a VanA phenotype and six were of the VanB phenotype. van genotypes were in agreement with phenotypes for all VRE isolates except one, which could not be genotyped. The broth method also resulted in significantly fewer bile esculin-positive, non-VRE isolates requiring further workup. We have thus developed an easily prepared vancomycin selective differential broth that is significantly more sensitive and specific in the detection of VRE than is direct fecal plating to BEA agar.

摘要

研究表明,对于耐万古霉素肠球菌(VRE)的检测,万古霉素肉汤增菌法优于直接平板接种法,但万古霉素选择性肉汤一般无商业供应。我们开发了一种易于制备的VRE选择性鉴别肉汤,并将其与在胆汁七叶苷叠氮化物(BEA)琼脂上直接平板接种法进行比较,用于从粪便样本中分离VRE。总共528份连续的直肠拭子和粪便样本接种到BEA琼脂上,并接种到含有浓度为15微克/毫升万古霉素的BEA肉汤(BEA VAN15微克/毫升肉汤)中。孵育1至2天后,将肉汤转种到BEA VAN6微克/毫升琼脂上。通过标准微生物学技术评估直接平板培养和肉汤传代培养平板上胆汁七叶苷阳性菌落中VRE的存在情况。添加肉汤增菌步骤比单独直接平板接种法检测到的VRE分离株明显更多(分别为28株和18株VRE分离株)。总共从29份培养物中分离出30株VRE菌株,均为粪肠球菌。万古霉素的最低抑菌浓度范围为32微克/毫升(n = 2)至>256微克/毫升(n = 28)。22株VRE分离株可用于进一步检测:16株表现为VanA表型,6株为VanB表型。除1株无法进行基因分型外,所有VRE分离株的van基因型与表型一致。肉汤法还使需要进一步检查的胆汁七叶苷阳性、非VRE分离株显著减少。因此,我们开发了一种易于制备的万古霉素选择性鉴别肉汤,在检测VRE方面比粪便直接接种到BEA琼脂上更敏感、更特异。