首页> 外文期刊>Journal of Clinical Microbiology >Development of a Multiplex PCR for the Detection of asa1, gelE, cylA, esp, and hyl Genes in Enterococci and Survey for Virulence Determinants among European Hospital Isolates of Enterococcus faecium
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Development of a Multiplex PCR for the Detection of asa1, gelE, cylA, esp, and hyl Genes in Enterococci and Survey for Virulence Determinants among European Hospital Isolates of Enterococcus faecium

机译:开发用于检测肠球菌中的asa1,gelE,cylA,esp和hyl基因的多重PCR以及欧洲粪肠球菌分离株中毒力决定因素的调查

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A multiplex PCR for the simultaneous detection of five virulence genes (asa1, gelE, cylA, esp, and hyl) in enterococci was developed. The presence of these genes was investigated in 153 clinical and 118 fecal Enterococcus faecium isolates from inpatients at an increased risk of developing infections (such as patients in intensive care units and hematology wards) from 13 hospitals in eight European countries. Of the 271 E. faecium isolates, 135 were vancomycin resistant E. faecium (VREF) isolates and 136 were vancomycin susceptible E. faecium (VSEF) isolates. Susceptibilities to ampicillin, gentamicin, streptomycin, vancomycin, teicoplanin, ramoplanin, quinupristin-dalfopristin, and linezolid were tested by the microdilution method. Overall, the prevalence of esp was significantly higher (P = 0.03) in clinical VREF isolates (92%) than in fecal VREF isolates (73%). In Italy, the prevalence of esp was significantly higher (P = 0.02) in VREF isolates (91%) than in VSEF isolates (68%), whereas in the United Kingdom, hyl was significantly more prevalent (P = 0.01) in VREF isolates (71%) than in VSEF isolates (29%). No significant differences were found for the other countries. Pulsed-field gel electrophoresis was used to check the clonality among the strains tested and showed the spread of two center-specific (esp-positive) VREF clones in Italy and one center-specific (hyl-positive) clone in the United Kingdom. These clones were resistant to ampicillin, gentamicin, and streptomycin. The multiplex PCR reported in this study is a convenient and rapid method for the simultaneous detection of the virulence genes asa1, gelE, cylA, esp, and hyl in enterococci. Molecular analysis showed the intrahospital spread of esp-positive VREF clones (in Italy) and hyl-positive VREF clones (in the United Kingdom); the role of hyl remains to be elucidated.
机译:同时检测五个毒力基因( asa1 gelE cylA esp 和<开发了肠球菌中的em> hyl )。在来自欧洲八家医院的13家医院的153例临床和118例粪便肠屎肠球菌分离株中,这些细菌的感染发生风险增加的患者(例如重症监护病房和血液病房的患者)中检测了这些基因的存在国家。在271个 E。粪杆菌分离株中,有135株对万古霉素耐药。粪肠杆菌(VREF)分离株和136种是万古霉素易感性 E。粪肠杆菌(VSEF)分离株。通过微量稀释法测试了对氨苄西林,庆大霉素,链霉素,万古霉素,替考拉宁,雷莫拉宁,奎奴普丁-达福普汀和利奈唑胺的敏感性。总体而言,临床VREF分离株(92%)中 esp 的患病率( P = 0.03)明显高于粪便VREF分离株(73%)。在意大利,VREF分离株(91%)中 esp 的患病率(VS)分离株(68%)显着更高( P = 0.02),而在英国, hyl 在VREF分离株(71%)中的发生率( P = 0.01)显着高于VSEF分离株(29%)。其他国家没有发现显着差异。脉冲场凝胶电泳用于检查测试菌株之间的克隆性,并显示了意大利的两个中心特异性( esp 阳性)VREF克隆和一个中心特异性( hyl)的VREF克隆的传播-阳性)克隆。这些克隆对氨苄青霉素,庆大霉素和链霉素具有抗性。本研究报道的多重PCR是一种同时快速检测毒力基因 asa1 gelE cylA esp hyl 在肠球菌中。分子分析显示 esp 阳性的VREF克隆(在意大利)和 hyl 阳性的VREF克隆(在英国)在医院内的扩散; hyl 的作用还有待阐明。

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