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首页> 外文期刊>Journal of chemotherapy >Extended-spectrum beta-lactamase-producing Escherichia coli isolated in the Al-Amiri Hospital in 2003 and compared with isolates from the Farwania hospital outbreak in 1994-96 in Kuwait.
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Extended-spectrum beta-lactamase-producing Escherichia coli isolated in the Al-Amiri Hospital in 2003 and compared with isolates from the Farwania hospital outbreak in 1994-96 in Kuwait.

机译:于2003年在Al-Amiri医院分离出产生超广谱β-内酰胺酶的大肠杆菌,并与1994-96年在科威特的Farwania医院爆发的分离株进行了比较。

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Extended-spectrum beta-lactamases (ESBLs) are a major problem in Kuwait and an accurate method for their detection is essential. This study was designed to evaluate the efficacy of the commercial system (Vitek 2) to identify ESBLs in clinical isolates of Escherichia coli and relate this to their identification by agar dilution methods for use in a diagnostic laboratory. The presence of the major ESBLs parental enzyme groups was confirmed by PCR and the similarity of the strains was determined by pulsed field gel electrophoresis (PFGE) on DNA, cleaved using XbaI endonuclease, to identify clonal spread.Seventy-one separate E. coli isolates from 65 patients were tested. Sixty-two isolates were from 56 patients from the Al-Amiri Hospital and nine isolates from neonates from Farwania Hospital. The isolates were screened for ESBL activity by the Vitek 2 system. Isolates showing positive results were further tested with Etest ESBL strips and by the disc approximation methods. All the isolates were flagged as ESBL-positive by the Vitek 2 advanced expert system (AES). Isolates from all the 65 patients were detected as ESBL positive by the Etest, only if both ESBL strips were used. The double disc approximation test using five different antibiotics could detect ESBL presence in isolates from only 46 patients. In this test, the synergy with cefepime was the most sensitive in ESBL detection, showing their presence in 41 isolates. PCR with primers for bla(TEM) and bla(SHV) demonstrated that one or both of these enzymes in all isolates. PFGE revealed that many different clones were present amongst the isolates.The epidemiology of ESBL E. coli in Kuwait is complex. Many distinct strains are already present in the population, as shown by the results of PFGE. Several testing methods may be required to detect all strains harboring ESBLs.
机译:广谱β-内酰胺酶(ESBLs)是科威特的一个主要问题,准确的检测方法至关重要。这项研究旨在评估商用系统(Vitek 2)在大肠杆菌临床分离株中鉴定ESBLs的功效,并将其与通过琼脂稀释法鉴定用于诊断实验室有关。通过PCR确认了主要的ESBLs亲本酶基团的存在,并通过XbaI核酸内切酶裂解DNA的脉冲场凝胶电泳(PFGE)确定了菌株的相似性,以鉴定克隆的传播.71个分离的大肠杆菌分离株从65名患者中进行了测试。来自Al-Amiri医院的56名患者的62株分离菌,来自Farwania医院的新生儿的9株分离株。通过Vitek 2系统筛选分离物的ESBL活性。显示出阳性结果的分离株进一步用Etest ESBL试纸条和圆盘近似方法进行了测试。 Vitek 2高级专家系统(AES)将所有分离物标记为ESBL阳性。仅当使用两个ESBL试纸时,Etest才会将所有65例患者的分离株检测为ESBL阳性。使用五种不同的抗生素进行的双盘近似试验可以检测到仅46例患者的分离株中存在ESBL。在该测试中,与头孢吡肟的协同作用在ESBL检测中最为敏感,表明它们存在于41种分离物中。用bla(TEM)和bla(SHV)引物进行PCR证明,所有分离物中的一种或两种这些酶。 PFGE揭示了分离物中存在许多不同的克隆。科威特ESBL大肠杆菌的流行病学很复杂。如PFGE结果所示,种群中已经存在许多不同的菌株。要检测所有带有ESBL的菌株,可能需要几种测试方法。

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