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首页> 外文期刊>Journal of Clinical Microbiology >Diversity and stability of restriction enzyme profiles of plasmid DNA from methicillin-resistant Staphylococcus aureus.
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Diversity and stability of restriction enzyme profiles of plasmid DNA from methicillin-resistant Staphylococcus aureus.

机译:耐甲氧西林金黄色葡萄球菌质粒DNA限制性内切酶谱的多样性和稳定性。

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Nosocomial infections caused by methicillin-resistant Staphylococcus aureus (MRSA) are a significant epidemiological problem. Detecting the sources of epidemic strains and preventing their access to patients, however, depend upon the availability of techniques to reliably distinguish among MRSA strains. We evaluated restriction enzyme analysis of plasmid DNA for use as an epidemiological marker of MRSA strains. The diversity of plasmid types was assessed by examining 120 clinical and environmental MRSA isolates from five southern California hospitals and from the American Type Culture Collection. Thirty-seven distinctive EcoRI digestion patterns were observed. We characterized each strain by the number of plasmids it contained and the sizes of the fragments that were generated by EcoRI. Very few of the isolates (4.2%) lacked plasmids, and some (6.7%) contained DNA that was not digested by EcoRI. Several isolates (12.5%) contained two or more plasmids. We were able to assess the stability of MRSA plasmid types by tracking epidemic strains over a 2-year period. We also examined successive isolates from 10 individual patients during their hospitalization. In all but one case, the patient's plasmid profiles remained unchanged. We conclude that the diversity and stability of MRSA plasmid types make them excellent epidemiological markers. In support of this conclusion, we found that our data provided significant epidemiological insights. Two epidemic strains, accounting for more than half of the infections, were identified in the five hospitals. The remaining cases were sporadic, caused by MRSA strains that appeared very infrequently and that may have originated from sources outside the hospitals.
机译:由耐甲氧西林的金黄色葡萄球菌(MRSA)引起的医院感染是一个重大的流行病学问题。然而,检测流行毒株的来源并阻止其接触患者,取决于可靠区分MRSA毒株的技术的可用性。我们评估了质粒DNA的限制性内切酶分析,以用作MRSA菌株的流行病学标记。通过检查来自加利福尼亚南部五家医院和美国典型培养物保藏中心的120种临床和环境MRSA分离株,评估了质粒类型的多样性。观察到了37种独特的EcoRI消化模式。我们通过每个菌株包含的质粒数量以及EcoRI产生的片段大小来表征每个菌株。极少数分离株(4.2%)缺少质粒,而一些分离株(6.7%)含有未被EcoRI消化的DNA。几个分离株(12.5%)包含两个或多个质粒。我们能够通过跟踪流行病菌株在2年期间评估MRSA质粒类型的稳定性。我们还检查了10例患者在住院期间的连续分离株。除一种情况外,患者的质粒谱均保持不变。我们得出结论,MRSA质粒类型的多样性和稳定性使它们成为出色的流行病学标记。为了支持这一结论,我们发现我们的数据提供了重要的流行病学见解。在五家医院中发现了两种流行毒株,占感染的一半以上。其余病例是零星的,由很少出现的MRSA株引起,可能来自医院外的来源。

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