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首页> 外文期刊>Journal of Clinical Microbiology >Macrolide Resistance Determination and Molecular Typing of Mycoplasma pneumoniae in Respiratory Specimens Collected between 1997 and 2008 in The Netherlands
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Macrolide Resistance Determination and Molecular Typing of Mycoplasma pneumoniae in Respiratory Specimens Collected between 1997 and 2008 in The Netherlands

机译:1997年至2008年在荷兰收集的呼吸道样本中肺炎支原体的大环内酯抗性测定和分子分型

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摘要

An important role in the treatment regimens for Mycoplasma pneumoniae infections is played by macrolide (ML) antibiotics. In the past few years, however, a steady increase has been detected in the worldwide prevalence of ML-resistant (MLr) M. pneumoniae strains. It is obvious that this increase necessitates a continuous monitoring of MLr and, when detected, modification of antibiotic treatment modalities. Previously, we developed a pyrosequencing-based assay system for the genetic determination of MLr as well as molecular typing of M. pneumoniae. In this study, the sensitivity of this system was improved by the inclusion of a nested-PCR protocol. The modified system was applied to 114 M. pneumoniae-positive specimens that were obtained from a collection of 4,390 samples from patients with acute respiratory tract infections. These samples were collected between 1997 and 2008 in The Netherlands. The pyrosequencing system produced reliable data in 86% of the specimens that contained >500 M. pneumoniae genome copies/ml of patient sample. Each of these samples contained DNA of the ML-sensitive genotype. While 43% of the samples were found to harbor the M. pneumoniae subtype 1 genotype, 57% contained the subtype 2 genotype. We conclude that the pyrosequencing-based assay system is a useful tool for MLr determination and molecular typing of M. pneumoniae in patient samples. MLr-associated M. pneumoniae genotypes, however, were not found in the current study population.
机译:大环内酯(ML)抗生素在肺炎支原体感染的治疗方案中起着重要作用。然而,在过去的几年中,在全球范围内发现了耐ML的(ML r )肺炎支原体菌株的稳定增长。显然,这种增加需要对ML r 进行连续监测,并在检测到抗生素治疗方式时对其进行修改。以前,我们开发了一种基于焦磷酸测序的测定系统,用于ML r 的遗传测定以及肺炎支原体的分子分型。在这项研究中,通过加入巢式PCR方案提高了该系统的灵敏度。改进后的系统应用于114例肺炎支原体阳性标本,这些标本取自急性呼吸道感染患者的4390份样品。这些样本是在1997年至2008年之间在荷兰收集的。焦磷酸测序系统在86%的标本中提供了可靠的数据,这些标本包含> 500 M.这些样品中的每一个都含有ML敏感基因型的DNA。虽然发现有43%的样本具有肺炎支原体亚型1基因型,但57%包含亚型2基因型。我们得出的结论是,基于焦磷酸测序的测定系统是用于确定患者样品中肺炎支原体的ML r 和分子分型的有用工具。然而,在当前研究人群中未发现与ML r 相关的肺炎支原体基因型。

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