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首页> 外文期刊>Frontiers in Microbiology >A Rapid Antimicrobial Susceptibility Test for Determining Yersinia pestis Susceptibility to Doxycycline by RT-PCR Quantification of RNA Markers
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A Rapid Antimicrobial Susceptibility Test for Determining Yersinia pestis Susceptibility to Doxycycline by RT-PCR Quantification of RNA Markers

机译:通过RT-PCR定量RNA标记快速测定抗生素的药敏试验,以测定<斜体>鼠疫耶尔森氏菌对强力霉素的敏感性

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Great efforts are being made to develop new rapid antibiotic susceptibility tests to meet the demand for clinical relevance versus disease progression. This is important especially in diseases caused by bacteria such as Yersinia pestis , the causative agent of plague, which grows rapidly in vivo but relatively slow in vitro . This compromises the ability to use standard growth-based susceptibility tests to obtain rapid and proper antibiotic treatment guidance. Using our previously described platform of quantifying antibiotic-specific transcriptional changes, we developed a molecular test based on changes in expression levels of doxycycline response-dependent marker genes that we identified by transcriptomic analysis. This enabled us to determine the minimal inhibitory concentration of doxycycline within 7 h compared to the 24 h required by the standard CLSI test. This assay was validated with various Y. pestis strains. Moreover, we demonstrated the applicability of the molecular test, combined with a new rapid bacterial isolation step from blood cultures, and show its relevance as a rapid test in clinical settings.
机译:为了开发新的快速抗生素敏感性试验,正在做出巨大的努力,以满足对临床相关性和疾病进展的需求。这在细菌引起的疾病中尤其重要,例如鼠疫耶尔森菌是鼠疫的病原体,在体内生长迅速,但在体外则相对缓慢。这损害了使用基于生长的标准药敏试验来获得快速,适当的抗生素治疗指导的能力。使用我们先前描述的量化抗生素特异性转录变化的平台,我们基于转录组学分析确定的强力霉素反应依赖性标记基因表达水平的变化,开发了一种分子测试。与标准CLSI测试所需的24小时相比,这使我们能够确定7小时内的强力霉素最低抑菌浓度。用多种鼠疫耶尔森氏菌菌株验证了该测定。此外,我们证明了分子检测的适用性,并结合了从血液培养中快速分离细菌的新步骤,并证明了其在临床环境中作为快速检测的重要性。

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