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首页> 外文期刊>Journal of Clinical Microbiology >SNaPBcen: a Novel and Practical Tool for Genotyping Burkholderia cenocepacia
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SNaPBcen: a Novel and Practical Tool for Genotyping Burkholderia cenocepacia

机译:SNaPBcen:一种新的实用工具,用于对洋葱伯克霍尔德氏菌进行基因分型

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Burkholderia cenocepacia is the most prevalent and feared member of the Burkholderia cepacia complex in lung infections of cystic fibrosis (CF). Genotyping and monitoring of long-term colonization are critical at clinical units; however, the differentiation of specific lineages performed by multilocus sequence typing (MLST) is still limited to a small number of isolates due to the high cost and time-consuming procedure. The aim of this study was to optimize a protocol (the SNaPBcen assay) for extensive bacterial population studies. The strategy used for the SNaPBcen assay is based on targeting single nucleotide polymorphisms (SNPs) located in MLST genes instead of sequencing full MLST sequences. Nonpolymorphic and redundant MLST positions were eliminated, and a set of 24 polymorphisms included in the SNaPBcen assay ensures a high-resolution genomic characterization. These polymorphisms were identified based on the comparative analysis of 137 B. cenocepacia MLST profiles available online (http://pubmlst.org/bcc/). The group of 81 clinical isolates of B. cenocepacia examined in this study using the SNaPBcen assay revealed 51 distinct profiles, and a final discriminatory power of 0.9997 compared with MLST was determined. The SNaPBcen assay was able to reveal isolates with microvariations and the presence of multiple clonal variants in patients chronically colonized with B. cenocepacia. Main phylogenetic subgroups IIIA, IIIB, and IIIC of B. cenocepacia could be separated by the Gl94R polymorphism included in the panel. The SNaPBcen assay proved to be a rapid and robust alternative to the standard MLST for B. cenocepacia, allowing the simultaneous analysis of multiple polymorphisms following amplification and mini-sequencing reactions.
机译:Burkholderia ceocepacia是在囊性纤维化(CF)肺部感染中Burkholderia cepacia复合体中最普遍和最担心的成员。基因分型和长期定植的监测在临床部门至关重要。然而,由于高成本和费时的过程,通过多基因座序列分型(MLST)进行的特定谱系的分化仍然限于少数分离株。这项研究的目的是针对广泛的细菌种群研究优化方案( SNaPBcen 分析)。用于 SNaPBcen 分析的策略是基于靶向位于MLST基因中的单核苷酸多态性(SNP),而不是对完整的MLST序列进行测序。消除了非多态和冗余MLST位置, SNaPBcen 分析中包含的24种多态性可确保高分辨率的基因组表征。这些对多态性的确定是基于对在线提供的(137)cenocepacia MLST概况的比较分析(http://pubmlst.org/bcc/)。在本研究中,使用 SNaPBcen 分析检测的81例新细菌双歧杆菌临床分离群显示出51种不同的特征,与MLST相比,最终鉴别力为0.9997。通过 SNaPBcen 分析,能够揭示出长期存在高新芽孢杆菌的患者中存在微小变异的分离株以及多种克隆变异的存在。酿酒酵母的主要系统发育亚组IIIA,IIIB和IIIC可以通过面板中包含的Gl94R多态性进行分离。事实证明, SNaPBcen 分析是一种快速而可靠的替代方法,可用于cenocepacia的标准MLST,可同时分析扩增和微测序反应后的多种多态性。

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