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使用盒式聚合酶链反应排除类鼻疽的克隆性暴发。

Using BOX-PCR to exclude a clonal outbreak of melioidosis.

作者信息

Currie Bart J, Gal Daniel, Mayo Mark, Ward Linda, Godoy Daniel, Spratt Brian G, LiPuma John J

机构信息

Northern Territory Clinical School, Flinders University, Royal Darwin Hospital, Darwin, Northern Territory, Australia.

出版信息

BMC Infect Dis. 2007 Jun 30;7:68. doi: 10.1186/1471-2334-7-68.

Abstract

BACKGROUND

Although melioidosis in endemic regions is usually caused by a diverse range of Burkholderia pseudomallei strains, clonal outbreaks from contaminated potable water have been described. Furthermore B. pseudomallei is classified as a CDC Group B bioterrorism agent. Ribotyping, pulsed-field gel electrophoresis (PFGE) and multilocus sequence typing (MLST) have been used to identify genetically related B. pseudomallei isolates, but they are time consuming and technically challenging for many laboratories.

METHODS

We have adapted repetitive sequence typing using a BOX A1R primer for typing B. pseudomallei and compared BOX-PCR fingerprinting results on a wide range of well-characterized B. pseudomallei isolates with MLST and PFGE performed on the same isolates.

RESULTS

BOX-PCR typing compared favourably with MLST and PFGE performed on the same isolates, both discriminating between the majority of multilocus sequence types and showing relatedness between epidemiologically linked isolates from various outbreak clusters.

CONCLUSION

Our results suggest that BOX-PCR can be used to exclude a clonal outbreak of melioidosis within 10 hours of receiving the bacterial strains.

摘要

背景

尽管在流行地区类鼻疽通常由多种不同的伯克霍尔德菌假鼻疽菌株引起,但已报道过因受污染饮用水导致的克隆性暴发。此外,假鼻疽伯克霍尔德菌被列为美国疾病控制与预防中心(CDC)的B类生物恐怖主义病原体。核糖体分型、脉冲场凝胶电泳(PFGE)和多位点序列分型(MLST)已被用于鉴定基因相关的假鼻疽伯克霍尔德菌分离株,但对许多实验室来说,这些方法耗时且技术要求高。

方法

我们采用BOX A1R引物进行重复序列分型来对假鼻疽伯克霍尔德菌进行分型,并将一系列特征明确的假鼻疽伯克霍尔德菌分离株的BOX-PCR指纹图谱结果与对相同分离株进行的MLST和PFGE结果进行比较。

结果

BOX-PCR分型与对相同分离株进行的MLST和PFGE相比表现良好,既能区分大多数多位点序列类型,又能显示来自不同暴发集群的流行病学相关分离株之间的相关性。

结论

我们的结果表明,BOX-PCR可用于在收到细菌菌株后的10小时内排除类鼻疽的克隆性暴发。

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