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首页> 外文期刊>Clinical microbiology and infection: European Society of Clinical Microbiology and Infectious Diseases >Use of a multiplex PCR-based reverse line blot (mPCR/RLB) hybridisation assay for the rapid identification of bacterial pathogens.
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Use of a multiplex PCR-based reverse line blot (mPCR/RLB) hybridisation assay for the rapid identification of bacterial pathogens.

机译:使用基于多重PCR的反向线印迹(mPCR / RLB)杂交测定法快速鉴定细菌病原体。

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摘要

The aim of this study was to develop a sensitive and reliable method for the molecular identification of pathogenic bacteria. A multiplex PCR-based reverse line blot (mPCR/RLB) hybridisation assay was developed and evaluated for the rapid identification of 24 systemic and respiratory bacterial pathogens in routine diagnosis. All species-specific probes designed for the RLB hybridised with amplified DNA only from the corresponding species. Sensitivity limits of the mPCR/RLB assay varied among the 24 target organisms from 0.05 pg to 0.5 ng of genomic DNA. The sensitivity of the assay was 2 x 10(2) CFU/mL for Streptococcus pneumoniae and 6 x 10(2) CFU/mL for Escherichia coli. The specificity of each probe was tested against 24 species. There were no cross-reactions among any of the 43 probes. The mPCR/RLB assay appeared to be a useful alternative tool for the molecular identification of common pathogens.
机译:这项研究的目的是开发一种灵敏可靠的方法来鉴定病原细菌。开发了基于多重PCR的反向线印迹(mPCR / RLB)杂交测定法,并进行了评估,以用于常规诊断中24种系统性和呼吸道细菌病原体的快速鉴定。为RLB设计的所有物种特异性探针仅与来自相应物种的扩增DNA杂交。在24种靶标生物中,mPCR / RLB分析的灵敏度范围从0.05 pg至0.5 ng基因组DNA不等。该测定方法的敏感性对于肺炎链球菌为2 x 10(2)CFU / mL,对于大肠杆菌为6 x 10(2)CFU / mL。测试了每种探针针对24个物种的特异性。 43个探针中没有任何交叉反应。 mPCR / RLB测定法似乎是常见病原体分子鉴定的有用替代工具。

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