Development of Real-Time Fluorescent PCR for Rapid Detection of Haempohlius parasuis 被引量：1

Development of Real-Time Fluorescent PCR for Rapid Detection of Haempohlius parasuis

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摘要 [ Objective] To develop a real-time fluorescent PCR assay for rapid detection of Haempohlius parasuis （HPS）. [ Method] According to the conservative sequences of 16 S rRNA genes of HPS published in GenBank, a pair of specific primers was designed. The real-time fluorescent PCR was developed by optimizing primer concentration and annealing temperature. And its specificity and reproducibility were evaluated. Ten HPS- suspected samples were detected by the developed method. [ Result] The lowest detection limit of the developed real-time fluorescent PCR was 50 copies/μl. This method had good reproducibility, and its coefficient of variation was lower than 2%. Only HPS rather than Streptococcus suis type 2, Staphylococcus aureus, E. coli DH5 alpha, and swine Salmonella typhi could be detected by the developed real-time fluorescent PCR. The HPS-pesitive samples detected by this method were also positive when they were detected by isolation of bacteria or conventional PCR. [ Conclusion] The developed real-time fluorescent PCR is rapid, sensitive, specific and highly reproducible; thus, it can be used for rapid detection of HPS. [ Objective] To develop a real-time fluorescent PCR assay for rapid detection of Haempohlius parasuis （HPS）. [ Method] According to the conservative sequences of 16 S rRNA genes of HPS published in GenBank, a pair of specific primers was designed. The real-time fluorescent PCR was developed by optimizing primer concentration and annealing temperature. And its specificity and reproducibility were evaluated. Ten HPS- suspected samples were detected by the developed method. [ Result] The lowest detection limit of the developed real-time fluorescent PCR was 50 copies/μl. This method had good reproducibility, and its coefficient of variation was lower than 2%. Only HPS rather than Streptococcus suis type 2, Staphylococcus aureus, E. coli DH5 alpha, and swine Salmonella typhi could be detected by the developed real-time fluorescent PCR. The HPS-pesitive samples detected by this method were also positive when they were detected by isolation of bacteria or conventional PCR. [ Conclusion] The developed real-time fluorescent PCR is rapid, sensitive, specific and highly reproducible; thus, it can be used for rapid detection of HPS.

作者 LI Jun XIE Yu-zhou XUAN Xiong-biao CHEN Ze-xiang YANG Wei MA Chun-xia HU Shuai PENG Hao XU Li-gan XlE Yong-ping PAN Yan

机构地区 Guangxi Veterinary Research Institute

出处《Animal Husbandry and Feed Science》 CAS 2010年第10期22-25,共4页 动物与饲料科学（英文版）

基金 funded by the Key Technologies R&D Program of Guangxi of China (0993009-1)

关键词 Haempohlius parasuis Real-time fluorescent PCR 16 S rRNA Haempohlius parasuis Real-time fluorescent PCR 16 S rRNA

分类号 S513 [农业科学—作物学] S763.7 [农业科学—森林保护学]

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