用于多杀性巴氏杆菌分离株的种属和类型特异性鉴定的聚合酶链反应检测方法的开发。
Development of PCR assays for species- and type-specific identification of Pasteurella multocida isolates.
作者信息
Townsend K M, Frost A J, Lee C W, Papadimitriou J M, Dawkins H J
机构信息
Division of Veterinary Pathobiology, University of Queensland,, Brisbane, Australia.
出版信息
J Clin Microbiol. 1998 Apr;36(4):1096-100. doi: 10.1128/JCM.36.4.1096-1100.1998.
Abstract
Genomic subtractive hybridization of closely related Pasteurella multocida isolates has generated clones useful in distinguishing hemorrhagic septicemia-causing type B strains from other P. multocida serotypes. Oligonucleotide primers designed during the sequencing of these clones have proved valuable in the development of PCR assays for rapid species- and type-specific detection of P. multocida and of type B:2 in particular. This study demonstrated that the primer pair designed from the sequence of the clone 6b (KTT72 and KTSP61) specifically amplified a DNA fragment from types B:2, B:5, and B:2,5 P. multocida and that the primers KMT1T7 and KMT1SP6 produced an amplification product unique to all P. multocida isolates analyzed. It was also shown that PCR amplification performed directly on bacterial colonies or cultures represents an extremely rapid, sensitive method of P. multocida identification.
摘要
对密切相关的多杀巴斯德菌分离株进行基因组消减杂交,已产生了可用于区分引起出血性败血症的B型菌株与其他多杀巴斯德菌血清型的克隆。在对这些克隆进行测序过程中设计的寡核苷酸引物,已证明在开发用于快速进行多杀巴斯德菌物种和类型特异性检测,特别是B:2型检测的PCR检测方法方面很有价值。本研究表明,从克隆6b序列设计的引物对(KTT72和KTSP61)能特异性扩增来自B:2、B:5和B:2,5型多杀巴斯德菌的DNA片段,而引物KMT1T7和KMT1SP6产生的扩增产物是所有分析的多杀巴斯德菌分离株所特有的。研究还表明,直接对细菌菌落或培养物进行PCR扩增是一种极其快速、灵敏的多杀巴斯德菌鉴定方法。
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