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Detection of Aeromonas salmonicida from fish by using polymerase chain reaction amplification of the virulence surface array protein gene.

机译:毒力表面阵列蛋白基因的聚合酶链反应扩增检测鱼中的鲑鱼气单胞菌。

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摘要

A DNA-based assay was developed to detect Aeromonas salmonicida from infected fish by analyzing tissues, feces, and the tank water in which the infected fish were held. This analysis was done both by direct detection from samples and after a bacterial outgrowth step. Polymerase chain reaction (PCR) amplification of a 421-bp sequence from the 3' region of the surface array protein gene (vapA) of A. salmonicida provided a specific and sensitive method for the detection and identification of this important fish pathogen. The sensitivity of PCR detection of A. salmonicida directly from tissues was less than 10 CFU/mg. Furthermore, a detection level of 5 fg, equivalent to approximately 1 cell, was obtained by using purified chromosomal DNA as the template. This highly reproducible assay, which requires 45 min to complete, is therefore sensitive enough to be used as a noninvasive method for monitoring fish populations for the presence of carrier fish. Because the surface protein array (A-layer) is a virulence factor of A. salmonicida, PCR analysis with oligonucleotide primers directed at vapA can also be used to provide information on the potential virulence of a strain.
机译:通过分析组织,粪便和盛有被感染鱼的鱼缸水,开发了一种基于DNA的检测方法来检测被感染鱼中的鲑鱼气单胞菌。通过直接从样品中检测以及在细菌繁殖步骤之后进行此分析。鲑鱼拟南芥表面阵列蛋白基因(vapA)3'区域421 bp序列的聚合酶链反应(PCR)扩增为检测和鉴定这种重要的鱼类病原体提供了一种特异性和灵敏的方法。直接从组织中检测沙门氏菌的PCR灵敏度低于10 CFU / mg。此外,通过使用纯化的染色体DNA作为模板,获得了5 fg的检测水平,相当于大约1个细胞。因此,这种高度可重复的分析需要45分钟才能完成,因此非常灵敏,可以用作监测鱼类种群中是否存在携带鱼类的非侵入性方法。由于表面蛋白阵列(A层)是鲑鱼曲霉的毒力因子,因此针对vapA的寡核苷酸引物的PCR分析也可用于提供有关菌株潜在毒力的信息。

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