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嗜水气单胞菌菌落多重PCR方法的建立及应用
引用本文:张静,王永杰,陈红莲,鲍俊杰,孙雯. 嗜水气单胞菌菌落多重PCR方法的建立及应用[J]. 微生物学通报, 2022, 49(2): 841-850
作者姓名:张静  王永杰  陈红莲  鲍俊杰  孙雯
作者单位:安徽省农业科学院水产研究所, 安徽 合肥 230031;水产增养殖安徽省重点实验室, 安徽 合肥 230031
基金项目:安徽省农业科学院科研团队计划项目(18C0513);安徽省重点研究和开发计划项目(201904f06020021)
摘    要:[背景]嗜水气单胞菌(Aeromonas hydrophila)对水产动物、畜禽和人类均有致病性.基因表达的溶血素、气溶素和肠毒素是重要毒力因子,在致病性嗜水气单胞菌早期检测及防治中尤为重要.目前采用菌落直接提取DNA用于多重PCR研究的相关报道较少.[目的]基于菌落PCR方法建立针对嗜水气单胞菌溶血性基因、肠毒素基因...

关 键 词:多重PCR  嗜水气单胞菌  菌落PCR  毒力基因
收稿时间:2021-07-16
修稿时间:2021-08-08

Establishment and application of colony multiplex PCR for Aeromonas hydrophila
ZHANG Jing,WANG Yongjie,CHEN Honglian,BAO Junjie,SUN Wen. Establishment and application of colony multiplex PCR for Aeromonas hydrophila[J]. Microbiology China, 2022, 49(2): 841-850
Authors:ZHANG Jing  WANG Yongjie  CHEN Honglian  BAO Junjie  SUN Wen
Affiliation:Fisheries Research Institute, Anhui Academy of Agricultural Sciences, Hefei 230031, Anhui, China;Key Laboratory of Aquaculture & Stock Enhancement for Anhui Province, Hefei 230031, Anhui, China
Abstract:[Background] Aeromonas hydrophila is pathogenic to aquatic animals, livestock, poultry, and human. Hemolysin, aerolysin, and enterotoxin are major virulence factors particularly important in the early detection and prevention of A. hydrophila. There are few reports using colony PCR to extract templates for multiplex PCR. [Objective] Based on colony PCR, a multiplex PCR assay was established for rapid detection of five genes including hemolysin gene, enterotoxin gene, and 16s rRNA gene of A. hydrophila. [Methods] We used the selective Rimler-Shotts (RS) medium to enrich, isolate, and identify A. hydrophila in the sample. Subsequently, we established and optimized the multiplex PCR conditions for the 16S rRNA, ast, alt, aerA, and act of A. hydrophila and compared the results of multiplex PCR with the DNA templates extracted by different methods in colony PCR. Finally, we evaluated the specificity of the established method by using A. veronii, A. sobria and A. salmonicida. [Results] After 16S rRNA identification of single colonies on RS plates, the colony morphology of A. hydrophila and other cultivable bacteria was preliminarily characterized, and the enrichment degree of A. hydrophila was visually identified. The optimization results of the multiplex PCR system showed that the optimal primer concentration ratio was 16s rRNA:ast:alt:aerA:act=1:2:2:3:4. PCR for fresh bacterial liquids treated with both boiling-refrigerated centrifugation method and boiling-centrifugation method could produce clear bands, while the PCR of single colony required the former method. The established multiplex PCR method was specific. [Conclusion] Colony multiplex PCR can be used to easily and intuitively detect A. hydrophila and its virulence genes without the need of kit extraction of DNA templates, and it was specific.
Keywords:multiplex PCR  Aeromonas hydrophila  colony PCR  virulence gene
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