Saltatory Rolling Circle Amplification (SRCA): a Novel Nucleic Acid Isothermal Amplification Technique Applied for Rapid Detection of Shigella Spp. in Vegetable Salad

环介导等温扩增 核酸 志贺氏菌 滚动圆复制 等温过程 食品科学 生物 化学 微生物学 细菌 生物化学 沙门氏菌 遗传学 DNA 物理 热力学 DNA复制
作者
Zhiyan Wang,Qian Yang,Yunzhe Zhang,Zhaoxiang Meng,Xiaoyan Ma,Wei Zhang
出处
期刊:Food Analytical Methods [Springer Nature]
卷期号:11 (2): 504-513 被引量:20
标识
DOI:10.1007/s12161-017-1021-0
摘要

Shigella spp. are enteric pathogens that pose a serious threat to public health worldwide. A novel saltatory rolling circle amplification (SRCA) assay was developed to detect Shigella spp. in food targeting the ipaH gene. SRCA as an isothermal amplification method requires no expensive thermocycle instrument and could avoid electrophoresis as visualization results was successfully applied for SRCA. In order to confirm the specificity of this assay, 34 strains including 11 strains belonging to different Shigella species and 23 non-Shigella bacteria were detected with pure cultures. The sensitivity of Shigella flexneri by SRCA was evaluated using agarose gel electrophoresis, which was 7.3 × 101 fg/μL. In addition, the amplification results were also determined by adding the fluorochrome, SYBR Green I (1 μL of 1000×), allowing naked eye visualization of results, and the sensitivity was 7.3 × 100 fg/μL. Moreover, the sensitivity of PCR was 7.3 × 102 fg/μL, showing that the sensitivity of SRCA by electrophoresis and SYBR Green I fluorescence were 10- and 100-fold higher than that of PCR, respectively. The detection limit of SRCA was also evaluated with artificially inoculated vegetable salad without enrichment, and it was 4.7 × 102 and 4.7 × 101 CFU/g by electrophoresis and fluorescence, respectively. The detection limit by PCR was 4.7 × 103 CFU/g, which was 10- and 100-fold higher than that of SRCA. Therefore, SRCA is a potentially reliable tool for rapid and specific detection of Shigella in food and could be useful in underdeveloped countries with limited resources.
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