Establishment of the gene detection method of Schistosoma mansoni based on the recombinase-aided isothermal amplification assay

Song ZHAO; Yan-Hong LIU; Yu-Ying YE; Wei LI; Jian-Feng ZHANG; Li-Chuan GUO; Qing-Jie YING; Hai-Tao YANG; Kun YANG

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Establishment of the gene detection method of Schistosoma mansoni based on the recombinase-aided isothermal amplification assay

VernacularTitle:基于重组酶介导核酸等温扩增反应的曼氏血吸虫基因检测方法的建立
Author: Song ZHAO ¹ ; Yan-Hong LIU ² ; Yu-Ying YE ¹ ; Wei LI ¹ ; Jian-Feng ZHANG ¹ ; Li-Chuan GUO ² ; Qing-Jie YING ² ; Hai-Tao YANG ¹ ; Kun YANG ¹
Author Information

1. Key Laboratory of National Health Commission on Parasitic Disease Control and Prevention, Jiangsu Provincial Key Laboratory on Parasite and Vector Control Technology, Jiangsu Institute of Parasitic Diseases, Wuxi 214064, China
2. Jiangsu Qitian Gene Technology Co., Ltd., China
Publication Type:Journal Article
Keywords: Schistosoma mansoni; Gene detection; Isothermal amplification of nucleic acid; Fluorescent probe; Recombinase
From: Chinese Journal of Schistosomiasis Control 2020;32(4):335-339
CountryChina
Language:Chinese
Abstract: Objective To establish a recombinase-aided isothermal amplification (RAA) assay for nucleic acid detection of Schistosoma mansoni. Methods The 121 bp highly-repeated sequence of S. mansoni was selected as the target gene fragment to be detected. The primers and fluorescent probes were designed using the Amplfix software, and a fluorescent RAA assay was established and optimized. The fluorescent RAA assay was performed to detect gradient diluent recombinant plasmids containing target gene fragment and different concentrations of S. mansoni genomic DNA to determine the sensitivity, and this assay was applied to detect the genomic DNA of S. japonicum, S. haematobium, Ancylostoma duodenale and Clonorchis sinensis to evaluate the specificity. Results A fluorescent RAA assay was successfully established, which was effective to amplify the specific gene fragments of S. mansoni within 20 min at 39 ℃. The minimum detectable limit of the fluorescent RAA assay was 10 copies/μL using recombinant plasmids as templates and 0.1 fg/μL using S. mansoni genomic DNA samples as templates. The fluorescent RAA assays were all negative for detecting the genomic DNA from S. japonicum, S. haematobium, A. duodenale and C. sinensis. Conclusions A novel fluorescent RAA assay is successfully established, which is simple, rapid, sensitive and specific to detect genomic DNA of S. mansoni.