Tantrawatpan Chairat, Intapan Pewpan M, Thanchomnang Tongjit, Sanpool Oranuch, Janwan Penchom, Boonmars Thidarut, Morakote Nimit, Maleewong Wanchai
1 Research and Diagnostic Center for Emerging Infectious Diseases, Khon Kaen University , Khon Kaen, Thailand .
Vector Borne Zoonotic Dis. 2013 Sep;13(9):674-81. doi: 10.1089/vbz.2012.1221. Epub 2013 Jun 29.
Real-time fluorescence resonance energy transfer (FRET) PCR and melting curve analysis using newly developed fluorophore-labeled hybridization probes were applied for the detection of Trichinella spiralis DNA in muscle of mice following oral inoculation with 300 T. spiralis larvae. The developed assay could detect and differentiate T. spiralis, Trichinella papuae, and Trichinella pseudospiralis DNAs by the different melting temperatures (Tm). The assay had a detection limit of 5 × 10(2) positive control plasmid copies, which was equivalent to 1 ng of T. spiralis DNA spiked into 250 mg of muscle sample. No fluorescence signal was detected when the technique was applied to the DNA of 27 parasites other than Trichinella spp. The assay could detect T. spiralis DNA in muscle at 7, 14, and 21 days postinoculation. The range, mean ± standard deviation, and median of the Tm values of all positive muscle tissue samples were 60.4-60.8, 60.6 ± 0.2, and 60.5, respectively. This assay provides an effective tool for the specific, sensitive, and high-throughput detection of T. spiralis DNA in muscle during the early stage of infection. In addition, the technique can be useful for epidemiologic surveillance in naturally infected wildlife.
运用新开发的荧光团标记杂交探针进行实时荧光共振能量转移(FRET)聚合酶链反应(PCR)和熔解曲线分析,以检测经口接种300条旋毛虫幼虫的小鼠肌肉中的旋毛虫DNA。所开发的检测方法能够通过不同的熔解温度(Tm)检测并区分旋毛虫、巴布亚旋毛虫和伪旋毛虫的DNA。该检测方法的检测限为5×10²个阳性对照质粒拷贝,相当于掺入250mg肌肉样品中的1ng旋毛虫DNA。当该技术应用于旋毛虫属以外的27种寄生虫的DNA时,未检测到荧光信号。该检测方法能够在接种后7天、14天和21天检测到肌肉中的旋毛虫DNA。所有阳性肌肉组织样品的Tm值范围、平均值±标准差和中位数分别为60.4 - 60.8、60.6±0.2和60.5。该检测方法为感染早期肌肉中旋毛虫DNA的特异性、灵敏性和高通量检测提供了一种有效工具。此外,该技术可用于自然感染野生动物的流行病学监测。
