Research Center of Tropical and Infectious Diseases, Kerman University of Medical Sciences, Kerman, Iran.
Parasitol Res. 2013 Oct;112(10):3441-7. doi: 10.1007/s00436-013-3523-z. Epub 2013 Jul 7.
Reliable and rapid genotyping of large number of Echinococcus granulosus sensu lato isolates is crucial for understanding the epidemiology and transmission of cystic echinococcosis. We have developed a method for distinguishing and discriminating common genotypes of E. granulosus s.l. (G1, G3, and G6) in Iran. This method is based on polymerase chain reaction coupled with high resolution melting curve (HRM), ramping from 70 to 86 °C with fluorescence data acquisition set at 0.1 °C increments and continuous fluorescence monitoring. Consistency of this technique was assessed by inter- and intra-assays. Assessment of intra- and inter-assay variability showed low and acceptable coefficient of variations ranging from 0.09 to 0.17 %. Two hundred and eighty E. granulosus s.l. isolates from sheep, cattle, and camel were used to evaluate the applicability and accuracy of the method. The isolates were categorized as G1 (93, 94, and 25%), G3 (7, 4, and 4%), and G6 (0, 2, and 71%) for sheep, cattle, and camel, respectively. HRM results were completely compatible with those obtained from sequencing and rostellar hook measurement. This method proved to be a valuable screening tool for large-scale molecular epidemiological studies.
可靠且快速的大数量细粒棘球蚴(Echinococcus granulosus sensu lato)分离株基因分型对于了解包虫病的流行病学和传播至关重要。我们已经开发出一种在伊朗区分和鉴别常见细粒棘球蚴(E. granulosus s.l.)基因型(G1、G3 和 G6)的方法。该方法基于聚合酶链反应结合高分辨率熔解曲线(HRM),从 70°C 到 86°C 升温,荧光数据采集设置为 0.1°C 增量,连续荧光监测。通过内-和间试验评估了该技术的一致性。内-和间试验变异性评估显示,低且可接受的变异系数范围为 0.09 至 0.17%。使用 280 株来自绵羊、牛和骆驼的细粒棘球蚴 s.l. 分离株来评估该方法的适用性和准确性。这些分离株被归类为 G1(绵羊 93%、94%和 25%)、G3(绵羊 7%、牛 4%和 4%)和 G6(绵羊 0%、牛 2%和骆驼 71%)。HRM 结果与测序和棘球蚴钩测量的结果完全一致。该方法被证明是大规模分子流行病学研究的有价值的筛选工具。
