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A Loop-Mediated Isothermal Amplification (LAMP) Assay for Strongyloides stercoralis in Stool That Uses a Visual Detection Method with SYTO-82 Fluorescent Dye

机译:使用视觉检测方法和SYTO-82荧光染料的粪便中圆线虫类固醇的环介导等温扩增(LAMP)分析

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摘要

An assay to detect Strongyloides stercoralis in stool specimens was developed using the loop-mediated isothermal amplification (LAMP) method. Primers were based on the 28S ribosomal subunit gene. The reaction conditions were optimized and SYTO-82 fluorescent dye was used to allow real-time and visual detection of the product. The product identity was confirmed with restriction enzyme digestion, cloning, and sequence analysis. The assay was specific when tested against DNA from bacteria, fungi and parasites, and 30 normal stool samples. Analytical sensitivity was to < 10 copies of target sequence in a plasmid and up to a 10-2 dilution of DNA extracted from a Strongyloides ratti larva spiked into stool. Sensitivity was increased when further dilutions were made in water, indicative of reduced reaction inhibition. Twenty-seven of 28 stool samples microscopy and polymerase chain reaction positive for S. stercoralis were positive with the LAMP method. On the basis of these findings, the assay warrants further clinical validation.
机译:使用环介导的等温扩增(LAMP)方法开发了一种检测粪便标本中甾体类固线虫的方法。引物基于28S核糖体亚基基因。优化了反应条件,并使用SYTO-82荧光染料对产品进行实时和视觉检测。通过限制性内切酶消化,克隆和序列分析确认产物的同一性。当针对细菌,真菌和寄生虫以及30个正常粪便样本的DNA进行测试时,该检测方法具有特异性。分析灵敏度是对质粒中目标序列的<10个拷贝和从掺入粪便中的拟南芥(Strongyloides ratti)幼虫中提取的DNA的最高10 -2 稀释度。当在水中进一步稀释时,灵敏度增加,表明减少了反应抑制。 28个粪便样品中有27个在显微镜下显示为阳性,而SAMP阳性的聚合酶链反应在LAMP方法中为阳性。基于这些发现,该测定法值得进一步的临床验证。

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