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Simple and Rapid Visual Detection Methods of Orf Virus by B2L Gene based Loop-Mediated Isothermal Amplification Assay

机译:基于B2L基因的环介导等温扩增法简便快速地检测Orf病毒

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Comparison of three different visual detection methods namely the presence of turbidity, color change due to addition of SYBR green I and hydroxynaphthol blue has been studied for a loop-mediated isothermal amplification assay (LAMP) in rapid diagnosis of orf virus as an alternate to gel based analysis. This orf virus specific LAMP assay targeted the amplification of B2L gene sequence of the virus genome and shown specific amplification within 45 min at 60oC without any cross reactivity to other viruses of sheep and goats. Analytical specificity and sensitivity of the assay were evaluated by these visual detection methods and positive detection rates by LAMP and PCR assays over testing of clinical samples and cell culture adapted virus isolates were determined. B2L LAMP assay detected thirty-five (85.3%) samples, whereas the conventional PCR shown only thirty-three (80.5%) samples as positive from a total of forty one clinical samples tested. On analysis of these thirty five positive samples by three visual detection methods, it is found that HNB and SYBR green I dyes are equally sensitive (100%) and higher compared to turbidity method (94%) of monitoring the LAMP reaction. Use of HNB dye in B2L LAMP assay will be affordable in terms of cost involved and ease of visualization and can suit the less equipped field laboratories for rapid clinical diagnosis of orf virus in sheep and goats.
机译:已经研究了三种不同视觉检测方法的比较,即浊度的存在,由于添加了SYBR绿I和羟基萘酚蓝而引起的颜色变化,用于回路介导的等温扩增测定(LAMP),可快速诊断orf病毒,以替代凝胶基于分析。这项orf病毒特异性LAMP分析法靶向扩增病毒基因组的B2L基因序列,并在60oC下45分钟内显示出特异性扩增,而与绵羊和山羊的其他病毒没有任何交叉反应性。通过这些视觉检测方法评估了分析的特异性和敏感性,并通过LAMP和PCR分析对临床样品进行了检测,从而确定了阳性检测率,并确定了适合细胞培养的病毒分离株。 B2L LAMP分析检测到三十五个(85.3%)样品,而常规PCR显示在总共四十一个临床样品中仅三十三个(80.5%)样品为阳性。通过三种视觉检测方法对这35个阳性样品进行分析,发现HNB和SYBR green I染料对LAMP反应的监测具有同等敏感性(100%)和高于浊度法(94%)。就所涉及的成本和易于观察而言,在B2L LAMP分析中使用HNB染料将是负担得起的,并且可以满足装备不足的野外实验室对绵羊和山羊中orf病毒的快速临床诊断的需要。

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