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猪圆环病毒 2 型环介导等温扩增检测方法的建立。

Development of a loop-mediated isothermal amplification assay for porcine circovirus type 2.

机构信息

China Institute of Veterinary Drug Control, Beijing, China.

出版信息

Virol Sin. 2011 Jun;26(3):214-20. doi: 10.1007/s12250-011-3169-x. Epub 2011 Jun 12.

Abstract

In this study, the loop-mediated isothermal amplification (LAMP) method was used to develop a rapid and simple detection system for porcine circovirus type 2 (PCV2). According to the PCV2 sequences published in GenBank, multiple LAMP primers were designed targeting conserved sequences of PCV2. Using the DNA extracted from PCV2 isolates HUN-09 and SD-09 as the template, LAMP reactions in a PCV2 LAMP system was performed, the amplification products were detected by adding SYBR Green I and could be observed directly by the naked eye. The results showed highly-efficient and specific amplification in 30 min at 63°C with a LAMP real-time turbidimeter. Furthermore, PCV2 DNA templates, with a detection limit of 5.5×10(-5) ng of nucleic acid, indicated that this assay was highly sensitive. The results obtained with the naked eye after SYBR Green I staining were consistent with those detected by the real-time turbidimeter, showing the potential simplicity of interpretation of the assay results. The LAMP assay appeared to have greater accuracy than PCR and virus isolation for the analysis of 18 clinical samples. In addition it offers higher specificity and sensitivity, shorter reaction times and simpler procedures than the currently available methods of PCV2 detection. It is therefore a promising tool for the effective and efficient detection of PCV2.

摘要

在这项研究中,环介导等温扩增 (LAMP) 方法被用于开发一种快速简便的猪圆环病毒 2 型 (PCV2) 检测系统。根据 GenBank 中公布的 PCV2 序列,设计了多个针对 PCV2 保守序列的 LAMP 引物。使用从 PCV2 分离株 HUN-09 和 SD-09 中提取的 DNA 作为模板,在 PCV2 LAMP 系统中进行 LAMP 反应,通过添加 SYBR Green I 可以直接肉眼观察到扩增产物。结果表明,在 63°C 下 30 分钟内,LAMP 实时浊度计可以高效且特异性地扩增。此外,PCV2 DNA 模板的检测限为 5.5×10(-5)ng 核酸,表明该检测方法具有高度的灵敏性。SYBR Green I 染色后肉眼观察到的结果与实时浊度计检测到的结果一致,表明该检测方法的结果解释具有潜在的简单性。与 PCR 和病毒分离相比,该 LAMP 检测法在分析 18 个临床样本时具有更高的准确性。此外,与目前可用的 PCV2 检测方法相比,该方法具有更高的特异性和灵敏度、更短的反应时间和更简单的操作步骤。因此,它是一种有前途的有效检测 PCV2 的工具。

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