阿根廷东北部野外捕获的埃及伊蚊中登革热病毒的分子检测。

Domingo Javier Liotta, Gustavo Cabanne, Rodolfo Campos, Sergio Andrés Tonon
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引用次数: 0

摘要

迄今为止描述的大多数登革热病毒检测分子方案都是耗时且繁琐的蚊子样本。为了在阿根廷东北部现场捕获的埃及伊蚊种群中建立一个敏感和特异的分子检测系统,监测可能的登革热疫情和流行病毒血清型,开发了RT-PCR和RFLP测定方法。原Sudiro等人提出的人血清RT-PCR检测方法对蚊虫样本进行了优化。在RNA提取纯化和热剖面步骤中进行修饰。通过RFLP分析和循环测序验证了230 bp的扩增子。结果表明,由于所使用引物的共性,某些蚊子基因组区域可以被共扩增,因此通过RFLP分析确定登革热特异性扩增子是必要的步骤。在这些条件下,所提出的方法可作为埃及伊蚊样本中登革热病毒的通用筛选程序,估计99.52%的确诊阴性(207/208个检测样本)由我们掌握。
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Molecular detection of dengue viruses in field caught Aedes aegypti mosquitoes from northeastern Argentina.

Most molecular protocols for Dengue virus detection described so far are time consuming and cumbersome with mosquito samples. In order to count with a sensitive and specific molecular detection system for monitoring possible Dengue outbreaks and circulating viral serotypes in field-caught Aedes aegypti populations from Northeastern Argentina, a RT-PCR and RFLP assay was developed. The original RT-PCR assay proposed by Sudiro et al. for human serum was optimized for mosquito samples. Modifications were done at the RNA extraction-purification and at the thermal profile steps. The generic 230 bp amplicon was validated by RFLP assay and cycle sequencing. Results showed that, due to the generic characteristic of the primers used, certain mosquito genome regions could be co-amplified, making confirmation of the Dengue specific amplicon by RFLP assay a required step. Under these conditions, the proposed method can be employed as a Dengue viral generic screening procedure in Aedes aegypti mosquito samples, giving in our hands an estimated 99.52% of confirmed negatives (207/208 tested samples).

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