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用于同时检测诺如病毒并进行基因分型的DNA微阵列的研发。

Development of a DNA microarray for the simultaneous detection and genotyping of noroviruses.

作者信息

Pagotto Franco, Corneau Nathalie, Mattison Kirsten, Bidawid Sabah

机构信息

Microbiology Research Division, Bureau of Microbial Hazards, Food Directorate, Health Products and Food Branch, Health Canada, Sir FG Banting Research Centre, P.L. 2204E, Ottawa, Ontario, Canada.

出版信息

J Food Prot. 2008 Jul;71(7):1434-41. doi: 10.4315/0362-028x-71.7.1434.

Abstract

Current methods for detecting and genotyping noroviruses focus on the use of reverse transcriptase (RT)-mediated PCR. A major drawback of this approach is that short target RT-PCR products do not always encompass sequences that can be compared among research laboratories, resulting in difficulties for molecular epidemiology. We describe the use of a microarray-based system for simultaneous detection and molecular characterization of noroviruses. The protocol generates a 917-bp RT-PCR product that encompasses two major regions currently used for detection and analysis of norovirus genomes. The PCR products are then hybridized to an oligonucleotide array (NoroChip) based on 50-mer features, which allows for both confirmation of reaction specificity and molecular characterization of the amplified genome. Parallel sequence analyses of amplicons revealed that our microarray data were robust in separating genogroups I and II, and further subtyping to the cluster level was possible. This approach, combining detection and characterization, overcomes the need for expensive and time-consuming sequence analysis of amplified genome targets for molecular epidemiology.

摘要

目前检测诺如病毒并进行基因分型的方法主要集中在使用逆转录酶(RT)介导的PCR。这种方法的一个主要缺点是,短的目标RT-PCR产物并不总是包含可在研究实验室之间进行比较的序列,这给分子流行病学研究带来了困难。我们描述了一种基于微阵列的系统,用于同时检测诺如病毒并进行分子特征分析。该方案产生一个917bp的RT-PCR产物,其包含目前用于检测和分析诺如病毒基因组的两个主要区域。然后将PCR产物与基于50聚体特征的寡核苷酸阵列(NoroChip)杂交,这既可以确认反应特异性,又可以对扩增的基因组进行分子特征分析。对扩增子的平行序列分析表明,我们的微阵列数据在区分基因群I和II方面很可靠,并且进一步细分到簇水平也是可能的。这种将检测和特征分析相结合的方法,克服了分子流行病学中对扩增基因组靶点进行昂贵且耗时的序列分析的需求。

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