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全基因组测序可识别 H3N2 流感病毒的传播,并提供比传统分型方法更高的分辨率。

Whole genome sequencing identifies influenza A H3N2 transmission and offers superior resolution to classical typing methods.

机构信息

Bavarian Health and Food Safety Authority, Veterinärstraße 2, 85764, Oberschleißheim, Germany.

出版信息

Infection. 2018 Feb;46(1):69-76. doi: 10.1007/s15010-017-1091-3. Epub 2017 Oct 31.

Abstract

OBJECTIVES

Influenza with its annual epidemic waves is a major cause of morbidity and mortality worldwide. However, only little whole genome data are available regarding the molecular epidemiology promoting our understanding of viral spread in human populations.

METHODS

We implemented a RT-PCR strategy starting from patient material to generate influenza A whole genome sequences for molecular epidemiological surveillance. Samples were obtained within the Bavarian Influenza Sentinel. The complete influenza virus genome was amplified by a one-tube multiplex RT-PCR and sequenced on an Illumina MiSeq.

RESULTS

We report whole genomic sequences for 50 influenza A H3N2 viruses, which was the predominating virus in the season 2014/15, directly from patient specimens. The dataset included random samples from Bavaria (Germany) throughout the influenza season and samples from three suspected transmission clusters. We identified the outbreak samples based on sequence identity. Whole genome sequencing (WGS) was superior in resolution compared to analysis of single segments or partial segment analysis. Additionally, we detected manifestation of substantial amounts of viral quasispecies in several patients, carrying mutations varying from the dominant virus in each patient.

CONCLUSION

Our rapid whole genome sequencing approach for influenza A virus shows that WGS can effectively be used to detect and understand outbreaks in large communities. Additionally, the genomic data provide in-depth details about the circulating virus within one season.

摘要

目的

流感每年都会形成流行浪潮,是造成全球发病和死亡的主要原因。然而,关于促进我们了解病毒在人群中传播的分子流行病学的整个基因组数据非常有限。

方法

我们实施了一种 RT-PCR 策略,从患者标本开始生成流感 A 全基因组序列,进行分子流行病学监测。标本来自巴伐利亚流感监测哨点。通过单管多重 RT-PCR 扩增完整的流感病毒基因组,并在 Illumina MiSeq 上进行测序。

结果

我们报告了 50 株流感 A H3N2 病毒的全基因组序列,这是 2014/15 季节中占主导地位的病毒,直接从患者标本中获得。该数据集包括流感季节期间来自巴伐利亚(德国)的随机样本以及来自三个疑似传播集群的样本。我们根据序列同一性确定了暴发样本。全基因组测序(WGS)在分辨率方面优于单个片段或部分片段分析。此外,我们在几个患者中检测到大量病毒准种的表现,每个患者携带的突变与主要病毒不同。

结论

我们用于流感 A 病毒的快速全基因组测序方法表明,WGS 可有效用于检测和了解大型社区中的暴发情况。此外,基因组数据提供了一个季节内循环病毒的详细信息。

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