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Culturing of respiratory viruses in well‐differentiated pseudostratified human airway epithelium as a tool to detect unknown viruses

机译:在分化良好的伪分层人气道上皮细胞中培养呼吸道病毒,作为检测未知病毒的工具

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AbstractBackgroundCurrently, virus discovery is mainly based on molecular techniques. Here, we propose a method that relies on virus culturing combined with state-of-the-art sequencing techniques. The most natural ex vivo culture system was used to enable replication of respiratory viruses.MethodThree respiratory clinical samples were tested on well-differentiated pseudostratified tracheobronchial human airway epithelial (HAE) cultures grown at an air–liquid interface, which resemble the airway epithelium. Cells were stained with convalescent serum of the patients to identify infected cells and apical washes were analyzed by VIDISCA-454, a next-generation sequencing virus discovery technique.ResultsInfected cells were observed for all three samples. Sequencing subsequently indicated that the cells were infected by either human coronavirus OC43, influenzavirus B, or influenzavirus A. The sequence reads covered a large part of the genome (52%, 82%, and 57%, respectively).ConclusionWe present here a new method for virus discovery that requires a virus culture on primary cells and an antibody detection. The virus in the harvest can be used to characterize the viral genome sequence and cell tropism, but also provides progeny virus to initiate experiments to fulfill the Koch's postulates.
机译:摘要背景技术当前,病毒发现主要基于分子技术。在这里,我们提出了一种依靠病毒培养与最新测序技术相结合的方法。方法使用最自然的离体培养系统来复制呼吸道病毒。方法对三种呼吸道临床样品在气液界面上生长的高分化假分层气管支气管人气道上皮(HAE)培养物中进行测试,该培养物类似于气道上皮。用患者的恢复期血清对细胞进行染色,以鉴定感染的细胞,并通过下一代测序病毒发现技术VIDISCA-454分析根尖洗液。结果在所有三个样品中均观察到感染的细胞。随后的测序表明该细胞已被人冠状病毒OC43,流感病毒B或流感病毒A感染。该序列读码覆盖了基因组的很大一部分(分别为52%,82%和57%)。一种发现病毒的方法,需要在原代细胞上进行病毒培养并进行抗体检测。收获物中的病毒可用于表征病毒基因组序列和细胞嗜性,但也可提供子代病毒来启动实验,以完成科赫的假设。

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