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Differentiated swine airway epithelial cell cultures for the investigation of influenza A virus infection and replication

机译:分化的猪气道上皮细胞培养物用于研究甲型流感病毒的感染和复制

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AbstractPlease cite this paper as: Bateman et al. (2013) Differentiated swine airway epithelial cell cultures for the investigation of influenza A virus infection and replication. Influenza and Other Respiratory Viruses 7(2) 139–150.Background  Differentiated human airway epithelial cell cultures have been utilized to investigate cystic fibrosis, wound healing, and characteristics of viral infections. These cultures, grown at an air–liquid interface (ALI) in media with defined hormones and growth factors, recapitulate many aspects of the in vivo respiratory tract and allow for experimental studies at the cellular level.Objectives  To optimize growth conditions for differentiated swine airway epithelial cultures and to use these cultures to examine influenza virus infection and replication.Methods  Primary swine respiratory epithelial cells were grown at an air–liquid interface with varying amounts of retinoic acid and epidermal growth factor. Cells grown with optimized concentrations of these factors for 4 weeks differentiated into multilayer epithelial cell cultures resembling the lining of the swine respiratory tract. Influenza virus infection and replication were examined in these cultures.Results/Conclusions  Retinoic acid promoted ciliogenesis, whereas epidermal growth factor controlled the thickness of the pseudoepithelium. The optimal concentrations for differentiated swine cell cultures were 1·5 ng/ml epidermal growth factor and 100 nm retinoic acid. Influenza A viruses infected and productively replicated in these cultures in the absence of exogenous trypsin, suggesting that the cultures express a protease capable of activating influenza virus hemagglutinin. Differences in virus infection and replication characteristics found previously in pigs in vivo were recapitulated in the swine cultures. This system could be a useful tool for a range of applications, including investigating influenza virus species specificity, defining cell tropism of influenza viruses in the swine respiratory epithelium, and studying other swine respiratory diseases.
机译:摘要请以Bateman等人的身份引用本文。 (2013)分化的猪气道上皮细胞培养物,用于研究甲型流感病毒的感染和复制。流行性感冒和其他呼吸道病毒7(2)139–150。背景分化的人类气道上皮细胞培养物已用于研究囊性纤维化,伤口愈合和病毒感染的特征。这些培养物在气液界面(ALI)上生长在具有确定的激素和生长因子的培养基中,概括了体内呼吸道的许多方面,并允许在细胞水平上进行实验研究。目的优化分化猪呼吸道的生长条件方法:原代猪呼吸道上皮细胞在气液界面上生长,视黄酸和表皮生长因子的含量各不相同。在这些因子的优化浓度下生长的细胞持续4周分化为类似于猪呼吸道内膜的多层上皮细胞培养物。在这些培养物中检查了流感病毒的感染和复制。结果/结论维甲酸可促进纤毛发生,而表皮生长因子控制假上皮的厚度。分化的猪细胞培养物的最佳浓度为1·5 ng / ml表皮生长因子和100 nm视黄酸。在没有外源胰蛋白酶的情况下,在这些培养物中感染并生产性复制的甲型流感病毒表明该培养物表达的蛋白酶能够激活流感病毒血凝素。先前在猪体内发现的病毒感染和复制特性差异在猪培养物中得以概括。该系统对于一系列应用可能是有用的工具,包括研究流感病毒种类的特异性,确定猪呼吸道上皮中流感病毒的细胞嗜性,以及研究其他猪呼吸道疾病。

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