RNA Viruses Section, Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases, National Institutes of Health, Bethesda, Maryland, United States of America.
Institut für Mikrobiologie, Technische Universität Braunschweig, Braunschweig, Germany.
PLoS Pathog. 2019 Aug 5;15(8):e1007963. doi: 10.1371/journal.ppat.1007963. eCollection 2019 Aug.
Human respiratory syncytial virus (RSV) is the leading viral cause of acute pediatric lower respiratory tract infections worldwide, with no available vaccine or effective antiviral drug. To gain insight into virus-host interactions, we performed a genome-wide siRNA screen. The expression of over 20,000 cellular genes was individually knocked down in human airway epithelial A549 cells, followed by infection with RSV expressing green fluorescent protein (GFP). Knockdown of expression of the cellular ATP1A1 protein, which is the major subunit of the Na+,K+-ATPase of the plasma membrane, had one of the strongest inhibitory effects on GFP expression and viral titer. Inhibition was not observed for vesicular stomatitis virus, indicating that it was RSV-specific rather than a general effect. ATP1A1 formed clusters in the plasma membrane very early following RSV infection, which was independent of replication but dependent on the attachment glycoprotein G. RSV also triggered activation of ATP1A1, resulting in signaling by c-Src-kinase activity that transactivated epidermal growth factor receptor (EGFR) by Tyr845 phosphorylation. ATP1A1 signaling and activation of both c-Src and EGFR were found to be required for efficient RSV uptake. Signaling events downstream of EGFR culminated in the formation of macropinosomes. There was extensive uptake of RSV virions into macropinosomes at the beginning of infection, suggesting that this is a major route of RSV uptake, with fusion presumably occurring in the macropinosomes rather than at the plasma membrane. Important findings were validated in primary human small airway epithelial cells (HSAEC). In A549 cells and HSAEC, RSV uptake could be inhibited by the cardiotonic steroid ouabain and the digitoxigenin derivative PST2238 (rostafuroxin) that bind specifically to the ATP1A1 extracellular domain and block RSV-triggered EGFR Tyr845 phosphorylation. In conclusion, we identified ATP1A1 as a host protein essential for macropinocytic entry of RSV into respiratory epithelial cells, and identified PST2238 as a potential anti-RSV drug.
人类呼吸道合胞病毒(RSV)是全球导致小儿急性下呼吸道感染的主要病毒病原体,目前尚无可用的疫苗或有效的抗病毒药物。为了深入了解病毒-宿主相互作用,我们进行了全基因组 siRNA 筛选。我们在人呼吸道上皮 A549 细胞中单独敲低了超过 20000 种细胞基因的表达,然后用表达绿色荧光蛋白(GFP)的 RSV 感染这些细胞。细胞内 ATP1A1 蛋白的表达被敲低后,对 GFP 表达和病毒滴度有最强的抑制作用之一。然而,这种抑制作用不会出现在水疱性口炎病毒中,这表明它是 RSV 特异性的,而不是一般的作用。在 RSV 感染后,ATP1A1 很快就在质膜上形成簇,这一过程独立于复制,但依赖于附着糖蛋白 G。RSV 还触发了 ATP1A1 的激活,导致 c-Src-激酶活性的信号转导,通过 Tyr845 磷酸化使表皮生长因子受体(EGFR)反式激活。发现 ATP1A1 信号转导和 c-Src 和 EGFR 的激活对于 RSV 的有效摄取都是必需的。EGFR 下游的信号转导事件最终导致大吞噬体的形成。在感染初期,大量 RSV 病毒颗粒被内化到大吞噬体中,这表明这是 RSV 摄取的主要途径,融合可能发生在大吞噬体中,而不是在质膜上。这些重要发现已在原代人小气道上皮细胞(HSAEC)中得到验证。在 A549 细胞和 HSAEC 中,RSV 的摄取可以被强心甾类化合物哇巴因和地高辛衍生物 PST2238(罗司伐星)抑制,这两种化合物特异性结合 ATP1A1 细胞外结构域并阻断 RSV 触发的 EGFR Tyr845 磷酸化。总之,我们确定 ATP1A1 是一种宿主蛋白,对于 RSV 进入呼吸道上皮细胞的巨吞饮进入是必需的,并且确定 PST2238 是一种潜在的抗 RSV 药物。
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