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Co-infection with Staphylococcus aureus after primary influenza virus infection leads to damage of the endothelium in a human alveolus-on-a-chip model

金黄色葡萄球菌 毒力 生物 发病机制 免疫系统 病菌 微生物学 免疫学 病毒 体外 势垒函数 细胞生物学 细菌 遗传学 生物化学 基因
作者
Stefanie Deinhardt‐Emmer,Knut Rennert,Elisabeth Schicke,Zoltán Cseresnyés,Maximilian Windolph,Sándor Nietzsche,Regine Heller,Fatina Siwczak,Karoline Frieda Haupt,Swen Carlstedt,Michael Schacke,Marc Thilo Figge,Christina Ehrhardt,Bettina Löffler,Alexander S. Mosig
出处
期刊:Biofabrication [IOP Publishing]
卷期号:12 (2): 025012-025012 被引量:75
标识
DOI:10.1088/1758-5090/ab7073
摘要

Abstract Pneumonia is one of the most common infectious diseases worldwide. The influenza virus can cause severe epidemics, which results in significant morbidity and mortality. Beyond the virulence of the virus itself, epidemiological data suggest that bacterial co-infections are the major cause of increased mortality. In this context, Staphylococcus aureus represents a frequent causative bacterial pathogen. Currently available models have several limitations in the analysis of the pathogenesis of infections, e.g. some bacterial toxins strongly act in a species-specific manner. Human 2D mono-cell culture models often fail to maintain the differentiation of alveolus-specific functions. A detailed investigation of the underlying pathogenesis mechanisms requires a physiological interaction of alveolus-specific cell types. The aim of the present work was to establish a human in vitro alveolus model system composed of vascular and epithelial cell structures with cocultured macrophages resembling the human alveolus architecture and functions. We demonstrate that high barrier integrity maintained for up to 14 d in our model containing functional tissue-resident macrophages. We show that flow conditions and the presence of macrophages increased the barrier function. The infection of epithelial cells induced a high inflammatory response that spread to the endothelium. Although the integrity of the epithelium was not compromised by a single infection or co-infection, we demonstrated significant endothelial cell damage associated with loss of barrier function. We established a novel immune-responsive model that reflects the complex crosstalk between pathogens and host. The in vitro model allows for the monitoring of spatiotemporal spreading of the pathogens and the characterization of morphological and functional alterations attributed to infection. The alveolus-on-a-chip represents a promising platform for mechanistic studies of host-pathogen interactions and the identification of molecular and cellular targets of novel treatment strategies in pneumonia.
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