A three-dimensional A549 cell culture model to study respiratory syncytial virus infections

dc.contributor.authorSaleh, Fatima A.
dc.contributor.authorHarb, Aya
dc.contributor.authorSoudani, Nadia Y.
dc.contributor.authorZaraket, Hassan
dc.contributor.departmentExperimental Pathology, Microbiology, and Immunology
dc.contributor.facultyFaculty of Medicine (FM)
dc.contributor.institutionAmerican University of Beirut
dc.date.accessioned2025-01-24T11:39:05Z
dc.date.available2025-01-24T11:39:05Z
dc.date.issued2020
dc.description.abstractBackground: Respiratory syncytial virus (RSV) is a primary cause of morbidity and mortality worldwide, affecting infants, young children, and immune-compromised patients; however, currently no vaccine is available for prevention of RSV infections. The overwhelming majority of our knowledge of how RSV causes infection is based upon studies that have been carried out using traditional 2D methods, with cells cultured on flat plastic dishes. Although these simplified culture systems are essential to gain an insight into the fundamentals of host-pathogen interactions, cells in 2D are not exposed to the same conditions as cells in 3D tissues in the body and are therefore a poor representation of thein vivo microenvironment. In this study, we aim to develop the first 3D culture model for RSV infection using A549 cells to test its utility for RSV pathogenesis. Methods: To generate spheroids, A549 cells were cultured using ultra-low attachment plates to generate 25 × 103 cell spheroids. The viability of the spheroids was assessed by trypan blue exclusion assay and flow cytometry showing prominent live cells throughout the spheroids confirming high viability over seven days of incubation. Results: Immunostaining of A549 spheroids inoculated with RSV, showed time-dependent dissemination of the viral antigen RSV-F within the spheroid, resulting in syncytia formation and a 3-fold increase in mucin secretion compared to the uninfected cells. Additionally, RSV successfully replicated in the spheroids producing infectious virus as early as day one post-inoculation and was sustained for up to 7 days post-inoculation. Conclusions: Results show that A549 spheroids are susceptible and permissive for RSV since they exhibit the characteristics of RSV infection including syncytia formation and mucin overexpression, suggesting that A549 spheroids can be used a promising model for studying RSV in vitro. © 2020 The Authors
dc.identifier.doihttps://doi.org/10.1016/j.jiph.2020.03.011
dc.identifier.eid2-s2.0-85084067734
dc.identifier.pmid32360024
dc.identifier.urihttp://hdl.handle.net/10938/29170
dc.language.isoen
dc.publisherElsevier Ltd
dc.relation.ispartofJournal of Infection and Public Health
dc.sourceScopus
dc.subject3d culture
dc.subjectA549
dc.subjectInfection
dc.subjectMucin
dc.subjectRespiratory syncytial virus (rsv)
dc.subjectA549 cells
dc.subjectAnimals
dc.subjectCell culture techniques
dc.subjectChlorocebus aethiops
dc.subjectHumans
dc.subjectIn vitro techniques
dc.subjectRespiratory syncytial virus infections
dc.subjectRespiratory syncytial virus, human
dc.subjectVero cells
dc.subjectMucin 1
dc.subjectTrypan blue
dc.subjectVirus antigen
dc.subjectA-549 cell line
dc.subjectAnimal cell
dc.subjectAnimal tissue
dc.subjectArticle
dc.subjectCell count
dc.subjectCell viability
dc.subjectCell viability assay
dc.subjectControlled study
dc.subjectData analysis software
dc.subjectFlow cytometry
dc.subjectHuman
dc.subjectHuman respiratory syncytial virus
dc.subjectImmunohistochemistry
dc.subjectNonhuman
dc.subjectPlaque assay
dc.subjectPriority journal
dc.subjectProtein expression
dc.subjectRespiratory syncytial virus infection
dc.subjectSpheroid cell
dc.subjectSyncytium
dc.subjectThree dimensional cell culture
dc.subjectTrypan blue exclusion assay
dc.subjectVirus infectivity
dc.subjectVirus replication
dc.subjectAnimal
dc.subjectCell culture technique
dc.subjectIn vitro study
dc.subjectPathology
dc.subjectVero cell line
dc.titleA three-dimensional A549 cell culture model to study respiratory syncytial virus infections
dc.typeArticle

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