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dc.contributor.authorTrend, S.
dc.contributor.authorChang, B.J.
dc.contributor.authorO'Dea, M.
dc.contributor.authorStick, S.M.
dc.contributor.authorKicic, Anthony
dc.date.accessioned2019-11-09T20:31:23Z
dc.date.available2019-11-09T20:31:23Z
dc.date.issued2018
dc.identifier.citationTrend, S. and Chang, B.J. and O'Dea, M. and Stick, S.M. and Kicic, A. 2018. Use of a primary epithelial cell screening tool to investigate phage therapy in cystic fibrosis. Frontiers in Pharmacology. 9 (NOV): ARTN 1330.
dc.identifier.urihttp://hdl.handle.net/20.500.11937/76773
dc.identifier.doi10.3389/fphar.2018.01330
dc.description.abstract

© 2007 - 2018 Frontiers Media S.A. All Rights Reserved. Antimicrobial-resistant microbes are an increasing threat to human health. In cystic fibrosis (CF), airway infections with Pseudomonas aeruginosa remain a key driver of lung damage. With few new antibiotics on the development horizon, alternative therapeutic approaches are needed against antimicrobial-resistant pathogens. Phage therapy, or the use of viruses that infect bacteria, is one proposed novel therapy to treat bacterial infections. However, the airways are complex microenvironments with unique characteristics that may affect the success of novel therapies. Here, three phages of P. aeruginosa (E79, F116, and one novel clinically derived isolate, designated P5) were screened for activity against 21 P. aeruginosa strains isolated from children with CF. Of these, phage E79 showed broad antibacterial activity (91% of tested strains sensitive) and was selected for further assessment. E79 genomic DNA was extracted, sequenced, and confirmed to contain no bacterial pathogenicity genes. High titre phage preparations were then purified using ion-exchange column chromatography and depleted of bacterial endotoxin. Primary airway epithelial cells derived from children with CF (n = 8, age range 0.2-5.5 years, 5 males) or healthy non-CF controls (n = 8, age range 2.5-4.0 years, 4 males) were then exposed to purified phage for 48 h. Levels of inflammatory IL-1β, IL-6, and IL-8 cytokine production were measured in culture supernatant by immunoassays and the extent of cellular apoptosis was measured using a ssDNA kit. Cytokine and apoptosis levels were compared between E79-stimulated and unstimulated controls, and, encouragingly, purified preparations of E79 did not stimulate any significant inflammatory cytokine responses or induce apoptosis in primary epithelial cells derived from children with or without CF. Collectively, this study demonstrates the feasibility of utilizing pre-clinical in vitro culture models to screen therapeutic candidates, and the potential of E79 as a therapeutic phage candidate in CF.

dc.languageEnglish
dc.publisherFRONTIERS MEDIA SA
dc.rights.urihttp://creativecommons.org/licenses/by/4.0/
dc.subjectScience & Technology
dc.subjectLife Sciences & Biomedicine
dc.subjectPharmacology & Pharmacy
dc.subjectcystic fibrosis
dc.subjectphage therapy
dc.subjectpreclinical models
dc.subjectairway epithelial cells
dc.subjectPseudomonas aeruginosa
dc.subjectinfection
dc.subjectPSEUDOMONAS-AERUGINOSA
dc.subjectBACTERIOPHAGE
dc.subjectCHILDREN
dc.subjectAIRWAY
dc.subjectINFLAMMATION
dc.subjectINFECTION
dc.subjectBIOFILMS
dc.subjectEFFICACY
dc.subjectDELIVERY
dc.subjectINFANTS
dc.titleUse of a primary epithelial cell screening tool to investigate phage therapy in cystic fibrosis
dc.typeJournal Article
dcterms.source.volume9
dcterms.source.numberNOV
dcterms.source.issn1663-9812
dcterms.source.titleFrontiers in Pharmacology
dc.date.updated2019-11-09T20:31:18Z
curtin.departmentSchool of Public Health
curtin.accessStatusOpen access
curtin.facultyFaculty of Health Sciences
curtin.contributor.orcidKicic, Anthony [0000-0002-0008-9733]
curtin.identifier.article-numberARTN 1330
dcterms.source.eissn1663-9812
curtin.contributor.scopusauthoridKicic, Anthony [6507472922]


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