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Author Notes:

Luke Garratt, Wal‐Yan Respiratory Research Centre, Telethon Kids Institute, University of Western Australia, Nedlands, WA, Australia. Email: luke.garratt@telethonkids.org.au

Daniel R Laucirica: Conceptualization; Formal analysis; Investigation; Methodology; Writing – original draft; Writing – review and editing. Craig J Schofield: Investigation; Methodology; Writing – review and editing. Samantha A McLean: Investigation; Methodology; Writing – review and editing. Camilla Margaroli: Methodology; Writing – review and editing. Patricia Agudelo‐Romero: Formal analysis; Methodology; Writing – review and editing. Stephen M Stick: Supervision; Writing – review and editing. Rabindra Tirouvanziam: Methodology; Writing – review and editing. Anthony Kicic: Conceptualization; Supervision; Writing – original draft; Writing – review and editing. Luke W Garratt: Conceptualization; Methodology; Supervision; Writing – original draft; Writing – review and editing.

We thank the families, participants and staff of WAERP, AREST and PEARSS. Open access publishing facilitated by The University of Western Australia, as part of the Wiley–The University of Western Australia agreement via the Council of Australian University Librarians.

The authors declare no competing interests.

Subject:

Research Funding:

This study was supported by NHMRC project grant 1142505 and a Telethon Kids Institute Plus 10 Award.

SMS is a NHMRC Practitioner Fellow, AK is a Rothwell Family Fellow and LWG is a NHMRC Early Career Fellow (1141479).

CM is supported by a Cystic Fibrosis Foundation: Research Development Program Grant ROWE19R0.

DRL is funded by a Scholarship for International Research Fees and an Ad Hoc Postgraduate Scholarship through the University of Western Australia, as well as a Stan and Jean Perron Top Up Scholarship through Telethon Kids Institute.

This study was authored on behalf of WAERP (walyanrespirato‐ry.telethonkids.org.au/projects/WAERP/) and AREST CF (arestcf.telethonkids.org.au).

Keywords:

  • Science & Technology
  • Life Sciences & Biomedicine
  • Cell Biology
  • Immunology
  • Airway epithelium
  • cystic fibrosis
  • innate immunity
  • neutrophils
  • Pseudomonas
  • rhinovirus
  • SMALL-MOLECULE INHIBITOR
  • CYSTIC-FIBROSIS
  • HUMAN RHINOVIRUS
  • NLRP3 INFLAMMASOME
  • EPITHELIAL-CELLS
  • YOUNG-CHILDREN
  • ACTIVATION
  • LUNG
  • BIOMARKERS
  • SECRETION

Pseudomonas aeruginosa modulates neutrophil granule exocytosis in an in vitro model of airway infection

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Journal Title:

IMMUNOLOGY AND CELL BIOLOGY

Volume:

Volume 100, Number 5

Publisher:

, Pages 352-370

Type of Work:

Article | Final Publisher PDF

Abstract:

A population of neutrophils recruited into cystic fibrosis (CF) airways is associated with proteolytic lung damage, exhibiting high expression of primary granule exocytosis marker CD63 and reduced phagocytic receptor CD16. Causative factors for this population are unknown, limiting intervention. Here we present a laboratory model to characterize responses of differentiated airway epithelium and neutrophils following respiratory infection. Pediatric primary airway epithelial cells were cultured at the air–liquid interface, challenged individually or in combination with rhinovirus (RV) and Pseudomonas aeruginosa, then apically washed with medical saline to sample epithelial infection milieus. Cytokine multiplex analysis revealed epithelial antiviral signals, including IP-10 and RANTES, increased with exclusive RV infection but were diminished if P. aeruginosa was also present. Proinflammatory signals interleukin-1α and β were dominant in P. aeruginosa infection milieus. Infection washes were also applied to a published model of neutrophil transmigration into the airways. Neutrophils migrating into bacterial and viral–bacterial co-infection milieus exhibited the in vivo CF phenotype of increased CD63 expression and reduced CD16 expression, while neutrophils migrating into milieus of RV-infected or uninfected cultures did not. Individually, bacterial products lipopolysaccharide and N-formylmethionyl-leucyl-phenylalanine and isolated cytokine signals only partially activated this phenotype, suggesting that additional soluble factors in the infection microenvironment trigger primary granule release. Findings identify P. aeruginosa as a trigger of acute airway inflammation and neutrophil primary granule exocytosis, underscoring potential roles of airway microbes in prompting this neutrophil subset. Further studies are required to characterize microbes implicated in primary granule release, and identify potential therapeutic targets.

Copyright information:

© 2022 The Authors. Immunology & Cell Biology published by John Wiley & Sons Australia, Ltd on behalf of Australian and New Zealand Society for Immunology, Inc.

This is an Open Access work distributed under the terms of the Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International License (https://creativecommons.org/licenses/by-nc-nd/4.0/).
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