Frontiers in Pharmacology (Mar 2023)

A multiplex inhalation platform to model in situ like aerosol delivery in a breathing lung-on-chip

  • Arunima Sengupta,
  • Aurélien Dorn,
  • Aurélien Dorn,
  • Mohammad Jamshidi,
  • Magali Schwob,
  • Widad Hassan,
  • Lea Lara De Maddalena,
  • Andreas Hugi,
  • Andreas O. Stucki,
  • Patrick Dorn,
  • Patrick Dorn,
  • Thomas M. Marti,
  • Thomas M. Marti,
  • Oliver Wisser,
  • Janick D. Stucki,
  • Tobias Krebs,
  • Nina Hobi,
  • Olivier T. Guenat,
  • Olivier T. Guenat,
  • Olivier T. Guenat

DOI
https://doi.org/10.3389/fphar.2023.1114739
Journal volume & issue
Vol. 14

Abstract

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Prolonged exposure to environmental respirable toxicants can lead to the development and worsening of severe respiratory diseases such as asthma, chronic obstructive pulmonary disease (COPD) and fibrosis. The limited number of FDA-approved inhaled drugs for these serious lung conditions has led to a shift from in vivo towards the use of alternative in vitro human-relevant models to better predict the toxicity of inhaled particles in preclinical research. While there are several inhalation exposure models for the upper airways, the fragile and dynamic nature of the alveolar microenvironment has limited the development of reproducible exposure models for the distal lung. Here, we present a mechanistic approach using a new generation of exposure systems, the Cloud α AX12. This novel in vitro inhalation tool consists of a cloud-based exposure chamber (VITROCELL) that integrates the breathing AXLung-on-chip system (AlveoliX). The ultrathin and porous membrane of the AX12 plate was used to create a complex multicellular model that enables key physiological culture conditions: the air-liquid interface (ALI) and the three-dimensional cyclic stretch (CS). Human-relevant cellular models were established for a) the distal alveolar-capillary interface using primary cell-derived immortalized alveolar epithelial cells (AXiAECs), macrophages (THP-1) and endothelial (HLMVEC) cells, and b) the upper-airways using Calu3 cells. Primary human alveolar epithelial cells (AXhAEpCs) were used to validate the toxicity results obtained from the immortalized cell lines. To mimic in vivo relevant aerosol exposures with the Cloud α AX12, three different models were established using: a) titanium dioxide (TiO2) and zinc oxide nanoparticles b) polyhexamethylene guanidine a toxic chemical and c) an anti-inflammatory inhaled corticosteroid, fluticasone propionate (FL). Our results suggest an important synergistic effect on the air-blood barrier sensitivity, cytotoxicity and inflammation, when air-liquid interface and cyclic stretch culture conditions are combined. To the best of our knowledge, this is the first time that an in vitro inhalation exposure system for the distal lung has been described with a breathing lung-on-chip technology. The Cloud α AX12 model thus represents a state-of-the-art pre-clinical tool to study inhalation toxicity risks, drug safety and efficacy.

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