Development of a Widely Accessible, Advanced Large-Scale Microfluidic Airway-on-Chip

Brady Rae; Gwenda F. Vasse; Jalal Mosayebi; Maarten van den Berge; Simon D. Pouwels; Irene H. Heijink

doi:10.3390/bioengineering12020182

Development of a Widely Accessible, Advanced Large-Scale Microfluidic Airway-on-Chip

Brady Rae^*, Gwenda F. Vasse, Jalal Mosayebi, Maarten van den Berge, Simon D. Pouwels, Irene H. Heijink

^*Corresponding author for this work

Research output: Contribution to journal › Article › Academic › peer-review

Abstract

On-chip microfluidics are advanced in vitro models that simulate lung tissue's native 3D environment more closely than static 2D models to investigate the complex lung architecture and multifactorial processes that lead to pulmonary disease. Current microfluidic systems can be restrictive in the quantities of biological sample that can be retrieved from a single micro-channel, such as RNA, protein, and supernatant. Here, we describe a newly developed large-scale airway-on-chip model that employs a surface area for a cell culture wider than that in currently available systems. This enables the collection of samples comparable in volume to traditional cell culture systems, making the device applicable to any workflow utilizing these static systems (RNA isolation, ELISA, etc.). With our construction method, this larger culture area allows for easier handling, the potential for a wide range of exposures, as well as the collection of low-quantity samples (e.g., volatiles or mitochondrial RNA). The model consists of two large polydimethylsiloxane (PDMS) cell culture chambers under an independent flow of medium or air, separated by a semi-permeable polyethylene (PET) cell culture membrane (23 mu m thick, 0.4 mu m pore size). Each chamber carries a 5 x 18 mm, 90 mm2 (92 mm2 with tapered chamber inlets) surface area that can contain up to 1-2 x 104 adherent structural lung cells and can be utilized for close contact co-culture studies of different lung cell types, including airway epithelial cells, fibroblasts, smooth muscle cells, and endothelial cells. The parallel bi-chambered design of the chip allows for epithelial cells to be cultured at the air-liquid interface (ALI) and differentiation into a dense, multi-layered, pseudostratified epithelium under biological flow rates. This millifluidic airway-on-chip advances the field by providing a readily reproducible, easily adjustable, and cost-effective large-scale fluidic 3D airway cell culture platform.

Original language	English
Article number	182
Number of pages	22
Journal	Bioengineering
Volume	12
Issue number	2
DOIs	https://doi.org/10.3390/bioengineering12020182
Publication status	Published - 1 Feb 2025

Keywords

microfluidics
airway-on-chip
epithelial cells
PDMS
air-liquid interface

Access to Document

10.3390/bioengineering12020182Licence: CC BY

Cite this

@article{026b02156cba42d5ac98c635eebe090f,

title = "Development of a Widely Accessible, Advanced Large-Scale Microfluidic Airway-on-Chip",

abstract = "On-chip microfluidics are advanced in vitro models that simulate lung tissue's native 3D environment more closely than static 2D models to investigate the complex lung architecture and multifactorial processes that lead to pulmonary disease. Current microfluidic systems can be restrictive in the quantities of biological sample that can be retrieved from a single micro-channel, such as RNA, protein, and supernatant. Here, we describe a newly developed large-scale airway-on-chip model that employs a surface area for a cell culture wider than that in currently available systems. This enables the collection of samples comparable in volume to traditional cell culture systems, making the device applicable to any workflow utilizing these static systems (RNA isolation, ELISA, etc.). With our construction method, this larger culture area allows for easier handling, the potential for a wide range of exposures, as well as the collection of low-quantity samples (e.g., volatiles or mitochondrial RNA). The model consists of two large polydimethylsiloxane (PDMS) cell culture chambers under an independent flow of medium or air, separated by a semi-permeable polyethylene (PET) cell culture membrane (23 mu m thick, 0.4 mu m pore size). Each chamber carries a 5 x 18 mm, 90 mm2 (92 mm2 with tapered chamber inlets) surface area that can contain up to 1-2 x 104 adherent structural lung cells and can be utilized for close contact co-culture studies of different lung cell types, including airway epithelial cells, fibroblasts, smooth muscle cells, and endothelial cells. The parallel bi-chambered design of the chip allows for epithelial cells to be cultured at the air-liquid interface (ALI) and differentiation into a dense, multi-layered, pseudostratified epithelium under biological flow rates. This millifluidic airway-on-chip advances the field by providing a readily reproducible, easily adjustable, and cost-effective large-scale fluidic 3D airway cell culture platform.",

keywords = "microfluidics, airway-on-chip, epithelial cells, PDMS, air-liquid interface",

author = "Brady Rae and Vasse, {Gwenda F.} and Jalal Mosayebi and {van den Berge}, Maarten and Pouwels, {Simon D.} and Heijink, {Irene H.}",

year = "2025",

month = feb,

day = "1",

doi = "10.3390/bioengineering12020182",

language = "English",

volume = "12",

journal = "Bioengineering",

issn = "2306-5354",

publisher = "MDPI AG",

number = "2",

}

TY - JOUR

T1 - Development of a Widely Accessible, Advanced Large-Scale Microfluidic Airway-on-Chip

AU - Rae, Brady

AU - Vasse, Gwenda F.

AU - Mosayebi, Jalal

AU - van den Berge, Maarten

AU - Pouwels, Simon D.

AU - Heijink, Irene H.

PY - 2025/2/1

Y1 - 2025/2/1

N2 - On-chip microfluidics are advanced in vitro models that simulate lung tissue's native 3D environment more closely than static 2D models to investigate the complex lung architecture and multifactorial processes that lead to pulmonary disease. Current microfluidic systems can be restrictive in the quantities of biological sample that can be retrieved from a single micro-channel, such as RNA, protein, and supernatant. Here, we describe a newly developed large-scale airway-on-chip model that employs a surface area for a cell culture wider than that in currently available systems. This enables the collection of samples comparable in volume to traditional cell culture systems, making the device applicable to any workflow utilizing these static systems (RNA isolation, ELISA, etc.). With our construction method, this larger culture area allows for easier handling, the potential for a wide range of exposures, as well as the collection of low-quantity samples (e.g., volatiles or mitochondrial RNA). The model consists of two large polydimethylsiloxane (PDMS) cell culture chambers under an independent flow of medium or air, separated by a semi-permeable polyethylene (PET) cell culture membrane (23 mu m thick, 0.4 mu m pore size). Each chamber carries a 5 x 18 mm, 90 mm2 (92 mm2 with tapered chamber inlets) surface area that can contain up to 1-2 x 104 adherent structural lung cells and can be utilized for close contact co-culture studies of different lung cell types, including airway epithelial cells, fibroblasts, smooth muscle cells, and endothelial cells. The parallel bi-chambered design of the chip allows for epithelial cells to be cultured at the air-liquid interface (ALI) and differentiation into a dense, multi-layered, pseudostratified epithelium under biological flow rates. This millifluidic airway-on-chip advances the field by providing a readily reproducible, easily adjustable, and cost-effective large-scale fluidic 3D airway cell culture platform.

AB - On-chip microfluidics are advanced in vitro models that simulate lung tissue's native 3D environment more closely than static 2D models to investigate the complex lung architecture and multifactorial processes that lead to pulmonary disease. Current microfluidic systems can be restrictive in the quantities of biological sample that can be retrieved from a single micro-channel, such as RNA, protein, and supernatant. Here, we describe a newly developed large-scale airway-on-chip model that employs a surface area for a cell culture wider than that in currently available systems. This enables the collection of samples comparable in volume to traditional cell culture systems, making the device applicable to any workflow utilizing these static systems (RNA isolation, ELISA, etc.). With our construction method, this larger culture area allows for easier handling, the potential for a wide range of exposures, as well as the collection of low-quantity samples (e.g., volatiles or mitochondrial RNA). The model consists of two large polydimethylsiloxane (PDMS) cell culture chambers under an independent flow of medium or air, separated by a semi-permeable polyethylene (PET) cell culture membrane (23 mu m thick, 0.4 mu m pore size). Each chamber carries a 5 x 18 mm, 90 mm2 (92 mm2 with tapered chamber inlets) surface area that can contain up to 1-2 x 104 adherent structural lung cells and can be utilized for close contact co-culture studies of different lung cell types, including airway epithelial cells, fibroblasts, smooth muscle cells, and endothelial cells. The parallel bi-chambered design of the chip allows for epithelial cells to be cultured at the air-liquid interface (ALI) and differentiation into a dense, multi-layered, pseudostratified epithelium under biological flow rates. This millifluidic airway-on-chip advances the field by providing a readily reproducible, easily adjustable, and cost-effective large-scale fluidic 3D airway cell culture platform.

KW - microfluidics

KW - airway-on-chip

KW - epithelial cells

KW - PDMS

KW - air-liquid interface

U2 - 10.3390/bioengineering12020182

DO - 10.3390/bioengineering12020182

M3 - Article

SN - 2306-5354

VL - 12

JO - Bioengineering

JF - Bioengineering

IS - 2

M1 - 182

ER -

Development of a Widely Accessible, Advanced Large-Scale Microfluidic Airway-on-Chip

Abstract

Keywords

Access to Document

Fingerprint

Cite this