Epithelial-mesenchymal crosstalk influences cellular behavior in a 3D alveolus-fibroblast model system

Katherine J R Lewis; Jessica K Hall; Emi A Kiyotake; Tova Christensen; Vivek Balasubramaniam; Kristi S Anseth

doi:10.1016/j.biomaterials.2017.11.008

Epithelial-mesenchymal crosstalk influences cellular behavior in a 3D alveolus-fibroblast model system

Biomaterials. 2018 Feb:155:124-134. doi: 10.1016/j.biomaterials.2017.11.008. Epub 2017 Nov 15.

Authors

Katherine J R Lewis¹, Jessica K Hall¹, Emi A Kiyotake¹, Tova Christensen², Vivek Balasubramaniam³, Kristi S Anseth⁴

Affiliations

¹ Department of Chemical and Biological Engineering, The BioFrontiers Institute, University of Colorado at Boulder, 3415 Colorado Ave, 596 UCB, Boulder, CO, 80303, USA.
² Department of Molecular, Cellular, and Developmental Biology, BioFrontiers Institute, University of Colorado, Boulder, CO, 80309, USA.
³ Department of Pediatrics, University of Wisconsin-Madison, 600 Highland Avenue, K4/922, Madison, WI, 53792, USA.
⁴ Department of Chemical and Biological Engineering, The BioFrontiers Institute, University of Colorado at Boulder, 3415 Colorado Ave, 596 UCB, Boulder, CO, 80303, USA. Electronic address: kristi.anseth@colorado.edu.

Abstract

Interactions between lung epithelium and interstitial fibroblasts are increasingly recognized as playing a major role in the progression of several lung pathologies, including cancer. Three-dimensional in vitro co-culture systems offer tissue-relevant platforms to study the signaling interplay between diseased and healthy cell types. Such systems provide a controlled environment in which to probe the mechanisms involved in epithelial-mesenchymal crosstalk. To recapitulate the native alveolar tissue architecture, we employed a cyst templating technique to culture alveolar epithelial cells on photodegradable microspheres and subsequently encapsulated the cell-laden spheres within poly (ethylene glycol) (PEG) hydrogels containing dispersed pulmonary fibroblasts. A fibroblast cell line (CCL-210) was co-cultured with either healthy mouse alveolar epithelial primary cells or a cancerous alveolar epithelial cell line (A549) to probe the influence of tumor-stromal interactions on proliferation, migration, and matrix remodeling. In 3D co-culture, cancerous epithelial cells and fibroblasts had higher proliferation rates. When examining fibroblast motility, the fibroblasts migrated faster when co-cultured with cancerous A549 cells. Finally, a fluorescent peptide reporter for matrix metalloproteinase (MMP) activity revealed increased MMP activity when A549s and fibroblasts were co-cultured. When MMP activity was inhibited or when cells were cultured in gels with a non-degradable crosslinker, fibroblast migration was dramatically suppressed, and the increase in cancer cell proliferation in co-culture was abrogated. Together, this evidence supports the idea that there is an exchange between the alveolar epithelium and surrounding fibroblasts during cancer progression that depends on MMP activity and points to potential signaling routes that merit further investigation to determine targets for cancer treatment.

Keywords: Alveolar epithelium; Cancer; Co-culture; Fibroblast; Hydrogel; Matrix metalloproteinases.

MeSH terms

A549 Cells
Animals
Cell Line
Coculture Techniques
Fibroblasts / cytology*
Fibroblasts / metabolism*
Humans
Hydrogels / chemistry
Matrix Metalloproteinase 9 / metabolism
Matrix Metalloproteinases / metabolism
Mice
Polyethylene Glycols / chemistry
Pulmonary Alveoli / cytology
Signal Transduction

Substances

Hydrogels
Polyethylene Glycols
Matrix Metalloproteinases
Matrix Metalloproteinase 9

Grants and funding

T32 GM065103/GM/NIGMS NIH HHS/United States