| Literature DB >> 26650685 |
Marta F Estrada1, Sofia P Rebelo1, Emma J Davies2, Marta T Pinto3, Hugo Pereira4, Vítor E Santo1, Matthew J Smalley5, Simon T Barry6, Emilio J Gualda7, Paula M Alves1, Elizabeth Anderson8, Catarina Brito9.
Abstract
3D cell tumour models are generated mainly in non-scalable culture systems, using bioactive scaffolds. Many of these models fail to reflect the complex tumour microenvironment and do not allow long-term monitoring of tumour progression. To overcome these limitations, we have combined alginate microencapsulation with agitation-based culture systems, to recapitulate and monitor key aspects of the tumour microenvironment and disease progression. Aggregates of MCF-7 breast cancer cells were microencapsulated in alginate, either alone or in combination with human fibroblasts, then cultured for 15 days. In co-cultures, the fibroblasts arranged themselves around the tumour aggregates creating distinct epithelial and stromal compartments. The presence of fibroblasts resulted in secretion of pro-inflammatory cytokines and deposition of collagen in the stromal compartment. Tumour cells established cell-cell contacts and polarised around small lumina in the interior of the aggregates. Over the culture period, there was a reduction in oestrogen receptor and membranous E-cadherin alongside loss of cell polarity, increased collective cell migration and enhanced angiogenic potential in co-cultures. These phenotypic alterations, typical of advanced stages of cancer, were not observed in the mono-cultures of MCF-7 cells. The proposed model system constitutes a new tool to study tumour-stroma crosstalk, disease progression and drug resistance mechanisms.Entities:
Keywords: 3D; Alginate microencapsulation; Co-culture; Stirred-tank bioreactors; Tumour microenvironment; Tumour progression
Mesh:
Year: 2015 PMID: 26650685 DOI: 10.1016/j.biomaterials.2015.11.030
Source DB: PubMed Journal: Biomaterials ISSN: 0142-9612 Impact factor: 12.479