DISSECTING GLICO-VASCULAR BRAIN ORGANOID CO-CULTURES
Universiteit Utrecht
Presentation
Date TBA
Event Information
Poster Board
PS06-09PM-024
Poster
View posterAbstract
To establish this model, we genetically engineered patient derived GBM cells with a secreted luciferase construct to monitor live cell survival following different therapeutic treatments. Two glioblastoma cell lines were then co-cultured with iPSC-derived brain organoids and iPSC-derived endothelial cells for over a period of 15-40 days, both glioblastoma cell lines invaded and grew extensively into the brain vascular glico-organoid co-culture. Subsequently, the 3D vGlio-organoids will be treated with standard of care therapeutic agents at different dosages and compared to traditional 2D growth cell cultures.
Our results demonstrate that this 3DvGlico-coculture model is an optimal system for studying the mechanisms of GBM cells' interactions with the tumor microenvironment. The use of brain organoids that enable the simulation of the tumor microenvironment presents a powerful tool for investigating GBM pathogenesis.
Overall, our 3D in vitro model of GBM provides an innovative approach to improve preclinical models of glioblastoma, thereby offering opportunities for novel therapeutic interventions.
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