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Active NON-SBIR/STTR RPGS NIH (US)

Utilizing Bioprinted Human Stem Cells for Molecular Screening via Multi-Material Strategies

$4.61M USD

Funder NATIONAL INSTITUTE OF BIOMEDICAL IMAGING AND BIOENGINEERING
Recipient Organization University of New Hampshire
Country United States
Start Date Sep 18, 2024
End Date Sep 16, 2027
Duration 1,093 days
Number of Grantees 1
Roles Principal Investigator
Data Source NIH (US)
Grant ID 11043883
Grant Description

Abstract Neurodegenerative disorders, such as Alzheimer's and Parkinson's diseases, are fundamentally characterized by neuronal damage and cell death. Development of adult and pluripotent stem cells for cellular therapies or therapeutic screening platforms may enable and accelerate novel treatment options for neuronal diseases.

However, ensuring the precise differentiation of stem cells into functional neurons within 3D culture environments presents a significant challenge. To overcome this hurdle, this project aims to create novel bioprinting methodologies for the production of human stem cell-based organoids by developing novel functionally-

optimized bioinks and optimized hydrogel formulations for pharmacological screens. Aim 1 focuses on developing a customized bioink, which includes water, biopolymers, ions, and cells, to optimize biochemical activity and mechanobiological responses. This endeavor aims to create a brain-like matrix under 100 μL using

a multi-material approach involving proteins, polysaccharides, and functionalized nanoparticles. The goal is to reproducibly produce 3D constructs that reduce the variabilities introduced from under-defined commercial sources. For this research, the bioink formulation incorporates gelatin, collagen, crosslinking enzymes,

photoinitiators, silica nanoparticles, neuron-inducing chemicals, and human stem cells. This formulation aims to foster the emergence of functional neurons 2-4 weeks after the 3D bioprinting process. Aim 2 focuses on the high-throughput (HT) assessment of neurotoxic chemicals' effects on the differentiation process of 3D hydrogel-

encapsulated neural stem cells. Utilizing commercial hydrogels for initial tests, this research will explore chemical differentiation processes and evaluate the influence of neurotoxic chemicals on neuronal differentiation. Characterization efforts will involve high-throughput imaging analysis methods plus flow cytometry that will allow

drawing correlations among bioink components and differentiation potentials. By comparing the outcomes with those obtained using custom bioink formulations (from Aim 1) vs. commercial products such as Matrigel and Geltrex, this project aims to identify a new bioink formulation that has the potential to revolutionize how we

consider and conduct tissue engineering research, including high-throughput molecular screening work. This would accelerate progress toward the development of screening platforms and new therapies for neurodegenerative disorders.

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University of New Hampshire

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