AI Article Synopsis

  • Human pluripotent stem cell-derived astrocytes (hiPSC-A) and neurons (hiPSC-N) are useful for studying ALS in the lab.
  • Co-culturing hiPSC-A with spinal cord hiPSC-motor neurons (MN) enhances their development and function, while using multi-electrode array (MEA) recordings allows for the observation of their electrical activity.
  • The described method can be adapted for other types of neurons and astrocytes, aiming to explore glial-neuronal interactions and evaluate potential ALS treatments.

Article Abstract

Human pluripotent stem cell-derived astrocytes (hiPSC-A) and neurons (hiPSC-N) provide a powerful tool for modeling Amyotrophic Lateral Sclerosis (ALS) pathophysiology in vitro. Multi-electrode array (MEA) recordings are a means to record electrical field potentials from large populations of neurons and analyze network activity over time. It was previously demonstrated that the presence of hiPSC-A that are differentiated using techniques to promote a spinal cord astrocyte phenotype improved maturation and electrophysiological activity of regionally specific spinal cord hiPSC-motor neurons (MN) when compared to those cultured without hiPSC-A or in the presence of rodent astrocytes. Described here is a method to co-culture spinal cord hiPSC-A with hiPSC-MN and record electrophysiological activity using MEA recordings. While the differentiation protocols described here are particular to astrocytes and neurons that are regionally specific to the spinal cord, the co-culturing platform can be applied to astrocytes and neurons differentiated with techniques specific to other fates, including cortical hiPSC-A and hiPSC-N. These protocols aim to provide an electrophysiological assay to inform about glia-neuron interactions and provide a platform for testing drugs with therapeutic potential in ALS.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC9169687PMC
http://dx.doi.org/10.3791/62726DOI Listing

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