Method for cryopreservation of trigeminal ganglion for establishing primary cultures of neurons and glia

Authors

• Sophia R. Antonopoulos, Missouri State University
• Mikayla Scharnhorst, Missouri State University
• Nicole Nalley, Missouri State University
• Paul L. Durham, Missouri State UniversityFollow

Abstract

Background: Primary neuronal cultures are used to elucidate cellular and molecular mechanisms involved in disease pathology and modulation by pharmaceuticals and nutraceuticals, and to identify novel therapeutic targets. However, preparation of primary neuronal cultures from rodent embryos is labor-intensive, and it can be difficult to produce high-quality consistent cultures. To overcome these issues, cryopreservation can be used to obtain standardized, high-quality stocks of neuronal cultures. New method: In this study, we present a simplified cryopreservation method for rodent primary trigeminal ganglion neurons and glia from Sprague-Dawley neonates, using a 90:10 (v/v) fetal bovine serum/dimethyl sulfoxide cell freezing medium. Results: Cryopreserved trigeminal ganglion cells stored for up to one year in liquid nitrogen exhibited similar neuronal and glial cell morphology to fresh cultures and retained high cell viability. Proteins implicated in inflammation and pain signaling were expressed in agreement with the reported subcellular localization. Additionally, both neurons and glial cells exhibited an increase in intracellular calcium levels in response to a depolarizing stimulus. Cryopreserved cells were also transiently transfected with reporter genes. Comparison with existing methods: Our method is simple, does not require special reagents or equipment, will save time and money, increase flexibility in study design, and produce consistent cultures. Conclusions: This method for the preparation and cryopreservation of trigeminal ganglia results in primary cultures of neurons and glia similar in viability and morphology to fresh preparations that could be utilized for biochemical, cellular, and molecular studies, increase reproducibility, and save laboratory resources.

Department(s)

Biology

Document Type

Article

DOI

10.1016/j.jneumeth.2023.110034

Keywords

Calcium imaging, Cryopreservation, Immunocytochemistry, Satellite glia, Schwann cells, Trigeminal ganglion

Publication Date

2-1-2024

Recommended Citation

Antonopoulos, Sophia R.; Scharnhorst, Mikayla; Nalley, Nicole; and Durham, Paul L., "Method for cryopreservation of trigeminal ganglion for establishing primary cultures of neurons and glia" (2024). Faculty Scholarship. 409.
https://bearworks.missouristate.edu/articles00/409

Journal Title

Journal of Neuroscience Methods