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A Scalable Method to Study Neuronal Survival in Primary Neuronal Culture with Single-cell and Real-Time Resolution
In This Article
Summary
Here, we present a simple, potent, and versatile methodology to investigate neuronal survival upon cytotoxic stress in primary cortical neurons with cellular resolution in real time or in fixed material.
Abstract
Neuronal loss is at the core of many neuropathologies, including stroke, Alzheimer's disease, and Parkinson's disease. Different methods were developed to study the process of neuronal survival upon cytotoxic stress. Most methods are based on biochemical approaches that do not allow single-cell resolution or involve complex and costly methodologies. Presented here is a versatile, inexpensive, and effective experimental paradigm to study neuronal survival. This method takes advantage of sparse fluorescent labeling of the neurons followed by live imaging and automated quantification. To this aim, the neurons are electroporated to express fluorescent markers and co-cultured with non-electroporated neurons to easily regulate cell density and increase survival.
Sparse labeling by electroporation allows a simple and robust automated quantification. In addition, fluorescent labeling can be combined with the co-expression of a gene of interest to study specific molecular pathways. Here, we present a model of stroke as a neurotoxic model, namely, the oxygen-glucose deprivation (OGD) assay, which was performed in an affordable and robust homemade hypoxic chamber. Finally, two different workflows are described using IN Cell Analyzer 2200 or the open-source ImageJ for image analysis for semi-automatic data processing. This workflow can be easily adapted to different experimental models of toxicity and scaled up for high-throughput screening. In conclusion, the described protocol provides an approachable, affordable, and effective in vitro model of neurotoxicity, which can be suitable for testing the roles of specific genes and pathways in live imaging and for high-throughput drug screening.
Introduction
The study of neuronal disorders requires experimental models that are amenable to genetic, molecular, and cellular analyses. Primary cortical neurons are a very potent model for studying neuronal survival and toxicity1,2,3,4. Under the appropriate conditions, primary neurons will progressively develop synaptic contacts and present hallmarks of mature neurons. Therefore, this model is more reliable than immortalized cell lines in modeling the physiology of the neurons and more amenable to manipulations than animal models. However, in comparis....
Protocol
All procedures using animals should be supervised by the bioethical animal committee of the institute and performed in compliance with local regulations. The procedures presented herein were approved by the delegated authority and comply with the regulations in Spain and Europe.
1. Primary neuronal culture
NOTE: All the steps are performed inside the culture hood, using sterile materials and solutions to maintain sterile conditions.
- Poly-L-lysine (PLL) c.......
Representative Results
This protocol aims to establish an in vitro model of stroke. It is important to obtain an adequate neuronal density, which will allow the recognition of individual electroporated neurons to analyze them individually. The stage of the neuronal culture after plating is also crucial. The maturation of neurons in culture is progressive. The dependence on growth factors, neurite outgrowth, connectivity, and electrophysiological activity will vary greatly depending on the stage. In these specific conditions at 4-6 day.......
Discussion
This protocol shows an effective way of modeling a stroke in vitro. To achieve this goal, we proposed sparse labeling of cortical neurons using the electroporation system NEPA215. This is an open system that allows customization of the protocol with minimal operative cost compared to other systems that employ kits or specific devices. Mixed culture of naïve and electroporated neurons allows more flexibility and robustness as compared to low-density neuronal culture. This allows the s.......
Acknowledgements
We would like to thank Carlos Dotti for sharing his expertise in neuronal culture. We also thank Alicia Martínez-Romero from the Cytomics Core Facility of the Centro de Investigación Principe Felipe (CIPF), which is supported by European FEDERER funding. The project is supported by the Spanish Ministry of Economy and Competitiveness for (SAF2017-89020-R) reagents, materials, and the salaries of YDC and PF. PF is also supported by the grant RyC-2014-16410. CGN and PF are supported by Conselleria de Sanitat of the Generalitat Valenciana, as well as AGM (ACIF/2019/015). Ángela Rodríguez Prieto is supported by the Spanish Ministry of Science, Innovatio....
Materials
| Name | Company | Catalog Number | Comments |
| 10 cm petri dishes | FISHER SCIENTIFIC, S.L. | 1130-9283 | |
| 3.5 cm petri dishes | Sterilin | ||
| 75 cm2 flask | Corning | 430641U | |
| B-27 | Life Technologies | 17504-044 | |
| Cell culture plates | Corning incorporation Costar® | 3513 | |
| Cell incubator | Thermo Electron Corporation | Model 371 | |
| Cell strainer 70 µm | Falcon | 352350 | |
| Cold lights | Schott | 223488 | KL 1500 LCD |
| Coverslips (15 mm) | Marienfeld | 111530 | |
| CU500 Cuvette Chamber | Nepa Gene | ||
| CU600 Cuvette Stand Holder | Nepa Gene | ||
| DAPI | Sigma-Aldrich Quimica, S. L. | D9542-10MG | 1:2000 |
| DMSO | Panreac | A3672 | |
| Dumont Fine Forceps | FST | 11254-20 | |
| Dumont Fine Forceps | FST | 11252-00 | |
| EC-002S NEPA Electroporation Cuvettes, 2mm gap | Nepa Gene | ||
| Filter strainer | Falcon | 352350 | |
| Fine Scissors-Sharp-Blunt | FST | 14028-10 | |
| Fine Scissors-ToughCut r | FST | 14058-09 | |
| GFP chicken IgY | Aves Labs | GFP-1010 | 1:600 |
| Glucose | Sigma | 68769-100ml | |
| GlutaMAX-I Supplement 200 mM 100 mL | Fisher Scientific | 35050-061 | |
| HBSS | Thermofisher | 14175-095 | https://www.thermofisher.com/es/es/home/technical-resources/media-formulation.156.html |
| Hepes 1 M | ThermoFisher | 15630-080 | |
| Horse Serum | Invitrogen | 26050088 | |
| MEM | Thermofisher | 11095080 | https://www.thermofisher.com/order/catalog/product/11095080#/11095080 |
| Microscope slide (polilysine) | VWR | 631-0107 | Dimension: 25 x 75 x 1 mm |
| Mowiol 4-88 | Sigma-Aldrich Quimica, S. L. | 81381-250G | |
| Needles yellow, 30 gauge | BD Microlance™ 3 | 304000 | |
| NEPA21 electroporator | Nepa Gene | ||
| Neubauer chamber | Blau Brand | 717805 | |
| Neurobasal Medium | ThermoFisher | 21103-49 | |
| Opti-MEM | Invitrogen | 31985-062 | |
| Parafilm | Cole-Parmer | PM996 | |
| Paraformaldehyde (PFA), 95% | Sigma-Aldrich Quimica, S. L. | 158127-500G | Use solution: 4% |
| PEI | Polysciences | 23966-1 | |
| Plasmid for GFP | pCMV-GFP-ires-Cre, described in Fazzari et al., Nature, 2010 | ||
| Poly-L-Lysine | SIGMA | P2636 | |
| PS ( Penicillin, Streptomycin) | ThermoFisher | 15140122 | |
| Serrate forceps | FST | 11152-10 | |
| Stereomicroscope | WORLD PRECISION INSTRUMENTS | ||
| Syringes | BD Plastipak 1ml | 303176 | |
| Triton X-100 | Sigma-Aldrich Quimica, S. L. | MDL number: MFCD00128254 | Non-ionic |
| Trypsin-EDTA | ThermoFisher | 25300054 | |
| Tubes 15 mL | Fisher | 05-539-4 | |
| Tubes 50 mL | VWR | 21008-242 | |
| Tupperware | - | - | Hermetic tupperware with screw lid. SP Berner - Taper 1 L Redondo con Rosca. Any equivalent hermetic Tupperware may be purchased in any supermarket. |
| Water bath | SHELDON LABORATORY MODEL 1224 | 1641951 | |
References
- Salazar, I. L., Mele, M., Caldeira, M., Costa, R. O., Correia, B., Frisari, S., Duarte, C. B. Preparation of primary cultures of embryonic rat hippocampal and cerebrocortical neurons. Bio-protocol. 7 (18), 2551 (2017).
- Kaech, S., Banker, G.
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