| Literature DB >> 28605385 |
Monica L Gertz1, Zachary Baker2, Sharon Jose3, Nathalia Peixoto4.
Abstract
Micro-electrode arrays (MEAs) can be used to investigate drug toxicity, design paradigms for next-generation personalized medicine, and study network dynamics in neuronal cultures. In contrast with more traditional methods, such as patch-clamping, which can only record activity from a single cell, MEAs can record simultaneously from multiple sites in a network, without requiring the arduous task of placing each electrode individually. Moreover, numerous control and stimulation configurations can be easily applied within the same experimental setup, allowing for a broad range of dynamics to be explored. One of the key dynamics of interest in these in vitro studies has been the extent to which cultured networks display properties indicative of learning. Mouse neuronal cells cultured on MEAs display an increase in response following training induced by electrical stimulation. This protocol demonstrates how to culture neuronal cells on MEAs; successfully record from over 95% of the plated dishes; establish a protocol to train the networks to respond to patterns of stimulation; and sort, plot, and interpret the results from such experiments. The use of a proprietary system for stimulating and recording neuronal cultures is demonstrated. Software packages are also used to sort neuronal units. A custom-designed graphical user interface is used to visualize post-stimulus time histograms, inter-burst intervals, and burst duration, as well as to compare the cellular response to stimulation before and after a training protocol. Finally, representative results and future directions of this research effort are discussed.Entities:
Mesh:
Year: 2017 PMID: 28605385 PMCID: PMC5608154 DOI: 10.3791/55726
Source DB: PubMed Journal: J Vis Exp ISSN: 1940-087X Impact factor: 1.355
















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| 1 | Autoclaved glass reagent bottle (at least 100 mL size) |
| 20 | 15 mL sterile centrifuge tubes |
| 1 | 10 mL sterile serological pipette |
| 4 | 25 mL sterile serological pipette |
| 2 | 50 mL sterile serological pipette |
| 1 | Centrifuge tube rack |
| 150 mL | Sterile DI water |
| 5 mg | Poly-D-lysine vial |
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| 44 mL | DMEM with a stablilzed form of L-glutamine (see table of materials) |
| 1 mL | Serum-free supplement for neural cell culture (see table of materials) |
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| 49 mL | DMEM with a stablilzed form of L-glutamine (see table of materials) |
| 1 mL | Serum-free supplement for neural cell culture (see table of materials) |
| 100 µL | Ascorbic acid [4 mg/mL] |
| 0.5 mL | Pen strep (optional) |
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| 2 | 25 mL sterile serological pipette |
| 2 | 1 mL sterile serological pipette |
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