| Literature DB >> 25941477 |
Marianela Garcia-Munoz1, Eddy Taillefer2, Reuven Pnini2, Catherine Vickers3, Jonathan Miller2, Gordon W Arbuthnott1.
Abstract
Many of the methods available for the study of cortical influences on striatal neurons have serious problems. In vivo the connectivity is so complex that the study of input from an individual cortical neuron to a single striatal cell is nearly impossible. Mixed corticostriatal cultures develop many connections from striatal cells to cortical cells, in striking contrast to the fact that only connections from cortical cells to striatal cells are present in vivo. Furthermore, interneuron populations are over-represented in organotypic cultures. For these reasons, we have developed a method for growing cortical and striatal neurons in separated compartments that allows cortical neurons to innervate striatal cells in culture. The method works equally well for acutely dissociated or cryopreserved neurons and allows a number of manipulations that are not otherwise possible. Either cortical or striatal compartments can be transfected with channel rhodopsins. The activity of both areas can be recorded in multielectrode arrays or individual patch recordings from pairs of cells. Finally, corticostriatal connections can be severed acutely. This procedure enables determination of the importance of corticostriatal interaction in the resting pattern of activity. These cultures also facilitate development of sensitive analytical network methods to track connectivity.Entities:
Keywords: cortical neurons; interneurons; mutual information; neuronal cultures; striatal neurons; synaptic connections
Year: 2015 PMID: 25941477 PMCID: PMC4403293 DOI: 10.3389/fnsys.2015.00063
Source DB: PubMed Journal: Front Syst Neurosci ISSN: 1662-5137