In this experiment, the laser was turned on (5 Hz sinus pattern) when the animal was in a selected part of the maze (Fig. 7B) on every other trial. In addition to the neurons’ place fields, light-induced firing could be observed in three of the place cells recorded by the shank with Galunisertib cost an optical fiber
(Fig. 7C, red arrows). Because ChR2 or NpHR expression can be restricted to genetically specific cell types (Fig. 3) (Cardin et al., 2009; Sohal et al., 2009), a major advantage of optical stimulation is the possibility of affecting only neurons of a selective type. In this respect, the optrode can be a powerful tool for studying the contribution of specific cell types to the local network dynamic. For example, neurons of a specific type can be identified among the numerous recorded neurons from their response to light and, subsequently, their firing pattern can be analyzed in relation to the firing of other neurons, local field potential patterns and the animal’s behavior. In addition, the impact of their stimulation or inhibition on the rest of the network can be monitored. Figure 8 shows
the light responses of cells recorded simultaneously in the CA1 hippocampal area of an NpHR/PV-Cre mouse. PV-expressing cells can be readily identified by their fast square-shape inhibition caused by the light pulses. Their firing rate is relatively high, as expected, as most PV-expressing neurons are known to be fast-spiking GABAergic interneurons Nivolumab in vitro (Freund & Buzsaki, 1996). In contrast, many cells showed an increased firing rate, presumably as a result of their disinhibition following the suppression of PV neuron firing. We have described a procedure for the fabrication of optoelectronic probes (optrodes), Cytidine deaminase tools that combine the advantages of optogenetics and silicon probes,
enabling both fine-scale stimulation and large-scale recording of neurons in behaving animals. A key advantage of these devices is the enhanced spatial precision of stimulation that is achieved by delivering light close to the recording sites of the probe. Additional cell-type specificity is achieved through genetic targeting of the light-activated current sources. Our experimental findings illustrate these capabilities. Microstimulation is an important tool for investigating the contribution of small groups of neurons to the network patterns (Salzman et al., 1990; Seidemann et al., 2002; Butovas & Schwarz, 2003; Cohen & Newsome, 2004; Butovas et al., 2006). For this purpose, electrical stimulation has some limitations. First, it generates local electrical artifacts that are typically larger than the extracellular spike signals, requiring complex methods to extract the neuronal waveforms (Olsson et al., 2005). Second, it activates neurons in a highly synchronous manner, preventing the reliable isolation of individual neurons by clustering methods for large-scale recordings.