Affiliation:
1. Neuroscience Program University of Illinois Urbana‐Champaign Urbana Illinois USA
2. Department of Molecular and Integrative Physiology University of Illinois Urbana‐Champaign Urbana Illinois USA
3. Beckman Institute for Advanced Science and Technology University of Illinois Urbana‐Champaign Urbana Illinois USA
4. Department of Bioengineering Stanford University Stanford California USA
5. Molecular and Integrative Physiology University of Michigan Ann Arbor Michigan USA
Abstract
AbstractAstrocytes play active roles at synapses and can monitor, respond, and adapt to local synaptic activity. While there is abundant evidence that astrocytes modulate excitatory transmission in the hippocampus, evidence for astrocytic modulation of hippocampal synaptic inhibition remains more limited. Furthermore, to better investigate roles for astrocytes in modulating synaptic transmission, more tools that can selectively activate native G protein signaling pathways in astrocytes with both spatial and temporal precision are needed. Here, we utilized AAV8‐GFAP‐Optoα1AR‐eYFP (Optoα1AR), a viral vector that enables activation of Gq signaling in astrocytes via light‐sensitive α1‐adrenergic receptors. To determine if stimulating astrocytic Optoα1AR modulates hippocampal synaptic transmission, recordings were made in CA1 pyramidal cells with surrounding astrocytes expressing Optoα1AR, channelrhodopsin (ChR2), or GFP. Both high‐frequency (20 Hz, 45‐ms light pulses, 5 mW, 5 min) and low‐frequency (0.5 Hz, 1‐s pulses at increasing 1, 5, and 10 mW intensities, 90 s per intensity) blue light stimulation were tested. 20 Hz Optoα1AR stimulation increased both inhibitory and excitatory postsynaptic current (IPSC and EPSC) frequency, and the effect on miniature IPSCs (mIPSCs) was largely reversible within 20 min. However, low‐frequency stimulation of Optoα1AR did not modulate either IPSCs or EPSCs, suggesting that astrocytic Gq‐dependent modulation of basal synaptic transmission in the hippocampus is stimulation‐dependent. By contrast, low‐frequency stimulation of astrocytic ChR2 was effective in increasing both synaptic excitation and inhibition. Together, these data demonstrate that Optoα1AR activation in astrocytes changes basal GABAergic and glutamatergic transmission, but only following high‐frequency stimulation, highlighting the importance of temporal dynamics when using optical tools to manipulate astrocyte function.
Funder
Beckman Institute
Brain Research Foundation
Citizens United for Research in Epilepsy
National Institute of Neurological Disorders and Stroke
Whitehall Foundation