A double-sided microscope to realize whole-ganglion imaging of membrane potential in the medicinal leech

Studies of neuronal network emergence during sensory processing and motor control are greatly facilitated by technologies that allow us to simultaneously record the membrane potential dynamics of a large population of neurons in single cell resolution. To achieve whole-brain recording with the ability to detect both small synaptic potentials and action potentials, we developed a voltage-sensitive dye (VSD) imaging technique based on a double-sided microscope that can image two sides of a nervous system simultaneously. We applied this system to the segmental ganglia of the medicinal leech. Double-sided VSD imaging enabled simultaneous recording of membrane potential events from almost all of the identifiable neurons. Using data obtained from double-sided VSD imaging, we analyzed neuronal dynamics in both sensory processing and generation of behavior and constructed functional maps for identification of neurons contributing to these processes

A double-sided microscope to realize whole-ganglion imaging of membrane potential in the medicinal leech

Studies of neuronal network emergence during sensory processing and motor control are greatly facilitated by technologies that allow us to simultaneously record the membrane potential dynamics of a large population of neurons in single cell resolution. To achieve whole-brain recording with the ability to detect both small synaptic potentials and action potentials, we developed a voltage-sensitive dye (VSD) imaging technique based on a double-sided microscope that can image two sides of a nervous system simultaneously. We applied this system to the segmental ganglia of the medicinal leech. Double-sided VSD imaging enabled simultaneous recording of membrane potential events from almost all of the identifiable neurons. Using data obtained from double-sided VSD imaging, we analyzed neuronal dynamics in both sensory processing and generation of behavior and constructed functional maps for identification of neurons contributing to these processes

Whole-ganglion imaging of voltage in the medicinal leech using a double-sided microscope

Studies of neuronal network emergence during sensory processing and motor control are greatly promoted by technologies that allow us to simultaneously record the membrane potential dynamics of a large population of neurons in single cell resolution. To achieve whole-brain recording with the ability to detect both small synaptic potentials and action potentials, we developed a voltage-sensitive dye (VSD) imaging technique based on a double-sided microscope that can image two sides of a nervous system simultaneously. We applied this system to the segmental ganglia of the medicinal leech Hirudo verbana. Double-sided VSD imaging enabled simultaneous recording of membrane potential events from almost all of the identifiable neurons. Using data obtained from double-sided VSD imaging we analyzed neuronal dynamics in both sensory processing and generation of behavior and constructed functional maps for identification of neurons contributing to these processes

Dual-sided Voltage-sensitive Dye Imaging of Leech Ganglia

In this protocol, we introduce an effective method for voltage-sensitive dye (VSD) loading and imaging of leech ganglia as used in Tomina and Wagenaar (2017). Dissection and dye loading procedures are the most critical steps toward successful whole-ganglion VSD imaging. The former entails the removal of the sheath that covers neurons in the segmental ganglion of the leech, which is required for successful dye loading. The latter entails gently flowing a new generation VSD, VF2.1(OMe).H, onto both sides of the ganglion simultaneously using a pair of peristaltic pumps. We expect the described techniques to translate broadly to wide-field VSD imaging in other thin and relatively transparent nervous systems

Dual-sided Voltage-sensitive Dye Imaging of Leech Ganglia

In this protocol, we introduce an effective method for voltage-sensitive dye (VSD) loading and imaging of leech ganglia as used in Tomina and Wagenaar (2017). Dissection and dye loading procedures are the most critical steps toward successful whole-ganglion VSD imaging. The former entails the removal of the sheath that covers neurons in the segmental ganglion of the leech, which is required for successful dye loading. The latter entails gently flowing a new generation VSD, VF2.1(OMe).H, onto both sides of the ganglion simultaneously using a pair of peristaltic pumps. We expect the described techniques to translate broadly to wide-field VSD imaging in other thin and relatively transparent nervous systems

Encoding of Coordinating Information in a Network of Coupled Oscillators

Animal locomotion is driven by cyclic movements of the body or body appendages. These movements are under the control of neural networks that are driven by central pattern generators (CPG). In order to produce meaningful behavior, CPGs need to be coordinated. The crayfish swimmeret system is a model to investigate the coordination of distributed CPGs. Swimmerets are four pairs of limbs on the animal’s abdomen, which move in cycles of alternating power-strokes and return-strokes. The swimmeret pairs are coordinated in a metachronal wave from posterior to anterior with a phase lag of approximately 25% between segments. Each swimmeret is controlled by its own neural microcircuit, located in the body segment’s hemiganglion. Three neurons per hemiganglion are necessary and sufficient for the 25% phase lag. ASCE DSC encode information about their home ganglion’s activity state and send it to their anterior or posterior target ganglia, respectively. ComInt 1, which is electrically coupled to the CPG, receives the coordinating information. The isolated abdominal ganglia chain reliably produces fictive swimming. Motor burst strength is encoded by the number of spikes per ASCE and DSC burst. If motor burst strength varies spontaneously, the coordinating neurons track these changes linearly. The neurons are hypothesized to adapt their spiking range to the occurring motor burst strengths. One aim of this study was to investigate the putative adaptive encoding of the coordinating neurons in electrophysiological experiments. This revealed that the system’s excitation level influenced both the whole system and the individual coordinating neurons. These mechanisms allowed the coordinating neurons to adapt to the range of burst strengths at any given excitation level by encoding relative burst strengths. The second aim was to identify the transmitters of the coordinating neurons at the synapse to ComInt 1. Immunohistochemical experiments demonstrated that coordinating neurons were not co-localized with serotonin-immunoreactive positive neurons. MALDI-TOF mass spectrometry suggested acetylcholine as presumable transmitter