Your search keyword '"Kolkman, Kristine E."' showing total 17 results

1. A large field-of-view, single-cell-resolution two- and three-photon microscope for deep and wide imaging

Author

Mok, Aaron T., Wang, Tianyu, Zhao, Shitong, Kolkman, Kristine E., Wu, Danni, Ouzounov, Dimitre G., Seo, Changwoo, Wu, Chunyan, Fetcho, Joseph R., and Xu, Chris

Published

2024

2. Whole-brain optical access in a small adult vertebrate with two- and three-photon microscopy

Author

Akbari, Najva, Tatarsky, Rose L., Kolkman, Kristine E., Fetcho, Joseph R., Bass, Andrew H., and Xu, Chris

Published

2022

3. Deep three-photon imaging of the brain in intact adult zebrafish

Author

Chow, Dawnis M., Sinefeld, David, Kolkman, Kristine E., Ouzounov, Dimitre G., Akbari, Najva, Tatarsky, Rose, Bass, Andrew, Xu, Chris, and Fetcho, Joseph R.

Published

2020

4. Label-free, whole-brain in vivo mapping in an adult vertebrate with third harmonic generation microscopy.

Author

Akbari, Najva, Tatarsky, Rose L., Kolkman, Kristine E., Fetcho, Joseph R., Xu, Chris, and Bass, Andrew H.

Abstract

Comprehensive understanding of interconnected networks within the brain requires access to high resolution information within large field of views and over time. Currently, methods that enable mapping structural changes of the entire brain in vivo are extremely limited. Third harmonic generation (THG) can resolvemyelinated structures, blood vessels, and cell bodies throughout the brain without the need for any exogenous labeling. Together with deep penetration of long wavelengths, this enables in vivo brain-mapping of large fractions of the brain in small animals and over time. Here, we demonstrate that THG microscopy allows non-invasive label-free mapping of the entire brain of an adult vertebrate, Danionella dracula, which is a miniature species of cyprinid fish. We show this capability in multiple brain regions and in particular the identification of major commissural fiber bundles in the midbrain and the hindbrain. These features provide readily discernable landmarks for navigation and identification of regional-specific neuronal groups and even single neurons during in vivo experiments. We further show how this label-free technique can easily be coupled with fluorescence microscopy and used as a comparative tool for studies of other species with similar body features to Danionella, such as zebrafish (Danio rerio) and tetras (Trochilocharax ornatus). This new evidence, building on previous studies, demonstrates how small size and relative transparency, combinedwith the unique capabilities of THGmicroscopy, can enable label-free access to the entire adult vertebrate brain. [ABSTRACT FROM AUTHOR]

Published

2024

5. Graded Coexpression of Ion Channel, Neurofilament, and Synaptic Genes in Fast-Spiking Vestibular Nucleus Neurons.

Author

Takashi Kodama, Gittis, Aryn H., Minyoung Shin, Kelleher, Keith, Kolkman, Kristine E., McElvain, Lauren, Lam, Minh, and du Lac, Sascha

Subjects

ION channels, VOLTAGE-gated ion channels, GENE regulatory networks, CYTOPLASMIC filaments, NEURONS, VESTIBULO-ocular reflex, NEURAL codes

Abstract

Computations that require speed and temporal precision are implemented throughout the nervous system by neurons capable of firing at very high rates, rapidly encoding and transmitting a rich amount of information, but with substantial metabolic and physical costs. For economical fast spiking and high throughput information processing, neurons need to optimize multiple biophysical properties in parallel, but the mechanisms of this coordination remain unknown. We hypothesized that coordinated gene expression may underlie the coordinated tuning of the biophysical properties required for rapid firing and signal transmission. Taking advantage of the diversity of fast-spiking cell types in the medial vestibular nucleus of mice of both sexes, we examined the relationship between gene expression, ionic currents, and neuronal firing capacity. Across excitatory and inhibitory cell types, genes encoding voltage-gated ion channels responsible for depolarizing and repolarizing the action potential were tightly coexpressed, and their absolute expression levels increased with maximal firing rate. Remarkably, this coordinated gene expression extended to neurofilaments and specific presynaptic molecules, providing a mechanism for coregulating axon caliber and transmitter release to match firing capacity. These findings suggest the presence of a module of genes, which is coexpressed in a graded manner and jointly tunes multiple biophysical properties for economical differentiation of firing capacity. The graded tuning of fast-spiking capacity by the absolute expression levels of specific ion channels provides a counterexample to the widely held assumption that cell-type-specific firing patterns can be achieved via a vast combination of different ion channels. [ABSTRACT FROM AUTHOR]

Published

2020

6. Features of the structure, development, and activity of the zebrafish noradrenergic system explored in new CRISPR transgenic lines.

Author

Farrar, Matthew J., Kolkman, Kristine E., and Fetcho, Joseph R.

Abstract

The noradrenergic (NA) system of vertebrates is implicated in learning, memory, arousal, and neuroinflammatory responses, but is difficult to access experimentally. Small and optically transparent, larval zebrafish offer the prospect of exploration of NA structure and function in an intact animal. We made multiple transgenic zebrafish lines using the CRISPR/Cas9 system to insert fluorescent reporters upstream of slc6a2, the norepinephrine transporter gene. These lines faithfully express reporters in NA cell populations, including the locus coeruleus (LC), which contains only about 14 total neurons. We used the lines in combination with two‐photon microscopy to explore the structure and projections of the NA system in the context of the columnar organization of cell types in the zebrafish hindbrain. We found robust alignment of NA projections with glutamatergic neurotransmitter stripes in some hindbrain segments, suggesting orderly relations to neuronal cell types early in life. We also quantified neurite density in the rostral spinal cord in individual larvae with as much as 100% difference in the number of LC neurons, and found no correlation between neuronal number in the LC and projection density in the rostral spinal cord. Finally, using light sheet microscopy, we performed bilateral calcium imaging of the entire LC. We found that large‐amplitude calcium responses were evident in all LC neurons and showed bilateral synchrony, whereas small‐amplitude events were more likely to show interhemispheric asynchrony, supporting the potential for targeted LC neuromodulation. Our observations and new transgenic lines set the stage for a deeper understanding of the NA system. [ABSTRACT FROM AUTHOR]

Published

2018

7. Whole-brain optical access and longitudinal imaging in an adult vertebrate, Danionella dracula, with multiphoton microscopy.

Author

Akbari, Najva, Tatarsky, Rose L., Kolkman, Kristine E., Fetcho, Joseph R., Bass, Andrew H., and Xu, Chris

Published

2022

8. Diverse Precerebellar Neurons Share Similar Intrinsic Excitability.

Author

Kolkman, Kristine E., McElvain, Lauren E., and du Lac, Sascha

Abstract

The cerebellum dedicates a majority of the brain’s neurons to processing a wide range of sensory, motor, and cognitive signals. Stereotyped circuitry within the cerebellar cortex suggests that similar computations are performed throughout the cerebellum, but little is known about whether diverse precerebellar neurons are specialized for the nature of the information they convey. In vivo recordings indicatethatfiring responsesto sensory or motor stimuli vary dramatically across different precerebellar nuclei, but whetherthis reflects diverse synaptic inputs or differentiallytuned intrinsic excitability has not been determined.Wetargeted whole-cell patch-clamp recordings to neurons in eight precerebellar nuclei which were retrogradely labeled from different regions of the cerebellum in mice. Intrinsic physiology was compared across neuronsinthemedial vestibular, external cuneate, lateral reticular, prepositus hypoglossi, supragenual, Roller/intercalatus, reticularis tegmenti pontis, and pontine nuclei. Within the firing domain, precerebellar neurons were remarkably similar. Firing faithfully followed temporally modulated inputs, could be sustained at high rates, and was a linear function of input current over a wide range of inputs and firing rates. Pharmacological analyses revealed common expression of Kv3 currents, which were essential for a wide linear firing range, and of SK (small-conductance calcium-activated potassium) currents, which were essential for a wide linear input range. In contrast, membrane properties below spike threshold varied considerably within and across precerebellar nuclei, as evidenced by variability in postinhibitory rebound firing. Our findings indicate that diverse precerebellar neurons perform similar scaling computations on their inputs but may be differentially tuned to synaptic inhibition. [ABSTRACT FROM AUTHOR]

Published

2011

9. Multiple Types of Cerebellar Target Neurons and Their Circuitry in the Vestibulo-ocular Reflex.

Author

Minyoung Shin, Moghadam, Setareh H., Sekirnjak, Chris, Bagnall, Martha W., Kolkman, Kristine E., Jacobs, Richard, Faulstich, Michael, and du Lac, Sascha

Subjects

CEREBELLUM physiology, NEURAL physiology, VESTIBULO-ocular reflex, REFLEXES, CELL nuclei, PURKINJE cells, PHYSIOLOGY

Abstract

The cerebellum influences behavior and cognition exclusively via Purkinje cell synapses onto neurons in the deep cerebellar and vestibular nuclei. In contrast with the rich information available about the organization of the cerebellar cortex and its synaptic inputs, relatively little is known about microcircuitry postsynaptic to Purkinje cells. Here we examined the cell types and microcircuits through which Purkinje cells influence an oculomotor behavior controlled by the cerebellum, the horizontal vestibulo-ocular reflex, which involves only two eye muscles. Using a combination of anatomical tracing and electrophysiological recordings in transgenic mouse lines, we identified several classes of neurons in the medial vestibular nucleus that receive Purkinje cell synapses from the cerebellar flocculus. Glycinergic and glutamatergic flocculus target neurons (FTNs) with somata densely surrounded by Purkinje cell terminals projected axons to the ipsilateral abducens and oculomotor nuclei, respectively. Of three additional types of FTNs that were sparsely innervated by Purkinje cells, glutamatergic and glycinergic neurons projected to the contralateral and ipsilateral abducens, respectively, and GABAergic neurons projected to contralateral vestibular nuclei. Densely innervated FTNs had high spontaneous firing rates and pronounced postinhibitory rebound firing, and were physiologically homogeneous, whereas the intrinsic excitability of sparsely innervated FTNs varied widely. Heterogeneity in the molecular expression, physiological properties, and postsynaptic targets of FTNs implies that Purkinje cell activity influences the neural control of eye movements in several distinct ways. These results indicate that the cerebellum regulates a simple reflex behavior via at least five different cell types that are postsynaptic to Purkinje cells. [ABSTRACT FROM AUTHOR]

Published

2011

10. Intrinsic physiology of identified neurons in the prepositus hypoglossi and medial vestibular nuclei.

Author

Peusner, Kenna D., Kolkman, Kristine E., Moghadam, Setareh H., and du Lac, Sascha

Subjects

*INTRINSIC factor (Physiology), *NEURONS, *VESTIBULAR nuclei, *NEUROTRANSMITTERS, *BIOLOGICAL membranes, *PROTEINS, *BRAIN stem, *SPINAL cord, *GLUTAMIC acid

Abstract

Signal processing in the vestibular system is influenced by the intrinsic physiological properties of neurons that differ in neurotransmitters and circuit connections. Do membrane and firing properties differ across functionally distinct cell types? This study examines the intrinsic physiology of neurons in the medial vestibular nucleus (MVN) and nucleus prepositus hypoglossi (NPH) which express different neurotransmitters and have distinct axonal projections. NPH neurons expressing fluorescent proteins in glutamatergic, glycinergic, or GABAergic neurons were targeted for whole-cell patch recordings in brainstem slices obtained from transgenic mouse lines (YFP-16, GlyT2, and GIN). Recordings from MVN neurons projecting to the spinal cord, reticular formation, or oculomotor nucleus were obtained by targeting fluorescent neurons retrogradely labeled from tracer injections. Intrinsic physiological properties of identified neurons exhibited continuous variations but tended to differ between functionally defined cell types. Within the NPH, YFP-16 neurons had the narrowest action potentials and highest evoked firing rates and expressed high levels of Kv3.3 proteins, which speed repolarization. MVN neurons projecting to the spinal cord and oculomotor nucleus had similar action potential waveforms, but oculomotor-projecting neurons had higher intrinsic gains than those projecting to the spinal cord. These results indicate that intrinsic membrane properties are differentially tuned in MVN and NPH neurons subserving different functions. [ABSTRACT FROM AUTHOR]

Published

2011

11. Serotonergic modulation in aplysia. I. Distributed serotonergic network persistently activated by sensitizing stimuli.

Author

Marinesco St''phane, Kolkman Kristine E, and Carew Thomas J

Subjects

*SEROTONINERGIC mechanisms, *APLYSIA, *NERVOUS system, *STIMULUS intensity

Abstract

A common feature of arousing stimuli used as reinforcement in animal models of learning is that they promote memory formation through widespread effects in the CNS. In the marine mollusk Aplysia, sensitization is typically induced by tail-shock, an aversive reinforcer that triggers a state of defensive arousal characterized by escape locomotion and increased heart rate. Serotonin (5-HT) contributes importantly to sensitization of defensive reflexes as well as to the regulation of locomotion and heart rate. Although specific serotonergic neurons increase their firing after tail-shock, it remains unclear whether this effect is restricted to these neurons or whether tail-shock recruits a more global serotonergic system. In this study, we recorded from serotonergic neurons throughout the CNS, which were prelabeled with 5,7-dihydroxytryptamine, during an in vitro analog of sensitization training, tail-nerve shock. We found that most of the serotonergic neurons that we recorded from (80%) increased their firing rate for several minutes after nerve shock. Most serotonergic neurons in the pedal and abdominal ganglion were also excited by 5-HT and by intracellular activation of the two serotonergic neurons CB1/CC3. This interconnectivity between serotonergic neurons might contribute to spread excitation within a large proportion of the serotonergic system during sensitization training. It is also possible that serotonergic neurons could be activated by 5-HT present in the hemolymph via a neuro-humoral positive feedback mechanism. Overall, these data indicate that sensitization training activates a large proportion of Aplysia serotonergic neurons and that this form of learning occurs in a context of increased serotonergic tone. [ABSTRACT FROM AUTHOR]

Published

2004

12. Serotonergic modulation in aplysia. II. Cellular and behavioral consequences of increased serotonergic tone.

Author

Marinesco St''phane, Wickremasinghe Nimalee, Kolkman Kristine E, and Carew Thomas J

Subjects

SEROTONINERGIC mechanisms, APLYSIA, NERVOUS system, STIMULUS intensity

Abstract

Serotonin (5-HT) plays an important role in sensitization of defensive reflexes in Aplysia and is also involved in several aspects of arousal, such as the control of locomotion and of cardiovascular tone. In the preceding paper, we showed that tail-nerve shock, a noxious stimulus that readily induces sensitization, increases the firing rate of a large number of serotonergic neurons throughout the CNS. However, the functional consequences of such an increase in serotonergic tone are still poorly understood. In this study, we examined this question by using the 5-HT precursor 5-hydroxytryptophan (5-HTP) to specifically increase 5-HT release in the CNS. Increased tonic 5-HT release after 5-HTP treatment was manifested by facilitation of sensorimotor (SN-MN) synapses, increased firing rate of serotonergic neurons in the pedal and abdominal ganglia, and enhanced 5-HT release evoked by tail-nerve shock. When 5-HTP was administered to freely moving animals, it produced a strong arousal response characterized by increased locomotion and heart rate, which was reminiscent of the defensive arousal reaction triggered by noxious stimulation such as tail-shock. In contrast, 5-HTP actually inhibited the tail-induced siphon-withdrawal reflex. It is possible that 5-HT-induced facilitation of SN-MN synapses was counteracted by inhibition of polysynaptic reflex pathways between SNs and MNs, resulting in transient behavioral inhibition of the reflex, which could favor escape locomotion and/or respiration shortly after an aversive stimulus. We conclude that a major function associated with the activation of the Aplysia serotonergic system evoked by noxious stimuli is the triggering of a defensive arousal response. It is known that tail-shock-induced serotonergic activation contributes to memory encoding at least in part by facilitating SN-MN synapses. However, this effect in isolation might not be sufficient for the behavioral expression of sensitization. [ABSTRACT FROM AUTHOR]

Published

2004

13. A Large Field-of-view, Single-cell-resolution Two- and Three-Photon Microscope for Deep Imaging.

Author

Mok AT, Wang T, Zhao S, Kolkman KE, Wu D, Ouzounov DG, Seo C, Wu C, Fetcho JR, and Xu C

Abstract

In vivo imaging of large-scale neuron activity plays a pivotal role in unraveling the function of the brain's network. Multiphoton microscopy, a powerful tool for deep-tissue imaging, has received sustained interest in advancing its speed, field of view and imaging depth. However, to avoid thermal damage in scattering biological tissue, field of view decreases exponentially as imaging depth increases. We present a suite of innovations to overcome constraints on the field of view in three-photon microscopy and to perform deep imaging that is inaccessible to two-photon microscopy. These innovations enable us to image neuronal activities in a ~3.5-mm diameter field-of-view at 4 Hz with single-cell resolution and in the deepest cortical layer of mouse brains. We further demonstrate simultaneous large field-of-view two-photon and three-photon imaging, subcortical imaging in the mouse brain, and whole-brain imaging in adult zebrafish. The demonstrated techniques can be integrated into any multiphoton microscope for large-field-of-view and system-level neural circuit research., Competing Interests: Competing interests C.X., A.M., T.W., are listed as inventors on a US provisional patent application (serial no. 63/464,489) on Optical Pulse Generator and Method. The other authors declare no competing interests.

Published

2024

14. Deep-Tissue Three-Photon Fluorescence Microscopy in Intact Mouse and Zebrafish Brain.

Author

Hontani Y, Akbari N, Kolkman KE, Wu C, Xia F, Choe K, Wang GZ, Sokolova M, Fetcho JR, and Xu C

Subjects

Animals, Brain diagnostic imaging, Lasers, Mice, Microscopy, Fluorescence methods, Microscopy, Fluorescence, Multiphoton methods, Photons, Zebrafish

Abstract

Multiphoton microscopy techniques, such as two-photon microscopy (2PM) and three-photon microscopy (3PM), are powerful tools for deep-tissue in vivo imaging with subcellular resolution. 3PM has two major advantages for deep-tissue imaging over 2PM that has been widely used in biology laboratories: (i) longer attenuation length in scattering tissues by employing ~1,300 nm or ~1,700 nm excitation laser; (ii) less background fluorescence generation due to higher-order nonlinear excitation. As a result, 3PM allows high-contrast structural and functional imaging deep within scattering tissues such as intact mouse brain from the cortical layers to the hippocampus and the entire forebrain of adult zebrafish. Today, laser sources suitable for 3PM are commercially available, enabling the conversion of an existing two-photon (2P) imaging system to a three-photon (3P) system. Additionally, multiple commercial 3P microscopes are available, which makes this technique readily available to biology research laboratories. This paper shows the optimization of a typical 3PM setup, particularly targeting biology groups that already have a 2P setup, and demonstrates intravital 3D imaging in intact mouse and adult zebrafish brains. This protocol covers the full experimental procedure of 3P imaging, including microscope alignment, prechirping of ~1,300 and ~1,700 nm laser pulses, animal preparation, and intravital 3P fluorescence imaging deep in adult zebrafish and mouse brains.

Published

2022

15. Graded Coexpression of Ion Channel, Neurofilament, and Synaptic Genes in Fast-Spiking Vestibular Nucleus Neurons.

Author

Kodama T, Gittis AH, Shin M, Kelleher K, Kolkman KE, McElvain L, Lam M, and du Lac S

Subjects

Action Potentials, Animals, Axons metabolism, Axons physiology, Electrophysiological Phenomena genetics, Female, Gene Expression Regulation genetics, Genome-Wide Association Study, Male, Mice, Mice, Inbred C57BL, Patch-Clamp Techniques, Synaptic Transmission genetics, Synaptic Transmission physiology, Vestibular Nuclei cytology, Ion Channels biosynthesis, Neurofilament Proteins biosynthesis, Neurons metabolism, Synapses genetics, Vestibular Nuclei metabolism

Abstract

Computations that require speed and temporal precision are implemented throughout the nervous system by neurons capable of firing at very high rates, rapidly encoding and transmitting a rich amount of information, but with substantial metabolic and physical costs. For economical fast spiking and high throughput information processing, neurons need to optimize multiple biophysical properties in parallel, but the mechanisms of this coordination remain unknown. We hypothesized that coordinated gene expression may underlie the coordinated tuning of the biophysical properties required for rapid firing and signal transmission. Taking advantage of the diversity of fast-spiking cell types in the medial vestibular nucleus of mice of both sexes, we examined the relationship between gene expression, ionic currents, and neuronal firing capacity. Across excitatory and inhibitory cell types, genes encoding voltage-gated ion channels responsible for depolarizing and repolarizing the action potential were tightly coexpressed, and their absolute expression levels increased with maximal firing rate. Remarkably, this coordinated gene expression extended to neurofilaments and specific presynaptic molecules, providing a mechanism for coregulating axon caliber and transmitter release to match firing capacity. These findings suggest the presence of a module of genes, which is coexpressed in a graded manner and jointly tunes multiple biophysical properties for economical differentiation of firing capacity. The graded tuning of fast-spiking capacity by the absolute expression levels of specific ion channels provides a counterexample to the widely held assumption that cell-type-specific firing patterns can be achieved via a vast combination of different ion channels. SIGNIFICANCE STATEMENT Although essential roles of fast-spiking neurons in various neural circuits have been widely recognized, it remains unclear how neurons efficiently coordinate the multiple biophysical properties required to maintain high rates of action potential firing and transmitter release. Taking advantage of diverse fast-firing capacities among medial vestibular nucleus neurons of mice, we identify a group of ion channel, synaptic, and structural genes that exhibit mutually correlated expression levels, which covary with firing capacity. Coexpression of this fast-spiking gene module may be a basic strategy for neurons to efficiently and coordinately tune the speed of action potential generation and propagation and transmitter release at presynaptic terminals., (Copyright © 2020 the authors.)

Published

2020

16. Multiple types of cerebellar target neurons and their circuitry in the vestibulo-ocular reflex.

Author

Shin M, Moghadam SH, Sekirnjak C, Bagnall MW, Kolkman KE, Jacobs R, Faulstich M, and du Lac S

Subjects

Animals, Biophysics, Biotin analogs & derivatives, Biotin metabolism, Calbindins, Cerebellum ultrastructure, Dextrans metabolism, Electric Stimulation, Female, Glutamate Decarboxylase genetics, Glycine Plasma Membrane Transport Proteins genetics, In Vitro Techniques, Luminescent Proteins genetics, Male, Membrane Potentials genetics, Membrane Potentials physiology, Mice, Mice, Transgenic, Microscopy, Electron, Transmission methods, Nerve Net cytology, Nerve Net ultrastructure, Neurons classification, Neurons ultrastructure, Patch-Clamp Techniques, Rhodamines metabolism, S100 Calcium Binding Protein G metabolism, Synapses genetics, Synapses physiology, Vestibular Nuclei cytology, Vestibular Nuclei physiology, tau Proteins genetics, Cerebellum cytology, Nerve Net physiology, Neurons physiology, Reflex, Vestibulo-Ocular physiology

Abstract

The cerebellum influences behavior and cognition exclusively via Purkinje cell synapses onto neurons in the deep cerebellar and vestibular nuclei. In contrast with the rich information available about the organization of the cerebellar cortex and its synaptic inputs, relatively little is known about microcircuitry postsynaptic to Purkinje cells. Here we examined the cell types and microcircuits through which Purkinje cells influence an oculomotor behavior controlled by the cerebellum, the horizontal vestibulo-ocular reflex, which involves only two eye muscles. Using a combination of anatomical tracing and electrophysiological recordings in transgenic mouse lines, we identified several classes of neurons in the medial vestibular nucleus that receive Purkinje cell synapses from the cerebellar flocculus. Glycinergic and glutamatergic flocculus target neurons (FTNs) with somata densely surrounded by Purkinje cell terminals projected axons to the ipsilateral abducens and oculomotor nuclei, respectively. Of three additional types of FTNs that were sparsely innervated by Purkinje cells, glutamatergic and glycinergic neurons projected to the contralateral and ipsilateral abducens, respectively, and GABAergic neurons projected to contralateral vestibular nuclei. Densely innervated FTNs had high spontaneous firing rates and pronounced postinhibitory rebound firing, and were physiologically homogeneous, whereas the intrinsic excitability of sparsely innervated FTNs varied widely. Heterogeneity in the molecular expression, physiological properties, and postsynaptic targets of FTNs implies that Purkinje cell activity influences the neural control of eye movements in several distinct ways. These results indicate that the cerebellum regulates a simple reflex behavior via at least five different cell types that are postsynaptic to Purkinje cells.

Published

2011

17. Intrinsic physiology of identified neurons in the prepositus hypoglossi and medial vestibular nuclei.

Author

Kolkman KE, Moghadam SH, and du Lac S

Subjects

Animals, Medulla Oblongata cytology, Mice, Mice, Transgenic, Reflex, Vestibulo-Ocular physiology, Vestibular Nuclei cytology, Action Potentials physiology, Medulla Oblongata physiology, Neurons physiology, Vestibular Nuclei physiology

Abstract

Signal processing in the vestibular system is influenced by the intrinsic physiological properties of neurons that differ in neurotransmitters and circuit connections. Do membrane and firing properties differ across functionally distinct cell types? This study examines the intrinsic physiology of neurons in the medial vestibular nucleus (MVN) and nucleus prepositus hypoglossi (NPH) which express different neurotransmitters and have distinct axonal projections. NPH neurons expressing fluorescent proteins in glutamatergic, glycinergic, or GABAergic neurons were targeted for whole-cell patch recordings in brainstem slices obtained from transgenic mouse lines (YFP-16, GlyT2, and GIN). Recordings from MVN neurons projecting to the spinal cord, reticular formation, or oculomotor nucleus were obtained by targeting fluorescent neurons retrogradely labeled from tracer injections. Intrinsic physiological properties of identified neurons exhibited continuous variations but tended to differ between functionally defined cell types. Within the NPH, YFP-16 neurons had the narrowest action potentials and highest evoked firing rates and expressed high levels of Kv3.3 proteins, which speed repolarization. MVN neurons projecting to the spinal cord and oculomotor nucleus had similar action potential waveforms, but oculomotor-projecting neurons had higher intrinsic gains than those projecting to the spinal cord. These results indicate that intrinsic membrane properties are differentially tuned in MVN and NPH neurons subserving different functions.

Published

2011