Your search keyword '"Golding NL"' showing total 31 results

1. Directional Hearing by Linear Summation of Binaural Inputs at the Medial Superior Olive (vol 78, pg 936, 2013)

Author

Heyden, Marcel, Lorteije, Jeannette, Plauska, Andrius, Roberts, MT, Golding, NL, Borst, Gerard, and Neurosciences

Published

2013

2. Context-dependent synaptic action of glycinergic and GABAergic inputs in the dorsal cochlear nucleus

Author

Golding, NL, primary and Oertel, D, additional

Published

1996

3. Recordings from slices indicate that octopus cells of the cochlear nucleus detect coincident firing of auditory nerve fibers with temporal precision

Author

Golding, NL, primary, Robertson, D, additional, and Oertel, D, additional

Published

1995

4. Physiological Diversity Influences Detection of Stimulus Envelope and Fine Structure in Neurons of the Medial Superior Olive.

Author

Bondy BJ, Haimes DB, and Golding NL

Abstract

The neurons of the medial superior olive (MSO) of mammals extract azimuthal information from the delays between sounds reaching the two ears [interaural time differences (ITDs)]. Traditionally, all models of sound localization have assumed that MSO neurons represent a single population of cells with specialized and homogeneous intrinsic and synaptic properties that enable the detection of synaptic coincidence on a timescale of tens to hundreds of microseconds. Here, using patch-clamp recordings from large populations of anatomically labeled neurons in brainstem slices from male and female Mongolian gerbils ( Meriones unguiculatu s), we show that MSO neurons are far more physiologically diverse than previously appreciated, with properties that depend regionally on cell position along the topographic map of frequency. Despite exhibiting a similar morphology, neurons in the MSO exhibit subthreshold oscillations of differing magnitudes that drive action potentials at rates between 100 and 800 Hz. These oscillations are driven primarily by voltage-gated sodium channels and are distinct from resonant properties derived from other active membrane properties. We show that graded differences in these and other physiological properties across the MSO neuron population enable the MSO to duplex the encoding of ITD information in both fast, submillisecond time-varying signals as well as in slower envelopes. SIGNIFICANCE STATEMENT Neurons in the medial superior olive (MSO) encode sound localization cues by detecting microsecond differences in the arrival times of inputs from the left and right ears, and it has been assumed that this computation is made possible by highly stereotyped structural and physiological specializations. Here we report using a large (>400) sample size in which MSO neurons show a strikingly large continuum of functional properties despite exhibiting similar morphologies. We demonstrate that subthreshold oscillations mediated by voltage-gated Na + channels play a key role in conferring graded differences in firing properties. This functional diversity likely confers capabilities of processing both fast, submillisecond-scale synaptic activity (acoustic "fine structure"), and slow-rising envelope information that is found in amplitude-modulated sounds and speech patterns., (Copyright © 2021 the authors.)

Published

2021

5. Glycinergic axonal inhibition subserves acute spatial sensitivity to sudden increases in sound intensity.

Author

Franken TP, Bondy BJ, Haimes DB, Goldwyn JH, Golding NL, Smith PH, and Joris PX

Subjects

Animals, Excitatory Postsynaptic Potentials physiology, Female, Gerbillinae, Glycine metabolism, Inhibitory Postsynaptic Potentials physiology, Male, Neurons physiology, Olivary Nucleus cytology, Olivary Nucleus physiology, Sound Localization physiology

Abstract

Locomotion generates adventitious sounds which enable detection and localization of predators and prey. Such sounds contain brisk changes or transients in amplitude. We investigated the hypothesis that ill-understood temporal specializations in binaural circuits subserve lateralization of such sound transients, based on different time of arrival at the ears (interaural time differences, ITDs). We find that Lateral Superior Olive (LSO) neurons show exquisite ITD-sensitivity, reflecting extreme precision and reliability of excitatory and inhibitory postsynaptic potentials, in contrast to Medial Superior Olive neurons, traditionally viewed as the ultimate ITD-detectors. In vivo, inhibition blocks LSO excitation over an extremely short window, which, in vitro, required synaptically evoked inhibition. Light and electron microscopy revealed inhibitory synapses on the axon initial segment as the structural basis of this observation. These results reveal a neural vetoing mechanism with extreme temporal and spatial precision and establish the LSO as the primary nucleus for binaural processing of sound transients., Competing Interests: TF, BB, DH, JG, NG, PS, PJ No competing interests declared, (© 2021, Franken et al.)

Published

2021

6. Excitatory cholecystokinin neurons of the midbrain integrate diverse temporal responses and drive auditory thalamic subdomains.

Author

Kreeger LJ, Connelly CJ, Mehta P, Zemelman BV, and Golding NL

Subjects

Animals, Female, Gerbillinae, Male, Auditory Pathways metabolism, Cholecystokinin metabolism, Evoked Potentials, Auditory, Mesencephalon metabolism, Neurons metabolism, Thalamus metabolism

Abstract

The central nucleus of the inferior colliculus (ICC) integrates information about different features of sound and then distributes this information to thalamocortical circuits. However, the lack of clear definitions of circuit elements in the ICC has limited our understanding of the nature of these circuit transformations. Here, we combine virus-based genetic access with electrophysiological and optogenetic approaches to identify a large family of excitatory, cholecystokinin-expressing thalamic projection neurons in the ICC of the Mongolian gerbil. We show that these neurons form a distinct cell type, displaying uniform morphology and intrinsic firing features, and provide powerful, spatially restricted excitation exclusively to the ventral auditory thalamus. In vivo, these neurons consistently exhibit V-shaped receptive field properties but strikingly diverse temporal responses to sound. Our results indicate that temporal response diversity is maintained within this population of otherwise uniform cells in the ICC and then relayed to cortex through spatially restricted thalamic subdomains., Competing Interests: The authors declare no competing interest., (Copyright © 2021 the Author(s). Published by PNAS.)

Published

2021

7. De novo sequencing and initial annotation of the Mongolian gerbil (Meriones unguiculatus) genome.

Author

Zorio DAR, Monsma S, Sanes DH, Golding NL, Rubel EW, and Wang Y

Subjects

Animals, Base Sequence, Male, Molecular Sequence Annotation, Genome, Gerbillinae genetics, Sequence Analysis, DNA

Abstract

The Mongolian gerbil (Meriones unguiculatus) is a member of the rodent family that displays several features not found in mice or rats, including sensory specializations and social patterns more similar to those in humans. These features have made gerbils a valuable animal for research studies of auditory and visual processing, brain development, learning and memory, and neurological disorders. Here, we report the whole gerbil annotated genome sequence, and identify important similarities and differences to the human and mouse genomes. We further analyze the chromosomal structure of eight genes with high relevance for controlling neural signaling and demonstrate a high degree of homology between these genes in mouse and gerbil. This homology increases the likelihood that individual genes can be rapidly identified in gerbil and used for genetic manipulations. The availability of the gerbil genome provides a foundation for advancing our knowledge towards understanding evolution, behavior and neural function in mammals. ACCESSION NUMBER: The Whole Genome Shotgun sequence data from this project has been deposited at DDBJ/ENA/GenBank under the accession NHTI00000000. The version described in this paper is version NHTI01000000. The fragment reads, and mate pair reads have been deposited in the Sequence Read Archive under BioSample accession SAMN06897401., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published

2019

8. Glycinergic Inhibitory Plasticity in Binaural Neurons Is Cumulative and Gated by Developmental Changes in Action Potential Backpropagation.

Author

Winters BD and Golding NL

Subjects

Animals, Female, Gerbillinae, Male, Olivary Nucleus physiology, Action Potentials physiology, Inhibitory Postsynaptic Potentials physiology, Neural Inhibition physiology, Neuronal Plasticity physiology, Neurons physiology, Receptors, Glycine physiology

Abstract

Utilization of timing-based sound localization cues by neurons in the medial superior olive (MSO) depends critically on glycinergic inhibitory inputs. After hearing onset, the strength and subcellular location of these inhibitory inputs are dramatically altered, but the cellular processes underlying this experience-dependent refinement are unknown. Here we reveal a form of inhibitory long-term potentiation (iLTP) in MSO neurons that is dependent on spiking and synaptic activation but is not affected by their fine-scale relative timing at higher frequencies prevalent in auditory circuits. We find that iLTP reinforces inhibitory inputs coactive with binaural excitation in a cumulative manner, likely well suited for networks featuring persistent high-frequency activity. We also show that a steep drop in action potential size and backpropagation limits induction of iLTP to the first 2 weeks of hearing. These intrinsic changes would deprive more distal inhibitory synapses of reinforcement, conceivably establishing the mature, soma-biased pattern of inhibition., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published

2018

9. Amplitude Normalization of Dendritic EPSPs at the Soma of Binaural Coincidence Detector Neurons of the Medial Superior Olive.

Author

Winters BD, Jin SX, Ledford KR, and Golding NL

Subjects

Animals, Cells, Cultured, Female, Gerbillinae, Male, Dendrites physiology, Excitatory Postsynaptic Potentials physiology, Sensory Receptor Cells physiology, Sound Localization physiology, Superior Olivary Complex physiology, Synapses physiology

Abstract

The principal neurons of the medial superior olive (MSO) encode cues for horizontal sound localization through comparisons of the relative timing of EPSPs. To understand how the timing and amplitude of EPSPs are maintained during propagation in the dendrites, we made dendritic and somatic whole-cell recordings from MSO principal neurons in brain slices from Mongolian gerbils. In somatic recordings, EPSP amplitudes were largely uniform following minimal stimulation of excitatory synapses at visualized locations along the dendrites. Similar results were obtained when excitatory synaptic transmission was eliminated in a low calcium solution and then restored at specific dendritic sites by pairing input stimulation and focal application of a higher calcium solution. We performed dual dendritic and somatic whole-cell recordings to measure spontaneous EPSPs using a dual-channel template-matching algorithm to separate out those events initiated at or distal to the dendritic recording location. Local dendritic spontaneous EPSP amplitudes increased sharply in the dendrite with distance from the soma (length constant, 53.6 μm), but their attenuation during propagation resulted in a uniform amplitude of ∼0.2 mV at the soma. The amplitude gradient of dendritic EPSPs was also apparent in responses to injections of identical simulated excitatory synaptic currents in the dendrites. Compartmental models support the view that these results extensively reflect the influence of dendritic cable properties. With relatively few excitatory axons innervating MSO neurons, the normalization of dendritic EPSPs at the soma would increase the importance of input timing versus location during the processing of interaural time difference cues in vivo SIGNIFICANCE STATEMENT The neurons of the medial superior olive analyze cues for sound localization by detecting the coincidence of binaural excitatory synaptic inputs distributed along the dendrites. Previous studies have shown that dendritic voltages undergo severe attenuation as they propagate to the soma, potentially reducing the influence of distal inputs. However, using dendritic and somatic patch recordings, we found that dendritic EPSP amplitude increased with distance from the soma, compensating for dendritic attenuation and normalizing EPSP amplitude at the soma. Much of this normalization reflected the influence of dendritic morphology. As different combinations of presynaptic axons may be active during consecutive cycles of sound stimuli, somatic EPSP normalization renders spike initiation more sensitive to synapse timing than dendritic location., (Copyright © 2017 the authors 0270-6474/17/373138-12$15.00/0.)

Published

2017

10. Serotonin modulates spike probability in the axon initial segment through HCN channels.

Author

Ko KW, Rasband MN, Meseguer V, Kramer RH, and Golding NL

Subjects

Animals, Axons physiology, Dendrites physiology, Gerbillinae, Patch-Clamp Techniques methods, Action Potentials physiology, Axon Initial Segment metabolism, Cyclic Nucleotide-Gated Cation Channels metabolism, Hyperpolarization-Activated Cyclic Nucleotide-Gated Channels metabolism, Serotonin metabolism

Abstract

The axon initial segment (AIS) serves as the site of action potential initiation in most neurons, but difficulties in isolating the effects of voltage-gated ion channels in the AIS from those of the soma and dendrites have hampered understanding how AIS properties influence neural coding. Here we have combined confocal microscopy, patch-clamp recordings and light-sensitive channel blockers ('photoswitches') in binaural auditory gerbil neurons to show that hyperpolarization and cyclic-nucleotide-gated (HCN) channels are expressed in the AIS and decrease spike probability, in a manner distinct from that of HCN channels in the soma and dendrites. Furthermore, the control of spike threshold by HCN channels in the AIS can be altered through serotonergic modulation of 5-hydroxytryptamine 1A (5-HT1A) receptors, which hyperpolarizes the activation range of HCN channels. As release of serotonin signals changes in motivation and attention states, axonal HCN channels provide a mechanism to translate these signals into changes in the threshold for sensory stimuli.

Published

2016

11. In vivo coincidence detection in mammalian sound localization generates phase delays.

Author

Franken TP, Roberts MT, Wei L, Golding NL, and Joris PX

Subjects

Acoustic Stimulation, Animals, Dose-Response Relationship, Drug, Excitatory Amino Acid Antagonists pharmacology, Excitatory Postsynaptic Potentials physiology, Female, Gerbillinae, Glycine Agents pharmacology, In Vitro Techniques, Male, Patch-Clamp Techniques, Psychoacoustics, Quinoxalines pharmacology, Reaction Time physiology, Signal Detection, Psychological drug effects, Strychnine pharmacology, Auditory Pathways cytology, Brain cytology, Neurons physiology, Signal Detection, Psychological physiology, Sound Localization

Abstract

Sound localization critically depends on detection of differences in arrival time of sounds at the two ears (acoustic delay). The fundamental mechanisms are debated, but all proposals include a process of coincidence detection and a separate source of internal delay that offsets the acoustic delay and determines neural tuning. We used in vivo patch-clamp recordings of binaural neurons in the Mongolian gerbil and pharmacological manipulations to directly compare neuronal input to output and to separate excitation from inhibition. Our results cannot be accounted for by existing models and reveal that coincidence detection is not an instantaneous process, but is instead shaped by the interaction of intrinsic conductances with preceding synaptic activity. This interaction generates an internal delay as an intrinsic part of the process of coincidence detection. The multiplication and time-shifting stages thought to extract synchronous activity in many brain areas can therefore be combined in a single operation.

Published

2015

12. The relative contributions of MNTB and LNTB neurons to inhibition in the medial superior olive assessed through single and paired recordings.

Author

Roberts MT, Seeman SC, and Golding NL

Subjects

Action Potentials physiology, Animals, Cochlear Nerve physiology, Gerbillinae, Synapses physiology, Auditory Pathways physiology, Neural Inhibition physiology, Neurons physiology, Olivary Nucleus physiology, Pons physiology

Abstract

The medial superior olive (MSO) senses microsecond differences in the coincidence of binaural signals, a critical cue for detecting sound location along the azimuth. An important component of this circuit is provided by inhibitory neurons of the medial and lateral nuclei of the trapezoid body (MNTB and LNTB, respectively). While MNTB neurons are fairly well described, little is known about the physiology of LNTB neurons. Using whole cell recordings from gerbil brainstem slices, we found that LNTB and MNTB neurons have similar membrane time constants and input resistances and fire brief action potentials, but only LNTB neurons fire repetitively in response to current steps. We observed that LNTB neurons receive graded excitatory and inhibitory synaptic inputs, with at least some of the latter arriving from other LNTB neurons. To address the relative timing of inhibition to the MSO from the LNTB versus the MNTB, we examined inhibitory responses to auditory nerve stimulation using a slice preparation that retains the circuitry from the auditory nerve to the MSO intact. Despite the longer physical path length of excitatory inputs driving contralateral inhibition, inhibition from both pathways arrived with similar latency and jitter. An analysis of paired whole cell recordings between MSO and MNTB neurons revealed a short and reliable delay between the action potential peak in MNTB neurons and the onset of the resulting IPSP (0.55 ± 0.01 ms, n = 4, mean ± SEM). Reconstructions of biocytin-labeled neurons showed that MNTB axons ranged from 580 to 858 μm in length (n = 4). We conclude that while both LNTB and MNTB neurons provide similarly timed inhibition to MSO neurons, the reliability of inhibition from the LNTB at higher frequencies is more constrained relative to that from the MNTB due to differences in intrinsic properties, the strength of excitatory inputs, and the presence of feedforward inhibition.

Published

2014

13. Directional hearing by linear summation of binaural inputs at the medial superior olive.

Author

van der Heijden M, Lorteije JA, Plauška A, Roberts MT, Golding NL, and Borst JG

Subjects

Acoustic Stimulation, Action Potentials, Animals, Animals, Newborn, Auditory Pathways physiology, Biophysical Phenomena, Brain Mapping, Electric Stimulation, Gerbillinae, In Vitro Techniques, Inhibitory Postsynaptic Potentials physiology, Models, Neurological, Neural Inhibition physiology, Olivary Nucleus cytology, Patch-Clamp Techniques, Reaction Time, Functional Laterality physiology, Hearing, Linear Models, Neurons physiology, Olivary Nucleus physiology, Sound Localization physiology

Abstract

Neurons in the medial superior olive (MSO) enable sound localization by their remarkable sensitivity to submillisecond interaural time differences (ITDs). Each MSO neuron has its own "best ITD" to which it responds optimally. A difference in physical path length of the excitatory inputs from both ears cannot fully account for the ITD tuning of MSO neurons. As a result, it is still debated how these inputs interact and whether the segregation of inputs to opposite dendrites, well-timed synaptic inhibition, or asymmetries in synaptic potentials or cellular morphology further optimize coincidence detection or ITD tuning. Using in vivo whole-cell and juxtacellular recordings, we show here that ITD tuning of MSO neurons is determined by the timing of their excitatory inputs. The inputs from both ears sum linearly, whereas spike probability depends nonlinearly on the size of synaptic inputs. This simple coincidence detection scheme thus makes accurate sound localization possible., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2013

14. A mechanistic understanding of the role of feedforward inhibition in the mammalian sound localization circuitry.

Author

Roberts MT, Seeman SC, and Golding NL

Subjects

4-Aminopyridine pharmacology, Action Potentials drug effects, Action Potentials physiology, Animals, Animals, Newborn, Auditory Pathways physiology, Biophysical Phenomena drug effects, Biophysical Phenomena physiology, Biophysics, Elapid Venoms pharmacology, Electric Stimulation, Excitatory Postsynaptic Potentials physiology, Functional Laterality, Gerbillinae, In Vitro Techniques, Nerve Net drug effects, Neural Inhibition drug effects, Neurons drug effects, Neurotoxins pharmacology, Potassium Channel Blockers pharmacology, Nerve Net physiology, Neural Inhibition physiology, Neurons physiology, Olivary Nucleus cytology, Sound Localization physiology

Abstract

Feedforward inhibition sharpens the precision of neurons throughout ascending auditory pathways, including the binaural neurons of the medial superior olive (MSO). However, the biophysical influence of inhibition is poorly understood, particularly at higher frequencies at which the relative phase of inhibition and excitation becomes ambiguous. Here, we show in gerbil MSO principal cells in vitro that feedforward inhibition precedes direct excitation, providing a concurrent hyperpolarization and conductance shunt during EPSP summation. We show with dual-patch recordings and dynamic clamp that both the linearity and temporal fidelity of synaptic integration is improved by reducing Kv1 potassium channel conductance during inhibition, which counters membrane shunting even at high frequencies at which IPSPs sum. The reduction of peak excitation by preceding inhibition lowers spike probability, narrowing but not shifting the window for detecting binaural coincidence. The interplay between inhibition and potassium conductances thus improves the consistency and resolution of ITD coding across different frequencies., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2013

15. Synaptic integration in dendrites: exceptional need for speed.

Author

Golding NL and Oertel D

Subjects

Animals, Auditory Pathways physiology, Excitatory Postsynaptic Potentials, Octopodiformes, Reaction Time, Dendrites physiology, Synapses physiology

Abstract

Some neurons in the mammalian auditory system are able to detect and report the coincident firing of inputs with remarkable temporal precision. A strong, low-voltage-activated potassium conductance (g(KL)) at the cell body and dendrites gives these neurons sensitivity to the rate of depolarization by EPSPs, allowing neurons to assess the coincidence of the rising slopes of unitary EPSPs. Two groups of neurons in the brain stem, octopus cells in the posteroventral cochlear nucleus and principal cells of the medial superior olive (MSO), extract acoustic information by assessing coincident firing of their inputs over a submillisecond timescale and convey that information at rates of up to 1000 spikes s(-1). Octopus cells detect the coincident activation of groups of auditory nerve fibres by broadband transient sounds, compensating for the travelling wave delay by dendritic filtering, while MSO neurons detect coincident activation of similarly tuned neurons from each of the two ears through separate dendritic tufts. Each makes use of filtering that is introduced by the spatial distribution of inputs on dendrites.

Published

2012

16. GABAB receptors sharpen tuning of a sound localization circuit.

Author

Roberts MT and Golding NL

Subjects

Animals, Olivary Nucleus physiology, Receptors, GABA-B physiology, Sound Localization physiology

Published

2012

17. An essential role for modulation of hyperpolarization-activated current in the development of binaural temporal precision.

Author

Khurana S, Liu Z, Lewis AS, Rosa K, Chetkovich D, and Golding NL

Subjects

Age Factors, Analysis of Variance, Androstadienes pharmacology, Animals, Biophysical Phenomena drug effects, Bucladesine pharmacology, Colforsin pharmacology, Cyclic Nucleotide-Gated Cation Channels genetics, Cyclic Nucleotide-Gated Cation Channels metabolism, Electric Stimulation, Enzyme Inhibitors pharmacology, Female, Gene Expression Regulation, Developmental drug effects, Gerbillinae, Imidazoles pharmacology, In Vitro Techniques, Ion Channel Gating drug effects, Male, Neurons drug effects, Olivary Nucleus cytology, Olivary Nucleus growth & development, Patch-Clamp Techniques, Pyridines pharmacology, Pyrimidines pharmacology, Wortmannin, Biophysical Phenomena physiology, Gene Expression Regulation, Developmental physiology, Ion Channel Gating physiology, Neurons physiology

Abstract

In sensory circuits of the brain, developmental changes in the expression and modulation of voltage-gated ion channels are a common occurrence, but such changes are often difficult to assign to clear functional roles. We have explored this issue in the binaural neurons of the medial superior olive (MSO), whose temporal precision in detecting the coincidence of binaural inputs dictates the resolution of azimuthal sound localization. We show that in MSO principal neurons of gerbils during the first week of hearing, a hyperpolarization-activated current (I(h)) progressively undergoes a 13-fold increase in maximal conductance, a >10-fold acceleration of kinetics, and, most surprisingly, a 30 mV depolarizing shift in the voltage dependence of activation. This period is associated with an upregulation of the hyperpolarization-activated and cyclic nucleotide-gated (HCN) channel subunits HCN1, HCN2, and HCN4 in the MSO, but only HCN1 and HCN4 were expressed strongly in principal neurons. I(h) recorded in nucleated patches from electrophysiologically mature MSO neurons (>P18) exhibited kinetics and an activation range nearly identical to the I(h) found in whole-cell recordings before hearing onset. These results indicate that the developmental changes in I(h) in MSO neurons can be explained predominantly by modulation from diffusible intracellular factors, and not changes in channel subunit composition. The exceptionally large modulatory changes in I(h), together with refinements in synaptic properties transform the coding strategy from one of summation and integration to the submillisecond coincidence detection known to be required for transmission of sound localization cues.

Published

2012

18. Dynamic interaction of Ih and IK-LVA during trains of synaptic potentials in principal neurons of the medial superior olive.

Author

Khurana S, Remme MW, Rinzel J, and Golding NL

Subjects

Animals, Animals, Newborn, Biophysics, Cardiotonic Agents pharmacology, Computer Simulation, Electric Stimulation methods, Female, Gerbillinae, In Vitro Techniques, Ion Channel Gating drug effects, Male, Models, Neurological, Neurons drug effects, Normal Distribution, Patch-Clamp Techniques, Peptides pharmacology, Potassium Channels, Voltage-Gated drug effects, Pyrimidines pharmacology, Synaptic Potentials drug effects, Time Factors, Ion Channel Gating physiology, Neurons physiology, Nonlinear Dynamics, Olivary Nucleus cytology, Potassium Channels, Voltage-Gated physiology, Synaptic Potentials physiology

Abstract

In neurons of the medial superior olive (MSO), voltage-gated ion channels control the submillisecond time resolution of binaural coincidence detection, but little is known about their interplay during trains of synaptic activity that would be experienced during auditory stimuli. Here, using modeling and patch-clamp recordings from MSO principal neurons in gerbil brainstem slices, we examined interactions between two major currents controlling subthreshold synaptic integration: a low-voltage-activated potassium current (I(K-LVA)) and a hyperpolarization-activated cation current (I(h)). Both I(h) and I(K-LVA) contributed strongly to the resting membrane conductance and, during trains of simulated EPSPs, exhibited cumulative deactivation and inactivation, respectively. In current-clamp recordings, regular and irregular trains of simulated EPSCs increased input resistance up to 60%, effects that accumulated and decayed (after train) over hundreds of milliseconds. Surprisingly, the mean voltage and peaks of EPSPs increased by only a few millivolts during trains. Using a model of an MSO cell, we demonstrated that the nearly uniform response during modest depolarizing stimuli relied on changes in I(h) and I(K-LVA), such that their sum remained nearly constant over time. Experiments and modeling showed that, for simplified binaural stimuli (EPSC pairs in a noisy background), spike probability gradually increased in parallel with the increasing input resistance. Nevertheless, the interplay between I(h) and I(K-LVA) helps to maintain a nearly uniform shape of individual synaptic responses, and we show that the time resolution of synaptic coincidence detection can be maintained during trains if EPSC size gradually decreases (as in synaptic depression), counteracting slow increases in excitability.

Published

2011

19. Control of submillisecond synaptic timing in binaural coincidence detectors by K(v)1 channels.

Author

Mathews PJ, Jercog PE, Rinzel J, Scott LL, and Golding NL

Subjects

Age Factors, Animals, Animals, Newborn, Biophysics, Brain Stem cytology, Dendrites physiology, Elapid Venoms pharmacology, Electric Stimulation methods, Excitatory Postsynaptic Potentials physiology, Gerbillinae, In Vitro Techniques, Models, Neurological, Neurons cytology, Patch-Clamp Techniques methods, Reaction Time drug effects, Time Factors, Neurons physiology, Reaction Time physiology, Shaker Superfamily of Potassium Channels metabolism, Synapses physiology

Abstract

Neurons in the medial superior olive process sound-localization cues via binaural coincidence detection, in which excitatory synaptic inputs from each ear are segregated onto different branches of a bipolar dendritic structure and summed at the soma and axon with submillisecond time resolution. Although synaptic timing and dynamics critically shape this computation, synaptic interactions with intrinsic ion channels have received less attention. Using paired somatic and dendritic patch-clamp recordings in gerbil brainstem slices together with compartmental modeling, we found that activation of K(v)1 channels by dendritic excitatory postsynaptic potentials (EPSPs) accelerated membrane repolarization in a voltage-dependent manner and actively improved the time resolution of synaptic integration. We found that a somatically biased gradient of K(v)1 channels underlies the degree of compensation for passive cable filtering during propagation of EPSPs in dendrites. Thus, both the spatial distribution and properties of K(v)1 channels are important for preserving binaural synaptic timing.

Published

2010

20. Perisomatic voltage-gated sodium channels actively maintain linear synaptic integration in principal neurons of the medial superior olive.

Author

Scott LL, Mathews PJ, and Golding NL

Subjects

Action Potentials, Animals, Dendrites physiology, Gerbillinae, In Vitro Techniques, Ion Channel Gating, Patch-Clamp Techniques, Synaptic Potentials, Neurons physiology, Olivary Nucleus physiology, Sodium Channels physiology, Synapses physiology

Abstract

Principal neurons of the medial superior olive (MSO) compute azimuthal sound location by integrating phase-locked inputs from each ear. While previous experimental and modeling studies have proposed that voltage-gated sodium channels (VGSCs) play an important role in synaptic integration in the MSO, these studies appear at odds with the unusually weak active backpropagation of action potentials into the soma and dendrites. To understand the spatial localization and biophysical properties of VGSCs, we isolated sodium currents in MSO principal neurons in gerbil brainstem slices. Nucleated and cell-attached patches revealed that VGSC density at the soma is comparable to that of many other neuron types, but channel expression is largely absent from the dendrites. Further, while somatic VGSCs activated with conventional voltage dependence (V(1/2) = -30 mV), they exhibited an unusually negative range of steady-state inactivation (V(1/2) = -77 mV), leaving approximately 92% of VGSCs inactivated at the resting potential (approximately -58 mV). In current-clamp experiments, non-inactivated VGSCs were sufficient to amplify subthreshold EPSPs near action potential threshold, counterbalancing the suppression of EPSP peaks by low voltage-activated potassium channels. EPSP amplification was restricted to the perisomatic region of the neuron, and relatively insensitive to preceding inhibition. Finally, computational modeling showed that the exclusion of VGSCs from the dendrites equalizes somatic EPSP amplification across synaptic locations and lowered the threshold for bilateral versus unilateral excitatory synaptic inputs. Together, these findings suggest that the pattern of sodium channel expression in MSO neurons contributes to these neurons' selectivity for coincident binaural inputs.

Published

2010

21. Weak action potential backpropagation is associated with high-frequency axonal firing capability in principal neurons of the gerbil medial superior olive.

Author

Scott LL, Hage TA, and Golding NL

Subjects

Action Potentials, Animals, Auditory Pathways chemistry, Auditory Pathways cytology, Axons chemistry, Dendrites physiology, Gerbillinae, In Vitro Techniques, Myelin Basic Protein analysis, Nerve Fibers, Myelinated chemistry, Nerve Fibers, Myelinated physiology, Neurons chemistry, Olivary Nucleus chemistry, Olivary Nucleus cytology, Patch-Clamp Techniques, Synaptic Transmission, Time Factors, Auditory Pathways physiology, Axons physiology, Neural Conduction, Neurons physiology, Olivary Nucleus physiology, Sound Localization

Abstract

Principal neurons of the medial superior olive (MSO) convey azimuthal sound localization cues through modulation of their rate of action potential firing. Previous intracellular studies in vitro have shown that action potentials appear highly attenuated at the soma of MSO neurons, potentially reflecting specialized action potential initiation and/or a physically distant site of generation. To examine this more directly, we made dual patch-clamp recordings from MSO principal neurons in gerbil brainstem slices. Using somatic and dendritic whole-cell recordings, we show that graded action potentials at the soma are highly sensitive to the rate of rise of excitation and undergo strong attenuation in their backpropagation into the dendrites (length constant, 76 microm), particularly during strong dendritic excitation. Using paired somatic whole-cell and axonal loose-patch recordings, we show that action potentials recorded in the axon at distances > 25 microm are all-or-none, and uniform in amplitude even when action potentials appear graded at the soma. This proximal zone corresponded to the start of myelination in the axon, as assessed with immunocytochemical staining for myelin basic protein in single-labelled neurons. Finally, the axon was capable of sustaining remarkably high firing rates, with perfect entrainment occurring at frequencies of up to 1 kHz. Together, our findings show that action potential signalling in MSO principal neurons is highly secure, but shows a restricted invasion of the somatodendritic compartment of the cell. This restriction may be important for minimizing distortions in synaptic integration during the high frequencies of synaptic input encountered in the MSO.

Published

2007

22. Factors mediating powerful voltage attenuation along CA1 pyramidal neuron dendrites.

Author

Golding NL, Mickus TJ, Katz Y, Kath WL, and Spruston N

Subjects

Animals, Excitatory Postsynaptic Potentials physiology, Hippocampus ultrastructure, In Vitro Techniques, Male, Models, Neurological, Neural Conduction physiology, Patch-Clamp Techniques, Pyramidal Cells ultrastructure, Rats, Rats, Wistar, Synaptic Transmission, Dendrites physiology, Hippocampus physiology, Pyramidal Cells physiology

Abstract

We performed simultaneous patch-electrode recordings from the soma and apical dendrite of CA1 pyramidal neurons in hippocampal slices, in order to determine the degree of voltage attenuation along CA1 dendrites. Fifty per cent attenuation of steady-state somatic voltage changes occurred at a distance of 238 microm from the soma in control and 409 microm after blocking the hyperpolarization-activated (H) conductance. The morphology of three neurons was reconstructed and used to generate computer models, which were adjusted to fit the somatic and dendritic voltage responses. These models identify several factors contributing to the voltage attenuation along CA1 dendrites, including high axial cytoplasmic resistivity, low membrane resistivity, and large H conductance. In most cells the resting membrane conductances, including the H conductances, were larger in the dendrites than the soma. Simulations suggest that synaptic potentials attenuate enormously as they propagate from the dendrite to the soma, with greater than 100-fold attenuation for synapses on many small, distal dendrites. A prediction of this powerful EPSP attenuation is that distal synaptic inputs are likely only to be effective in the presence of conductance scaling, dendritic excitability, or both.

Published

2005

23. Posthearing developmental refinement of temporal processing in principal neurons of the medial superior olive.

Author

Scott LL, Mathews PJ, and Golding NL

Subjects

Age Factors, Animals, Animals, Newborn, Auditory Perception physiology, Gerbillinae, In Vitro Techniques, Olivary Nucleus cytology, Olivary Nucleus physiology, Time Perception physiology, Excitatory Postsynaptic Potentials physiology, Hearing physiology, Neurons physiology, Olivary Nucleus growth & development

Abstract

In mammals, principal neurons of the medial superior olive (MSO) exhibit biophysical specializations that enable them to detect sound localization cues with microsecond precision. In the present study, we used whole-cell patch recordings to examine the development of the intrinsic electrical properties of these neurons in brainstem slices from postnatal day 14 (P14) to P38 gerbils. In the week after hearing onset (P14-P21), we observed dramatic reductions in somatic EPSP duration, input resistance, and membrane time constant. Surprisingly, somatically recorded action potentials also dramatically declined in amplitude over a similar period (38 +/- 3 to 17 +/- 2 mV; tau = 5.2 d). Simultaneous somatic and dendritic patch recordings revealed that these action potentials were initiated in the axon, which primarily emerged from the soma. In older gerbils, the rapid speed of membrane voltage changes and the attenuation of action potential amplitudes were mediated extensively by low voltage-activated potassium channels containing the Kv1.1 subunit. In addition, whole-cell voltage-clamp recordings revealed that these potassium channels increase nearly fourfold from P14 to P23 and are thus a major component of developmental changes in excitability. Finally, the electrophysiological features of principal neurons of the medial nucleus of the trapezoid body did not change after P14, indicating that posthearing regulation of intrinsic membrane properties is not a general feature of all time-coding auditory neurons. We suggest that the striking electrical segregation of the axon from the soma and dendrites of MSO principal neurons minimizes spike-induced distortion of synaptic potentials and thus preserves the accuracy of binaural comparisons.

Published

2005

24. Dendritic spikes as a mechanism for cooperative long-term potentiation.

Author

Golding NL, Staff NP, and Spruston N

Subjects

Animals, Axons physiology, Calcium metabolism, Calcium Signaling, Excitatory Postsynaptic Potentials physiology, Rats, Rats, Wistar, Synapses physiology, Theta Rhythm, Action Potentials, Dendrites physiology, Long-Term Potentiation, Pyramidal Cells cytology, Pyramidal Cells physiology

Abstract

Strengthening of synaptic connections following coincident pre- and postsynaptic activity was proposed by Hebb as a cellular mechanism for learning. Contemporary models assume that multiple synapses must act cooperatively to induce the postsynaptic activity required for hebbian synaptic plasticity. One mechanism for the implementation of this cooperation is action potential firing, which begins in the axon, but which can influence synaptic potentiation following active backpropagation into dendrites. Backpropagation is limited, however, and action potentials often fail to invade the most distal dendrites. Here we show that long-term potentiation of synapses on the distal dendrites of hippocampal CA1 pyramidal neurons does require cooperative synaptic inputs, but does not require axonal action potential firing and backpropagation. Rather, locally generated and spatially restricted regenerative potentials (dendritic spikes) contribute to the postsynaptic depolarization and calcium entry necessary to trigger potentiation of distal synapses. We find that this mechanism can also function at proximal synapses, suggesting that dendritic spikes participate generally in a form of synaptic potentiation that does not require postsynaptic action potential firing in the axon.

Published

2002

25. Dichotomy of action-potential backpropagation in CA1 pyramidal neuron dendrites.

Author

Golding NL, Kath WL, and Spruston N

Subjects

Action Potentials physiology, Animals, Calcium metabolism, Dendrites ultrastructure, Diagnostic Imaging, Electrophysiology, Fluorescent Dyes, Fura-2, Hippocampus cytology, In Vitro Techniques, Male, Models, Neurological, Patch-Clamp Techniques, Potassium Channels physiology, Pyramidal Cells ultrastructure, Rats, Rats, Wistar, Sodium Channels physiology, Dendrites physiology, Hippocampus physiology, Pyramidal Cells physiology

Abstract

In hippocampal CA1 pyramidal neurons, action potentials are typically initiated in the axon and backpropagate into the dendrites, shaping the integration of synaptic activity and influencing the induction of synaptic plasticity. Despite previous reports describing action-potential propagation in the proximal apical dendrites, the extent to which action potentials invade the distal dendrites of CA1 pyramidal neurons remains controversial. Using paired somatic and dendritic whole cell recordings, we find that in the dendrites proximal to 280 microm from the soma, single backpropagating action potentials exhibit <50% attenuation from their amplitude in the soma. However, in dendritic recordings distal to 300 microm from the soma, action potentials in most cells backpropagated either strongly (26-42% attenuation; n = 9/20) or weakly (71-87% attenuation; n = 10/20) with only one cell exhibiting an intermediate value (45% attenuation). In experiments combining dual somatic and dendritic whole cell recordings with calcium imaging, the amount of calcium influx triggered by backpropagating action potentials was correlated with the extent of action-potential invasion of the distal dendrites. Quantitative morphometric analyses revealed that the dichotomy in action-potential backpropagation occurred in the presence of only subtle differences in either the diameter of the primary apical dendrite or branching pattern. In addition, action-potential backpropagation was not dependent on a number of electrophysiological parameters (input resistance, resting potential, voltage sensitivity of dendritic spike amplitude). There was, however, a striking correlation of the shape of the action potential at the soma with its amplitude in the dendrite; larger, faster-rising, and narrower somatic action potentials exhibited more attenuation in the distal dendrites (300-410 microm from the soma). Simple compartmental models of CA1 pyramidal neurons revealed that a dichotomy in action-potential backpropagation could be generated in response to subtle manipulations of the distribution of either sodium or potassium channels in the dendrites. Backpropagation efficacy could also be influenced by local alterations in dendritic side branches, but these effects were highly sensitive to model parameters. Based on these findings, we hypothesize that the observed dichotomy in dendritic action-potential amplitude is conferred primarily by differences in the distribution, density, or modulatory state of voltage-gated channels along the somatodendritic axis.

Published

2001

26. Dendritic calcium spike initiation and repolarization are controlled by distinct potassium channel subtypes in CA1 pyramidal neurons.

Author

Golding NL, Jung HY, Mickus T, and Spruston N

Subjects

4-Aminopyridine pharmacology, Action Potentials, Animals, Elapid Venoms pharmacology, Electrophysiology, Hippocampus cytology, Large-Conductance Calcium-Activated Potassium Channels, Male, Potassium Channel Blockers, Protein Isoforms physiology, Rats, Rats, Wistar, Sodium physiology, Tetraethylammonium pharmacology, Calcium physiology, Dendrites physiology, Hippocampus physiology, Potassium Channels physiology, Potassium Channels, Calcium-Activated, Pyramidal Cells physiology

Abstract

In CA1 pyramidal neurons of the hippocampus, calcium-dependent spikes occur in vivo during specific behavioral states and may be enhanced during epileptiform activity. However, the mechanisms that control calcium spike initiation and repolarization are poorly understood. Using dendritic and somatic patch-pipette recordings, we show that calcium spikes are initiated in the apical dendrites of CA1 pyramidal neurons and drive bursts of sodium-dependent action potentials at the soma. Initiation of calcium spikes at the soma was suppressed in part by potassium channels activated by sodium-dependent action potentials. Low-threshold, putative D-type potassium channels [blocked by 100 microM 4-aminopyridine (4-AP) and 0.5-1 microM alpha-dendrotoxin (alpha-DTX)] played a prominent role in setting a high threshold for somatic calcium spikes, thus restricting initiation to the dendrites. DTX- and 4-AP-sensitive channels were activated during sodium-dependent action potentials and mediated a large component of their afterhyperpolarization. Once initiated, repetitive firing of calcium spikes was limited by activation of putative BK-type calcium-activated potassium channels (blocked by 250 microM tetraethylammonium chloride, 70 nM charybdotoxin, or 100 nM iberiotoxin). Thus, the concerted action of calcium- and voltage-activated potassium channels serves to focus spatially and temporally the membrane depolarization and calcium influx generated by calcium spikes during strong, synchronous network excitation.

Published

1999

27. Role of intrinsic conductances underlying responses to transients in octopus cells of the cochlear nucleus.

Author

Golding NL, Ferragamo MJ, and Oertel D

Subjects

4-Aminopyridine pharmacology, Action Potentials physiology, Animals, Cesium pharmacology, Cochlear Nucleus cytology, Cochlear Nucleus drug effects, Excitatory Postsynaptic Potentials, In Vitro Techniques, Mice, Mice, Inbred Strains, Microelectrodes, Neural Conduction drug effects, Patch-Clamp Techniques, Cochlear Nucleus physiology, Neural Conduction physiology

Abstract

Recognition of acoustic patterns in natural sounds depends on the transmission of temporal information. Octopus cells of the mammalian ventral cochlear nucleus form a pathway that encodes the timing of firing of groups of auditory nerve fibers with exceptional precision. Whole-cell patch recordings from octopus cells were used to examine how the brevity and precision of firing are shaped by intrinsic conductances. Octopus cells responded to steps of current with small, rapid voltage changes. Input resistances and membrane time constants averaged 2.4 MOmega and 210 microseconds, respectively (n = 15). As a result of the low input resistances of octopus cells, action potential initiation required currents of at least 2 nA for their generation and never occurred repetitively. Backpropagated action potentials recorded at the soma were small (10-30 mV), brief (0.24-0.54 msec), and tetrodotoxin-sensitive. The low input resistance arose in part from an inwardly rectifying mixed cationic conductance blocked by cesium and potassium conductances blocked by 4-aminopyridine (4-AP). Conductances blocked by 4-AP also contributed to the repolarization of the action potentials and suppressed the generation of calcium spikes. In the face of the high membrane conductance of octopus cells, sodium and calcium conductances amplified depolarizations produced by intracellular current injection over a time course similar to that of EPSPs. We suggest that this transient amplification works in concert with the shunting influence of potassium and mixed cationic conductances to enhance the encoding of the onset of synchronous auditory nerve fiber activity.

Published

1999

28. Golgi cells in the superficial granule cell domain overlying the ventral cochlear nucleus: morphology and electrophysiology in slices.

Author

Ferragamo MJ, Golding NL, Gardner SM, and Oertel D

Subjects

Animals, Electric Stimulation, Electrophysiology, Excitatory Postsynaptic Potentials physiology, In Vitro Techniques, Mice, Mice, Inbred CBA, Neural Inhibition physiology, Synapses physiology, Cochlear Nucleus cytology, Cochlear Nucleus physiology, Interneurons cytology, Interneurons physiology

Abstract

Golgi cells are poised to integrate multimodal influences by participating in circuits involving granule cells in the cochlear nuclei. To understand their physiological role, intracellular recordings were made from anatomically identified Golgi cells in slices of the cochlear nuclei from mice. Cell bodies, dendrites, and terminals for all seven labeled cells were restricted to the narrow plane of the superficial granule cell domain over the ventral cochlear nucleus. The axonal arborization was the most striking feature of all Golgi cells; a dense plexus of terminals covered an area 200-400 microm in diameter in the vicinity of the cell body and dendrites. Axonal beads often surrounded granule cell bodies, indicating that granule cells are probable targets. Cells had input resistances up to 130 M omega and fired regular, overshooting action potentials. Golgi cells probably receive auditory nerve input, because shocks to the cut end of the auditory nerve excited Golgi cells with excitatory postsynaptic potentials (EPSPs). The latency of EPSPs shortened to a minimum and the amplitude of EPSPs grew in several steps as the strength of shocks was increased. The minimum latency of EPSPs in Golgi cells was on average 1.3 milliseconds, 0.6 milliseconds longer than the minimum latencies of EPSPs in nearby octopus and T stellate cells. The long latency raises the possibility that Golgi cells receive input from slowly conducting, unmyelinated auditory nerve fibers. Golgi cells are also excited by interneurons with N-methyl-D-aspartate receptors, probably granule cells, because repetitive shocks and single shocks in the absence of extracellular Mg2+ evoked late EPSPs that were reversibly blocked by DL-2-amino-5-phosphono-valeric acid.

Published

1998

29. Dendritic sodium spikes are variable triggers of axonal action potentials in hippocampal CA1 pyramidal neurons.

Author

Golding NL and Spruston N

Subjects

Action Potentials physiology, Animals, Axons physiology, Electric Stimulation methods, Hippocampus cytology, In Vitro Techniques, Male, Neurons physiology, Patch-Clamp Techniques, Rats, Rats, Wistar, Sodium metabolism, Sodium Channels physiology, Synapses physiology, Dendrites physiology, Hippocampus physiology, Pyramidal Cells physiology, Sodium physiology

Abstract

Several early studies suggested that spikes can be generated in the dendrites of CA1 pyramidal neurons, but their functional significance and the conditions under which they occur remain poorly understood. Here, we provide direct evidence from simultaneous dendritic and somatic patch-pipette recordings that excitatory synaptic inputs can elicit dendritic sodium spikes prior to axonal action potential initiation in hippocampal CA1 pyramidal neurons. Both the probability and amplitude of dendritic spikes depended on the previous synaptic and firing history of the cell. Moreover, some dendritic spikes occurred in the absence of somatic action potentials, indicating that their propagation to the soma and axon is unreliable. We show that dendritic spikes contribute a variable depolarization that summates with the synaptic potential and can act as a trigger for action potential initiation in the axon.

Published

1998

30. Synaptic inputs to stellate cells in the ventral cochlear nucleus.

Author

Ferragamo MJ, Golding NL, and Oertel D

Subjects

Action Potentials drug effects, Action Potentials physiology, Animals, Bicuculline pharmacology, Electric Stimulation, Excitatory Amino Acid Antagonists pharmacology, Excitatory Postsynaptic Potentials, Glutamic Acid pharmacology, In Vitro Techniques, Interneurons drug effects, Interneurons physiology, Mice, Mice, Inbred CBA, Mice, Inbred ICR, Models, Neurological, Nerve Fibers drug effects, Nerve Fibers physiology, Neurons cytology, Neurons drug effects, Picrotoxin pharmacology, Quinoxalines pharmacology, Receptors, AMPA drug effects, Receptors, AMPA physiology, Receptors, GABA-A physiology, Receptors, N-Methyl-D-Aspartate drug effects, Receptors, N-Methyl-D-Aspartate physiology, Strychnine pharmacology, Auditory Perception physiology, Cochlear Nucleus cytology, Cochlear Nucleus physiology, Neurons physiology, Synapses physiology, Vestibulocochlear Nerve physiology

Abstract

Auditory information is carried from the cochlear nuclei to the inferior colliculi through six parallel ascending pathways, one of which is through stellate cells of the ventral cochlear nuclei (VCN) through the trapezoid body. To characterize and identify the synaptic influences on T stellate cells, intracellular recordings were made from anatomically identified stellate cells in parasagittal slices of murine cochlear nuclei. Shocks to the auditory nerve consistently evoked five types of synaptic responses in T stellate cells, which reflect sources intrinsic to the cochlear nuclear complex. 1) Monosynaptic excitatory postsynaptic potentials (EPSPs) that were blocked by 6,7-dinitroquinoxaline-2,3-dione (DNQX), an antagonist of alpha-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid receptors, probably reflected activation by auditory nerve fibers. Electrophysiological estimates indicate that about five auditory nerve fibers converge on one T stellate cell. 2) Disynaptic, glycinergic inhibitory postsynaptic potentials (IPSPs) arise through inhibitory interneurons in the VCN or in the dorsal cochlear nucleus (DCN). 3) Slow depolarizations, the source of which has not been identified, that lasted between 0.2 and 1 s and were blocked by -2-amino-5-phosphonovaleric acid (APV), the N-methyl-D-aspartate (NMDA) receptor antagonist. 4) Rapid, late glutamatergic EPSPs are polysynaptic and may arise from other T stellate cells. 5) Trains of late glycinergic IPSPs after single or repetitive shocks match the responses of D stellate cells, showing that D stellate cells are one source of glycinergic inhibition to T stellate cells. The source of late, polysynaptic EPSPs and IPSPs was assessed electrophysiologically and pharmacologically. Late synaptic responses in T stellate cells were enhanced by repetitive stimulation, indicating that the interneurons from which they arose should fire trains of action potentials in responses to trains of shocks. Late EPSPs and late IPSPs were blocked by APV and enhanced by the removal of Mg2+, indicating that the interneurons were driven at least in part through NMDA receptors. Bicuculline, a gamma-aminobutyric acid-A (GABAA) receptor antagonist, enhanced the late PSPs, indicating that GABAergic inhibition suppresses both the glycinergic interneurons responsible for the trains of IPSPs in T-stellate cells and the interneuron responsible for late EPSPs in T stellate cells. The glycinergic interneurons that mediate the series of IPSPs are intrinsic to the ventral cochlear nucleus because long series of IPSPs were recorded from T stellate cells in slices in which the DCN was removed. These experiments indicate that T stellate cells are a potential source of late EPSPs and that D stellate cells are a potential source for trains of late IPSPs.

Published

1998

31. Physiological identification of the targets of cartwheel cells in the dorsal cochlear nucleus.

Author

Golding NL and Oertel D

Subjects

Action Potentials physiology, Animals, In Vitro Techniques, Membrane Potentials physiology, Mice, Synapses physiology, Cochlear Nucleus cytology, Neurotransmitter Agents physiology

Abstract

The integrative contribution of cartwheel cells of the dorsal cochlear nucleus (DCN) was assessed with intracellular recordings from anatomically identified cells. Recordings were made, in slices of the cochlear nuclei of mice, from 58 cartwheel cells, 22 fusiform cells, 3 giant cells, 5 tuberculoventral cells, and 1 cell that is either a superficial stellate or Golgi cell. Cartwheel cells can be distinguished electrophysiologically from other cells of the cochlear nuclei by their complex spikes, which comprised two to four rapid action potentials superimposed on a slower depolarization. The rapid action potentials were blocked by tetrodotoxin (n = 17) and were therefore mediated by voltage-sensitive sodium currents. The slow spikes were eliminated by the removal of calcium from the extracellular saline (n = 3) and thus were mediated by voltage-sensitive calcium currents. The spontaneous and evoked firing patterns of cartwheel cells were distinctive. Cartwheel cells usually fired single and complex spikes spontaneously at irregular intervals of between 100 ms and several seconds. Shocks to the DCN elicited firing that lasted tens to hundreds of milliseconds. With the use of these distinctive firing patterns, together with a pharmacological dissection of postsynaptic potentials (PSPs), possible targets of cartwheel cells were identified and the function of the connections was examined. Not only cartwheel and fusiform cells, but also giant cells, received patterns of synaptic input consistent with their having originated from cartwheel cells. These cell types responded to shocks of the DCN with variable trains of PSPs that lasted hundreds of milliseconds. PSPs within these trains appeared both singly and in bursts of two to four, and were blocked by 0.5 or 1 microM strychnine (n = 4 cartwheel, 4 fusiform, and 2 giant cells), indicating that cartwheel cells are likely to be glycinergic. In contrast with cartwheel cells, which are weakly excited by glycinergic input, glycinergic PSPs consistently inhibited fusiform and giant cells. Tuberculoventral cells and the putative superficial stellate cell received little or no spontaneous synaptic activity. Shocks to the DCN evoked synaptic activity that lasted approximately 5 ms. These cells therefore probably do not receive input from cartwheel cells. In addition, the brief firing of tuberculoventral cells and of the putative superficial stellate cell in response to shocks indicates that these cells are unlikely to contribute to the late, glycinergic synaptic potentials observed in cartwheel, fusiform, and giant cells.

Published

1997