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The Journal of Neuroscience, July 16, 2003, 23(15):6357-6361
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BRIEF COMMUNICATION
Fast Inhibition Underlies the Transmission of Auditory Information between Cochlear Nuclei
Karina Needham1 andAntonio G. Paolini2,3 1Department of Otolaryngology, The University of Melbourne, East Melbourne, Victoria 3002, Australia, 2The Bionic Ear Institute, East Melbourne, Victoria 3002, Australia, and 3School of Psychological Science, La Trobe University, Bundoora, Victoria 3086, Australia
Abstract
Top
Abstract
Introduction
A direct commissural connection between cochlear nuclei provides a pathway by which binaural input can influence the processing of acoustic information through the ventral cochlear nucleus. Despite anatomical evidence to suggest the existence of such a pathway, its nature and behavior have not been investigated previously. This in vivo intracellular electrophysiological study provides direct evidence of monosynaptic (mean latency, 1.43 msec), inhibitory commissural input to T stellate cells. This inhibition is fast acting (duration, <10 msec), occurring with little synaptic delay (0.3 msec). Electrical stimulation also revealed the initiation of antidromic responses in the onset chopper population, signifying D stellate neurons as a source of commissural inputs. Activation of the commissural connection was most evident in response to broadband stimuli. These results provide the first compelling evidence of a fast, monosynaptic commissural pathway arising from contralateral D stellate neurons providing broadband inhibitory input to T stellate cells.
Key words: ventral cochlear nucleus; commissural connection; stellate neurons; inhibition; in vivo intracellular electrophysiology; antidromic action potential
Introduction
The cochlear nucleus (CN) complex, as the first brain center of the ascending auditory pathway, serves to process information received from the cochlea into numerous parallel processing streams for transmission to higher central auditory nuclei (Young, 1998). One such pathway is through the stellate (multipolar) population of the ventral CN (VCN), a population divided into T and D stellate cells on the basis of dendritic morphology and axonal projections (Oertel et al., 1990
Speculation has surrounded the existence of this pathway because studies revealed contralateral acoustic stimulation as capable of inhibiting and exciting cells throughout the CN (Pfalz, 1962
In this study, we examine the commissural connection through in vivo intracellular and extracellular electrophysiological recordings in the rat. Our investigation explores the influence of direct commissural input on the ipsilateral VCN through electrical and acoustic stimulation of the contralateral CN. Of particular interest is the role of the stellate populations. Thus, we report on the effects of contralateral stimulation on onset chopper (OC) and chopper [sustained (CS) and transient (CT)] neurons, the physiological response patterns displayed by D and T stellate cells, respectively (Blackburn and Sachs, 1989
Materials and Methods
Preparation. Electrophysiological experiments were performed on 20 male Hooded Wistar rats (250–350 gm). The main components of this protocol have been outlined previously (Paolini and Clark, 1999Animals were anesthetized with intraperitoneal aqueous urethane (20% w/v: total dose, 2.6 gm/kg; Sigma, Sydney, Australia). After a craniotomy, the cerebellum was aspirated to expose the brainstem. Visualization of the CN at the lateral extreme allowed a recording electrode to be inserted into the left (ipsilateral) VCN in a caudorostral direction away from the octopus cell area. Placement of the stimulating electrode into the right (contralateral) VCN was also made under visual control. Both electrodes were stabilized in the tissue with 4% agar. Core body temperature, controlled by a DC homeothermic blanket, was maintained at
Recording. Microelectrodes (quartz thin-walled; 1.0 mm outer diameter; Sutter Instruments, Novato, CA), containing 1 M potassium acetate (KAc; 70–80 M
) or 4% Neurobiotin (Vector Laboratories, Burlingame, CA) in 1 M KAc, were advanced through the VCN in 2 µm steps by a motorized microdrive (Sutter Instruments). The concentric bipolar stimulating electrode (tungsten metal, 76 µm core, 3–4 µm tip diameter; World Precision Instruments, Sarasota, FL) was advanced into the contralateral VCN until a small field potential was visible on the recording trace.
A "search stimulus" of 70–80 dB white noise (50 msec duration, every 500 msec) was presented continuously to the ipsilateral side with advancement of the microelectrode. Intracellular stable impalements (typically possible for 10–90 min) were signaled by a prolonged (> 3 min), stable drop (> 30 mV) in the DC level and the presence of synaptic or large action potentials (APs) (> 20 mV) with monophasic rise and fall times. During stable cellular impalements, single shocks (typically from 10 to 600 µA, 1 Hz presentation; charge balanced biphasic pulses, 100 µsec per phase) were delivered to the contralateral CN, followed by acoustic stimuli (delayed 20–40 msec) presented to the left ear. Although we could not discount the possibility that electrical stimulation evoked the middle ear muscles through facial nerve activation, there is no evidence to suggest that such mechanisms are capable of decreasing the spontaneous activity of primary afferent inputs and therefore tonic drive to CN neurons.
After the generation of an antidromic AP, a collision test was performed, in which an ipsilaterally click-generated AP was presented at varying intervals before electrical stimulation. The characteristic frequency (CF) of the neuron and spike input–output (IO) function to CF tones were then determined. CF was calculated from a threshold tuning curve constructed online (Liberman, 1978
Digitally synthesized acoustic stimuli were generated by Beyer DT48 transducers (Beyerdynamic, Farmingdale, NY), positioned at the end of the hollow ear bars and controlled using a Tucker-Davis signal generator (Tucker-Davis Technologies, Gainesville, FL). The acoustic system was calibrated using a Bruel & Kjaer (B&K) measuring amplifier (type 2606; Bruel & Kjaer, Naerum, Denmark) and a B&K
inch condenser microphone, coupled to a small probe tube positioned
The "Neurophysiology Laboratory System" of the Department of Otolaryngology (NLS software, by R. E. Millard, The University of Melbourne, Victoria, Australia), was used to control the Tucker-Davis unit and collate spike time information. Cellular responses were recorded using an Axoclamp 2B amplifier (Axon Instruments, Union City, CA), and electrophysiological traces were stored on a MacLab 4S system (ADInstruments, Sydney, Australia).
Classification. Neuron classification was made using neural discharge patterns displayed in poststimulus time (PST) and interspike interval (ISI) histograms constructed online (Pfeiffer, 1966
Results
Intracellular recordings were taken from 18 VCN neurons, and extracellular recordings were obtained for an additional nine. The mean resting membrane potential (±SE) for intracellularly recorded neurons was -51.3 ± 1.57 mV, with an average AP amplitude of 39.9 ± 2.61 mV (range, 24–65 mV). Mean CF was 18.3 ± 1.99 kHz, with a mean firing threshold of 38.1 ± 5.53 dB SPL. Using aforementioned classification criteria, 15 neurons (14 intracellular and one extracellular) were identified as choppers, including both CS and CT subclasses, and 12 (four intracellular and eight extracellular) were classified as OC neurons.Antidromic activity in OC neurons
Electrical stimulation of the contralateral CN often resulted in AP activation in OC neurons (Fig. 1). This activity was confirmed as antidromic in one (25%) intracellular and six (75%) extracellularly recorded OC neurons on the basis of four criteria (Kitai and Park, 1990
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Figure 1. Electrically stimulated antidromic activity. a, Collision test performed on the intracellularly recorded OC neuron (02-712-017). The interval between ipsilateral click (vertical dashed line, denoted i) and contralateral electrical stimulation (artifact denoted s) was decreased from 8 msec (top) to 3 msec (bottom), thereby colliding the APs and eliminating the antidromic AP. b, The orthodromic AP (bottom), but not the antidromic AP (top), is accompanied by a spike prepotential (arrow) before activation. The vertical dotted line indicates time of maximal AP depolarization. The horizontal dashed line indicates resting membrane potential. APs are truncated for better illustration of depolarizing properties at AP onset. c, PST histograms constructed in response to suprathreshold CF tone bursts (50 repetitions) shown for the first 15 msec of presentation and 50 msec (inset) provide confirmation of the response type of neuron 02-712-017. d, High-frequency electrical stimulation of an extracellularly recorded OC neuron (02-717-006) displaying antidromic activity.
Activation of commissural inhibition in chopper neurons
The presence of short-latency membrane hyperpolarization (mean of 1.43 ± 0.12 msec onset) in response to contralateral electrical stimulation was observed in seven (50%) intracellularly recorded chopper (CS and CT) neurons. As displayed by the intracellularly recorded CT neuron (intracellular profile, PST histogram, and CV) (Fig. 2a,b), large hyperpolarizing potentials were evoked with little delay (1.1 msec) after electrical stimulation (Fig. 2c). Although the mean average maximum amplitude of hyperpolarization (5.30 ± 0.68 mV) across all chopper neurons was large, hyperpolarization amplitude within each neuron was dependent on stimulus strength (Fig. 2c). Examination of the mechanisms underlying the activation of electrically evoked hyperpolarization (Fig. 2d,e) through injection of hyperpolarizing and depolarizing current revealed a reversal of hyperpolarization between -68 and -70 mV, results consistent with the reversal potential (-67 mV) of glycinergic IPSPs in VCN neurons (Wu and Oertel, 1986
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Figure 2. Initiation of hyperpolarization through contralateral electrical stimulation. a, Single intracellular response of neuron 02-712-002 to suprathreshold CF (13.2 kHz) 50 msec tone bursts displaying a typical CT response pattern. b, PST histogram and CV calculations of the response to CF tone bursts (50 repetitions). c, Increasing the strength of electrical stimulation (50, 100, and 200 µA; artifact denoted s), as displayed in single intracellular traces, increases the amplitude of hyperpolarization. Horizontal dashed line indicates resting membrane potential. d, Effect of membrane potential on amplitude of hyperpolarization; intracellular traces at varying membrane potentials in response to electrical stimulation (200 µA). Horizontal dashed lines indicate membrane potential at time of stimulation [resting membrane potential (RMP)]. Introducing negative current reduced the amplitude of hyperpolarization, with reversal of the membrane potential occurring between -68 and -70 mV. e, Amplitude of hyperpolarization after electrical shock as a function of membrane potential for single responses of neuron shown in d. A negative change in the membrane potential from resting (0 mV; horizontal dashed line) indicates hyperpolarization, whereas a positive value indicates depolarization. Vertical dashed line denotes resting membrane potential.
Whereas the short and highly consistent onset latency of hyperpolarization induced through electrical stimulation (Figs. 2, 3c,f) indicated the monosynaptic nature of the commissural pathway [Power Test (Kitai and Park, 1990
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Figure 3. Inhibition through acoustic and electrical stimulation. a, IPSP produced in CT neuron 02-716-001 after a 100 dB SPL contralateral click (dashed vertical line denoted c). Horizontal dashed line indicates resting membrane potential. b, IPSPs resulting from electrical stimulation (stimulus artifact denoted s) of the contralateral CN (10, 100, 200, and 400 µA). c, Expanded time base of responses shown in b, with membrane potential standardized to zero demonstrating the synchronization of IPSP onset latency across varying stimulus strengths. d, Change in hyperpolarization amplitude in response to changing strength of contralateral acoustic click (60, 70, and 80 dB), represented in averaged intracellular traces from CS neuron 02-715-007. e, Average intracellular responses to increasing levels of contralateral electrical stimulation (200, 400, and 600 µA). f, Expanded time base of responses shown in e, standardized as in c.
Inhibition in chopper neurons was also activated in response to broadband stimuli, such as noise (Fig. 4). Contralaterally presented white noise (80 dB SPL) induced short-latency (4.2 msec) short-lived hyperpolarization (Fig. 4a1, arrow) in the CT neuron shown in Figure 2. The time course of this hyperpolarization (expanded time base) (Fig. 4a2, asterisk) is similar to that seen in response to both electrical and acoustic click stimulation (Figs. 2, 3). However, hyperpolarization initiated by noise was soon exceeded by excitatory inputs (
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Figure 4. Chopper neuron responses to contralateral broadband stimuli and high-frequency electrical stimulation. a1, Average intracellular response of a CT neuron (02-712-002) to the presentation of a contralateral 50 msec 80 dB white noise burst (over 50 repetitions). Arrow indicates period of sustained hyperpolarization after contralateral presentation. a2, The first 30 msec of the average response displayed in a1; asterisks denote periods of hyperpolarization similar in time course to those displayed in response to electrical stimulation (Fig. 3). Horizontal dashed lines indicate resting membrane potential. b1–b4, Response of neuron 02-712-002 (CF of 13.2 kHz) to 50 msec pure tone bursts (averaged over 50 repetitions) below CF (11 and 12 kHz), near CF (13 kHz), and above CF (14 kHz). c, Average response of neuron 02-716-001 to train of multiple electrical pulses of 100 µA presented with increasing frequency (200, 300, 400, and 500 Hz).
In addition, high-frequency electrical stimulation was used to simulate the effects of OC activity on the behavior of hyperpolarization in chopper neurons (Fig. 4c). As the stimulation frequency increased from 200 to 500 Hz (two to five pulses; 100 µA), the IPSPs summated, resulting in longer periods of inhibition (Fig. 4c), thereby indicating that the behavior of inhibition initiated by D stellate neurons is dependent on the extent of the intrinsic firing activity.
Discussion
Combining in vivo intracellular electrophysiological recordings with electrical and acoustic stimulation of the contralateral CN, this study is the first to demonstrate a fast, monosynaptic inhibitory commissural connection between cochlear nuclei. The isolation of inhibitory potentials in VCN neurons after stimulation of the contralateral CN has permitted the nature and behavior of the commissural pathway to be examined in a manner not permitted by previous methods of investigation.Commissural inhibition
Inhibitory responses exhibiting monosynaptic transmission from the contralateral CN were detected in neurons responding to ipsilateral tones in a chopping (CS or CT) manner. The input of commissural inhibitory projections to chopper neurons, associated with the T stellate population, confirms anatomical observations (Schofield and Cant, 1996aConversely, the activation of antidromic APs in response to electrical stimulation indicated that the projections of OC neurons terminate in the contralateral VCN. These results, given the association between the OC response and D stellate neurons (Oertel et al., 1990
The presence of antidromic activity in a small proportion of OC responses may reflect either (1) an inability to activate all D stellate cells through electrical stimulation, or (2) the presence of contralateral projections in only a subset of the population. Although the latter hypothesis cannot be confirmed nor refuted by the results, the first scenario appears less likely because acoustically evoked inhibition was only observed in those chopper neurons also inhibited by electrical stimulation. Although inhibition evoked through both electrical and acoustic means exhibited IPSPs of similar time course, differences in amplitude suggest that antidromically activated D stellate collaterals synapsing intrinsically within the VCN may contribute some inhibitory input during electrical stimulation.
Fast, monosynaptic pathway
This study provides definitive evidence to support the fast, monosynaptic nature of the commissural pathway. The results presented here consistently demonstrate the activation of short-latency (mean of 1.43 msec) hyperpolarization in response to electrical stimulation. Similarly, acoustic stimuli presented to the contralateral ear produced short-latency (mean of 3.55 msec) responses, reflecting the activation of synaptic relays through the cochlea and auditory nerve. Because OC ipsilaterally induced APs are activatedFunctional implications
Although the influence of a single IPSP is transient, the overall extent of inhibition is essentially dependent on the intrinsic firing behavior of the D stellate neuron. As exhibited by our results, inhibition is most evident when activated through broadband stimuli, to which OC neurons respond most vigorously. Given that inhibition is postulated to influence the regularity of chopping activity in chopper neurons (Blackburn and Sachs, 1989
Footnotes
Received Apr. 11, 2003; revised May. 19, 2003; accepted May. 20, 2003.This work was supported by a Melbourne Research Scholarship (The University of Melbourne) and The Bionic Ear Institute. We thank J. C. Clarey for suggestions and comments regarding experiments and this manuscript, R. E. Millard for technical assistance, and G. M. Clark for encouragement and support.
Correspondence should be addressed to A. G. Paolini, School of Psychological Science, La Trobe University, Bundoora, Victoria 3086, Australia. E-mail: a.paolini{at}latrobe.edu.au.
Copyright © 2003 Society for Neuroscience 0270-6474/03/236357-05$15.00/0
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