 |
||||
|
||||
|
||||
|
||||
|
||||
The Journal of Neuroscience, June 6, 2007, 27(23):6091-6102; doi:10.1523/JNEUROSCI.4848-06.2007
Previous Article | Next Article
Behavioral/Systems/Cognitive
Transformation of Temporal Properties between Auditory Midbrain and Cortex in the Awake Mongolian Gerbil
Maria Ter-Mikaelian,1 Dan H. Sanes,1,2 andMalcolm N. Semple1,3 1Center for Neural Science and Departments of 2Biology and 3Psychology, New York University, New York, New York 10003
Abstract
Top
Abstract
Introduction
The neural representation of meaningful stimulus features is thought to rely on precise discharge characteristics of the auditory cortex. Precisely timed onset spikes putatively carry the majority of stimulus-related information in auditory cortical neurons but make a small contribution to stimulus representation in the auditory midbrain. Because these conclusions derive primarily from anesthetized preparations, we reexamined temporal coding properties of single neurons in the awake gerbil inferior colliculus (IC) and compared them with primary auditory cortex (AI). Surprisingly, AI neurons displayed a reduction of temporal precision compared with those in the IC. Furthermore, this hierarchical transition from high to low temporal fidelity was observed for both static and dynamic stimuli. Because most of the data that support temporal precision were obtained under anesthesia, we also reexamined response properties of IC and AI neurons under these conditions. Our results show that anesthesia has profound effects on the trial-to-trial variability and reliability of discharge and significantly improves the temporal precision of AI neurons to both tones and amplitude-modulated stimuli. In contrast, IC temporal properties are only mildly affected by anesthesia. These results underscore the pitfalls of using anesthetized preparations to study temporal coding. Our findings in awake animals reveal that AI neurons combine faster adaptation kinetics and a longer temporal window than evident in IC to represent ongoing acoustic stimuli.
Key words: inferior colliculus; auditory cortex; anesthetic effects; adaptation; amplitude modulation; binary coding
Introduction
Precise spike timing to the onset of an acoustic feature is thought to support many auditory percepts, including discrimination of consecutive sounds, the differentiation of phonemes in speech, and the spatial position of a sound source (Phillips and Farmer, 1990; Phillips and Hall, 1990
It has been demonstrated that auditory cortical discharge patterns containing only the first spike may carry as much as 89% of the information about stimulus location available in the full spiking response (Furukawa and Middlebrooks, 2002
Our goal was to assess the evolution of temporal precision between two loci in the ascending auditory pathway in the awake gerbil. Surprisingly, we observed a decrease in temporal fidelity between the IC and AI in responses to either static or amplitude- modulated stimuli. A reexamination of temporal processing under anesthesia revealed significant anesthetic effects on temporal coding properties in AI but not IC. These effects have previously led to a different conclusion about hierarchical processing in the auditory system. We present a new interpretation of the IC–AI coding transformation. IC neurons exhibit greater temporal precision, slower adaptation kinetics, and a shorter "temporal window" (the time interval during which a neuron integrates input), allowing for the representation of continuous, rapidly modulated sounds. In contrast, the temporal response properties of AI neurons are better suited for representing slow temporal modulations in the acoustic environment.
Materials and Methods
Animal preparation
All procedures relating to the maintenance and use of animals in this study were approved by the University Animal Welfare Committee at New York University.Surgical preparation for chronic recordings. Adult gerbils were premedicated with ketoprophen (1.5 mg/kg, i.n.) and dexamethasone (0.35 mg/kg, i.p.) and hydrated with normosol (1.5 ml, s.c.). The animals were anesthetized with isoflurane, maintained by monitoring withdrawal reflexes and respiration rate. A small threaded metal post was positioned horizontally along the midline and secured with small bone screws and dental acrylic. A silver ground wire was secured in a small hole drilled into the anterior skull. For recording access to the IC, a plate of intraparietal bone was removed over the cerebellum (Spitzer and Semple, 1993
Surgical preparation for acute recordings. Adult gerbils were anesthetized with a surgical dose of sodium pentobarbital (50 mg/kg, i.p.) and ketamine (30 mg/kg, i.p.). A tracheotomy was performed to prevent airway obstruction during the experiment, and atropine (0.08 mg/kg, i.m.) was administered to minimize mucous secretions. Preparation of the craniotomy and head cap were similar to the procedures described above for unanesthetized recording. Throughout the experiment, the withdrawal reflex was monitored, and 20% supplemental doses of both sodium pentobarbital and ketamine were administered intramuscularly as needed. The body temperature of the animal was maintained at 37°C for the duration of the surgery and recording. The experiment was terminated by administrating an overdose of sodium pentobarbital (>150 mg/kg, i.p.).
For all recordings, the animal was placed in a soundproof chamber (Industrial Acoustics Company, Bronx, NY), and the head was stabilized using the head post. During chronic recording sessions, animals stood comfortably on a platform and were free to move their limbs while the head position remained fixed. If an animal exhibited heightened anxiety or restlessness, medetomidine (a relaxant that acts on
2-adrenoceptors) was administered intranasally at the beginning of the recording session at a dosage of one to three drops (
0.1–0.3 mg/kg) and supplemented as necessary. It has been demonstrated that medetomidine lowers motivation but does not affect attention or response accuracy in rats performing a short-term memory task (Ruotsalainen et al., 1997
Nine animals (four IC and five AI) were used for acute recordings under anesthesia and 16 animals (four IC and 12 AI) were used for chronic awake recording experiments. One animal was excluded from the study because of a difference in the position of the craniotomy.
Electrophysiological recording
Tungsten electrodes (1.5–2.5 MW; MicroProbe, Gaithersburg, MD) were advanced ventrally through the craniotomy. For AI recording, an electrode tip angle of
View larger version (47K):
[in this window]
[in a new window]
Figure 1. Location and tuning characteristics of recording sites. A, Dark-field image of a coronal section through the left AI showing an electrode track in which a fluorescein injection was made. Dorsal is toward the top and lateral is to the left. B, Sagittal section through IC showing an electrode track terminating in a lesion site. Both sections are counterstained with cresyl violet. C, D, Histograms of BF of all recorded units in AI and IC. E, Electrode insertion depths for recorded units in anesthetized and awake AI. Horizontal lines indicate population medians.
Acoustic stimulation
The system used for stimulus generation and sound delivery as well as the calibration procedure have been described previously (Malone and Semple, 2001Each neuron was assessed with a battery of stimulus protocols designed to determine its response properties for static and modulated sounds. Typically, the approximate frequency range was obtained with an iso-intensity function at 10–30 dB above threshold. This was followed by a rate-level function at the estimated best frequency (BF). The standard stimulus battery included a 2 s tone delivered at the BF of the unit, and a 2 s narrow-band white-noise stimulus bandpassed geometrically (100%) about the BF. These long stimuli were shaped with a 5 ms cosine-ramped rise/fall time and were presented for at least 10 trials, with a 1 s intertrial interval. Brief tone and noise stimuli were identical to the longer stimuli, except that the duration was 50 ms and the intertrial interval was 950 ms. Stimulus thresholds were determined separately for each stimulus type, and responses were characterized at 10 dB above threshold for noise stimuli and 15 dB above threshold for tones (or at the peak of a nonmonotonic rate-level function if this was <15 dB above threshold).
SAM tones (10 s duration with 10 ms rise/fall) were presented at BF and at the SPL that produced the strongest synchronized response (often the same as the best SPL for tone stimulation). Modulation transfer functions (MTFs) were obtained by presenting two trials of multiple modulation frequencies at 100% modulation depth with an intertrial interval of 2 s. The following modulation frequencies were typically presented to each AC neuron: 0.1, 0.5, 1, 2, 3, 5, 10, 20, 30, 50, and 100 Hz. For IC neurons, 200, 300, and 400 Hz were also presented. If a neuron exhibited statistically significant synchrony to the modulation period at the highest modulation rate (100 Hz for AC and 400 Hz for IC), the modulation frequency was tested in additional 100 Hz increments until a cutoff frequency was obtained. An unmodulated tone at the same frequency and SPL and of the same duration as the SAM tones was included in the stimulus sequence as a control. For some cells, MTFs were also obtained for 400 ms SAM tones with a 10 ms rise time and an intertrial interval of 600 ms. Twenty trials were presented at each modulation frequency. In addition, the spontaneous firing rate and pattern of each cell was recorded during a continuous 30 s silent period.
Data analysis
Spike times were stored and viewed as raster plots or peristimulus time histograms (PSTHs). Minimum first-spike latency was determined at BF and at the SPL that produced the earliest response by selecting the first peak in the PSTH to a 200 ms tone (binned by 10 ms) as the region of interest (ROI). The corresponding raster plot was used to determine the mean onset time of the first spike over 10 or more trials. Using the same ROI, the SD of the first-spike time over all trials ("SD of the minimum latency") was calculated to provide an estimate of the temporal precision of the response onset. As an additional measure of temporal fidelity of the response onset, a 20 ms time window was positioned over the raster plot such that it contained the first spike of as many trials as possible. Trials that contained no spike in this time period were counted as "misses," and the proportion of misses over the total number of trials was determined.To analyze the kinetics of the firing response decay in response to long constant stimuli, the peristimulus time histogram of the response of each unit to a 2 s BF tone or noise burst or a 10 s SAM tone was fit with an exponential decay function of the form Y(t) = Ae–kt + P, where Y(t) is the firing rate at time t, k is the inverse of the decay time constant, A is a magnitude scaling factor, and P is the plateau firing rate. The resulting fit equation allowed us to interpolate the time at which the response declined to half and a quarter of the initial peak and also to estimate firing at set time points during the stimulus presentation. Additionally, population medians of the fit parameters A, k, and P were used to create typical response profiles for IC and AI neurons with and without anesthesia. Table 1 summarizes the number of cells used in the adaptation analysis from each population. In several cases, curve fit generation failed because the regression algorithm did not converge on best-fit values. Generally, this occurred when the number of spikes was insufficient to constrain the fit to a single solution. Additionally, several cells were excluded from the adaptation analysis because they had a buildup response pattern.
View this table:
[in this window]
[in a new window]
Table 1. Numbers of cells whose response PSTHs to BF tones, noise, and 20 Hz SAM were fit with a decaying exponential function
Average firing rates to tones and noise bursts were calculated over a time window equal to the stimulus duration but offset from the stimulus start time by the latency of the unit. Curve fits of spiking responses to tones and noise bursts were based on peristimulus time histograms, generated by sliding a 50 ms summation window in steps of 25 ms (equivalent to smoothing a histogram with 50 ms bins). For fitting responses to 10 s SAM tones, a 100 ms summation window was moved in steps of 50 ms. The peak response was defined as the largest bin in the histogram, which usually occurred near the onset of the stimulus. If the peak response occurred within the first seven bins of the histogram, the bins preceding it were excluded before curve fitting. This ensured that the fit best reflected the decaying phase of the response.Responses to SAM tones were analyzed for firing rate and synchrony to the stimulus period. The ROI excluded the first 100 ms to ensure that the response to the modulation was examined without contamination by the onset response (Liang et al., 2002
The temporal precision and coherence of the periodic response to SAM tones was assessed by summing period histograms of the responses of individual neurons to a 2 Hz SAM stimulus (binned by 10 ms, excluding the first 100 ms of each trial) to create a pooled period histogram for each of the four study populations. Each pooled period histogram was normalized to account for differences in sample size and maximum firing rate. All neurons displaying significant synchronization to SAM at 2 Hz were included in the analysis (34 anesthetized IC, 26 anesthetized AI, 41 awake IC, and 41 awake AI).
For both the tMTF and the rMTF, a best modulation frequency (BMF) was determined as the tested frequency that yielded the highest average firing rate (for rBMF) or the tested frequency that yielded the highest vector strength with statistical significance at the p < 0.001 level (for tBMF).
Histology
In all experiments, the location of the electrode in AI or in the IC central nucleus was determined based on a tonotopic progression matching those described previously for gerbil AI (Thomas et al., 1993
Results
Results are presented from 41 single units in anesthetized IC, 55 in anesthetized AI, 76 in awake IC, and 120 in awake AI.Temporal precision in auditory cortex is lower than in IC
We examined the temporal precision of discharges to an unmodulated stimulus in IC and AI of awake gerbils. To do this, we compared the first-spike timing variability (the SD of the latency; see Materials and Methods) in response to 200 ms BF tones. In Figure 2, example responses are shown in A and B, and C plots the population results. Surprisingly, the AI neuron population shows significantly higher first-spike timing variability compared with IC (Mann–Whitney U test, two-tailed, p = 0.0479; n = 113), indicating a loss of temporal precision in the ascending auditory pathway. The median values (indicated in Fig. 2C by horizontal black bars) were 2.5 ms for AI and 1.85 ms for IC.
View larger version (12K):
[in this window]
[in a new window]
Figure 2. First-spike timing is less precise in AI than in IC. A, B, Rasters of responses of an example awake AI (A) and awake IC (B) cell to a 200 ms BF tone. Windowed portions indicate the ROI for latency analysis, shown expanded on the right. The first spike in the ROI in each trial is shown in blue. C, Population plot of SD of the minimum latency in response to BF tone pips in AI and IC.
Improved temporal precision in AI is an artifact of anesthesia
This finding was paradoxical given previous reports of improved temporal precision in AI compared with subcortical auditory nuclei (Phillips and Hall, 1990
View larger version (12K):
[in this window]
[in a new window]
Figure 3. AI first-spike latency and latency variability are reduced by anesthesia. A, Response of an example anesthetized AI cell to a 200 ms BF tone; conventions as in Figure 2. B, Population plot of minimum first-spike latency and SD of the minimum latency in response to BF tone pips in anesthetized and awake AI. C, Histogram of SD of the latency in anesthetized and awake AI. Filled bars indicate anesthetized AI, and open bars indicate awake AI. Only values up to 4 ms are shown to highlight the difference between the populations.
View larger version (14K):
[in this window]
[in a new window]
Figure 4. IC latency variability is unaffected by anesthesia. A, Response of an example anesthetized IC cell to a 200 ms BF tone. B, Population plot of minimum first-spike latency and SD of the minimum latency in response to BF tone pips in anesthetized and awake IC. C, Histogram of SD of the latency in anesthetized and awake IC. Conventions as in Figure 3.
It has frequently been observed that cortical neurons under anesthesia tend to fire one or no spikes on each stimulus presentation (DeWeese et al., 2003
View larger version (11K):
[in this window]
[in a new window]
Figure 5. AI tone responses are more reliable in awake animals. A, B, Rasters of the first 100 ms of the responses of an example anesthetized (A) and awake (B) AI cell to a 200 ms BF tone. Windowed portions indicate the 20 ms ROI for determining the number of missed trials. C, Histogram of the proportion of missed trials in anesthetized and awake AI cells. Filled bars indicate anesthetized AI, and open bars indicate awake AI. D, Population plot of average firing rate for a 200 ms BF tone in anesthetized and awake AI. Horizontal lines indicate population medians.
Temporal response profiles differ dramatically between IC and AI
We have shown that the temporal characteristics of the early phase of the response of AI cells can be strongly affected by anesthesia and that these effects may obscure the response transformation between IC and AI. Are additional differences in the kinetics of IC and AI cell responses to long-lasting continuous stimuli confounded by anesthetic state? The response kinetics over a longer time period were examined by fitting a decaying exponential function to the PSTH for a 2 s tone (the PSTH of a typical awake AI cell is shown in Fig. 6A). This generated fit parameters A, k, and P for each cell, corresponding to a magnitude scaling factor, the inverse of the decay time constant, and the plateau firing rate, respectively (see Materials and Methods). We used the median values for each population to plot a "prototype" response adaptation profile for a typical anesthetized AI and a typical awake AI cell (Fig. 6C, gray lines). Clearly, the response profiles diverge considerably in both magnitude and shape: the anesthetized and awake AI cell populations differ significantly in all three fit parameters (Mann–Whitney U test, two-tailed; A, p = 0.0006, k, p = 0.0385, P, p = 0.0091; n = 65). The median awake AI cell fires at a rate of 37.2 spikes/s within the first 50 ms, and its response declines to a plateau of 0.4 spikes/s by the end of the 2 s stimulus; the median anesthetized AI cell, in contrast, progresses from an initial firing rate of 22 spikes/s to a plateau of 1.3 spikes/s. The time constant of firing rate decay is also significantly faster in awake AI cells, with a median value corresponding to 73 ms compared with 181 ms for anesthetized AI cells.
View larger version (19K):
[in this window]
[in a new window]
Figure 6. Temporal response profile to long constant stimuli in AI and IC. A, B, PSTH of the response of an example awake AI (A) and awake IC (B) cell to 10 trials of a 2 s BF tone. C, Response adaptation profiles in response to a 2 s BF tone for a typical cell in AI (gray lines) and IC (black lines), obtained from the population median parameters of an exponential decay curve fit to the PSTH of each cell. The curve begins at 50 ms to match the corresponding PSTH. Solid lines denote awake populations, and dashed lines denote anesthetized populations. Inset, Plateau firing rates for an example awake AI cell for four different types of continuous stimuli, from exponential decay curve fits.
Thus, AI response kinetics in the awake state are indeed substantially different from those predicted by anesthetized data. We analyzed the IC temporal response profile using the same method (the response of an example cell is shown in Fig. 6B). Interestingly, both the initial response level and the rate of decay are very similar with and without anesthesia; however, in anesthetized IC, the firing rate adaptation continues for a longer period (Fig. 6C, black lines). In this case, of the three fit parameters, only the plateau response magnitude differed significantly between anesthetized and awake IC (Mann–Whitney U test, one-tailed, p = 0.0016; n = 40), corresponding to a steady-state firing rate of 3.5 and 22.9 spikes/s, respectively.A direct comparison of response adaptation kinetics in IC and AI in the awake gerbil reveals a substantial coding transformation (Fig. 6C). In addition to responding with an initial firing rate equal to approximately half of that in IC, AI neurons exhibit a response that declines significantly faster (k, Mann–Whitney U test, two-tailed, p = 0.0369; n = 64) to a much lower steady-state firing level (P, Mann–Whitney U test, two-tailed, p < 0.0001; n = 64). The median values of k correspond to decay time constants of 257 ms for IC and 73 ms for AI neurons. The median plateau firing rates, as mentioned above, are 22.9 and 0.4 spikes/s for IC and AI cells, respectively. Comparing the curves in Figure 6C reveals that anesthesia reduces the apparent difference in temporal response profiles between IC and AI by lowering the steady-state firing rate of IC cells and increasing that of AI cells and by slowing adaptation in AI cells, thus obscuring the hierarchical transformation.
Interestingly, when a 2 s broadband noise burst stimulus is used instead of a BF tone, similar response adaptation is observed (data not shown). By 1.9 s after stimulus onset, the spike rate in the median awake IC cell declines to
It should be noted that, for individual AI cells, adaptation kinetics can vary significantly depending on how well the stimulus is optimized for the particular cell (Wang et al., 2005
Temporal responses to a dynamic stimulus transform greatly between IC and AI
We tested whether a hierarchical transformation also occurs in the temporal response profile to a dynamic stimulus modulated on a shorter timescale. We presented a series of SAM tones at different modulation frequencies and examined the ability of individual neurons to respond reliably at the same phase of every period (a quality that we termed "synchronization" to the stimulus). Long (10 s) stimuli were chosen to separate onset effects from ongoing temporal properties. First, we investigated the effects of anesthetic state on synchronization. Under anesthesia, a much larger proportion of AI neurons failed to show statistically significant synchrony (see Materials and Methods) to SAM at any of the tested modulation frequencies (36% in anesthetized AI vs 9% in unanesthetized AI). However, of the neurons responding synchronously to at least one modulation rate, a greater percentage continued to display significant synchrony to modulation rates above 5 Hz in the anesthetized AI population (Fig. 7D). This appears to be another example of improved temporal regularity in anesthetized AI. However, a greater proportion of awake AI cells than anesthetized AI cells synchronized to modulation rates below 2 Hz (Fig. 7D), and the corresponding vector strength values were generally much higher in the awake state (data not shown). For example, at 2 Hz the median vector strength for awake AI cells was 0.73 compared with 0.43 for anesthetized AI (Mann–Whitney U test, one-tailed, p < 0.0001; n = 70).
View larger version (20K):
[in this window]
[in a new window]
Figure 7. Temporal representation of envelope modulations in AI and IC. A, Period histograms of responses of four example cells, one from each study group, to six SAM frequencies. Normalization was performed separately for AI and IC. B, C, tMTFs of three representative awake AI (B) and IC (C) cells. A vertical line has been added to each graph at 20 Hz to facilitate comparison. D, Percentage of cells in AI (gray lines) and IC (black lines) showing significant synchrony (Rayleigh test, p < 0.001) to the period of SAM as a function of the modulation frequency. Solid lines denote awake and dashed lines denote anesthetized populations.
In the IC, nearly all cells synchronized to at least one SAM frequency in both awake and anesthetized conditions (97.7 and 94.5%, respectively). No difference was observed in the ability of these cells to fire synchronously to modulations at different rates (Fig. 7D).In the awake state, the temporal characteristics of SAM responses in IC and AI are strikingly different. Figure 7 shows examples of tMTFs of individual AI (Fig. 7B) and IC (Fig. 7C) neurons, generated by stimulating with 10-s-long SAM tones at different modulation frequencies and calculating a vector strength value for each. A vertical line has been added along the 20 Hz value on the abscissa for ease of comparison. It can be observed in these examples that, although tMTFs vary within each structure, IC tMTFs tend to be more bandpass and "roll over" at higher frequencies than those of AI cells. This difference in synchronization limit is very pronounced at the population level (Fig. 7D). We quantified this phenomenon by determining the synchrony cutoff frequency of each neuron tested with SAM in awake animals (see Materials and Methods). As expected, the median cutoff frequency for IC neurons (190 Hz) was significantly higher than for AI neurons (7 Hz) (Mann–Whitney U test, one-tailed, p < 0.0001; n = 88). To determine whether the synchronization limits of neurons were correlated with their response latency, we plotted these variables against one another (Fig. 8A). A negative relationship was observed in both the IC and AI population.
View larger version (16K):
[in this window]
[in a new window]
Figure 8. SAM tMTF cutoff is correlated with minimum latency and depends on stimulus duration. A, Individual cells in awake IC (filled squares) and AI (open circles). The sample is a subset of the full data because it was not always possible to obtain a reliable measure of minimum latency and SAM cutoff frequency in the same cell. B, Synchrony cutoff in 14 awake IC cells as assessed with 10 s and 400 ms SAM tones.
For some awake IC cells, we also tested brief SAM tones (400 ms) and compared the synchrony cutoff frequency for 400 ms and 10 s SAM stimuli. In most neurons, altering stimulus duration caused a change in the synchrony cutoff estimate; however, the direction of change varied across cells, and the overall range of cutoff values remained very similar (Fig. 8B).For a more detailed study of the way in which IC and AI represent modulations on the timescale important for speech (Houtgast and Steeneken, 1985
View larger version (29K):
[in this window]
[in a new window]
Figure 9. Discharge precision to the SAM envelope in AI and IC. Pooled period histograms of the responses of all tested AI (A) and IC (B) neurons to the period of a 10-s-long 2 Hz SAM tone. The stimulus envelope is indicated at the top. Awake data are represented by shaded bars, and anesthetized data are represented by semitransparent white bars, which are superimposed. Histograms were generated by adding the period histograms of individual cells in each population and normalizing. Values along the abscissa correspond to modulation phase, in which one 500 ms period equals 360°.
In IC, the difference between anesthetized and awake discharge patterns is less dramatic (Fig. 9B). The shapes of the pooled period histograms are very similar, although the maximal response in anesthetized IC occurs slightly earlier, and more adaptation is observed during the second half of the period.Is there a rate-coding transformation between IC and AI?
The previous sections have dealt with a temporal coding transformation between IC and AI and have shown how its interpretation has been complicated by anesthetic involvement. Others have demonstrated that firing rates in AI can also be strongly affected by anesthesia (Gaese and Ostwald, 2001Average firing rates to a 50 ms BF tone pip in awake and anesthetized AI constitute overlapping populations; however, responses in awake AI cells are significantly greater (Mann–Whitney U test, two-tailed, p = 0.0006; n = 72; median values, 18 spikes/s for anesthetized and 34 spikes/s for awake AI; data not shown). A similar trend is observed with 200-ms-long stimuli (Mann–Whitney U test, one-tailed, p = 0.0001; n = 86) (Fig. 5D). Conversely, no significant difference in firing rate was found between anesthetized and awake IC for either 50 ms (Mann–Whitney U test, one-tailed, p = 0.3948; n = 39; data not shown) or 200 ms tones (Mann–Whitney U test, one-tailed, p = 0.1405; n = 89; data not shown). Interestingly, any differences in sound-evoked discharge rate between our awake and anesthetized preparations cannot be attributed to an overall reduction in excitability: no significant difference in spontaneous firing rate was observed with anesthetic state in either IC (Mann–Whitney U test, one-tailed, p = 0.2161; n = 94; median, 3.8 spikes/s anesthetized and 2.4 awake; data not shown) or AI (Mann–Whitney U test, one-tailed, p = 0.1343; n = 74; median, 1.6 spikes/s anesthetized and 1.0 awake; data not shown).
In the absence of the suppressive effects of anesthetic, a substantial firing rate difference persists between IC and AI cells. In part, this distinction is amplified by the different adaptation kinetics in these structures; although in all cases, the IC neuron population tends to fire more strongly, the difference is more pronounced for longer stimuli (data not shown). Population comparisons of average firing rate for all three tested tone durations (50 ms, 200 ms, and 2 s) show IC and AI to be significantly different (50 ms: Mann–Whitney U test, one-tailed, p = 0.0289, n = 59; 200 ms: Mann–Whitney U test, one-tailed, p < 0.0001, n = 95; 2 s: Mann–Whitney U test, one-tailed, p < 0.0001, n = 71). A similar trend was observed with broadband noise burst stimulation (data not shown): although responses to 50 ms stimuli are significantly stronger in IC neurons than in AI cells (Mann–Whitney U test, one-tailed, p = 0.0085; n = 59), an even greater difference in firing rate was observed with 2 s noise bursts (Mann–Whitney U test, one-tailed, p < 0.0001; n = 95).
We also examined the modulation of firing rate as a function of SAM frequency. A best modulation frequency according to spike rate (rBMF) was determined for each cell and compared with its best modulation frequency for synchrony, or tBMF (see Materials and Methods). In awake IC neurons, no significant difference was observed between rBMF and tBMF values (data not shown; paired t test, one-tailed, p = 0.2326; n = 41), and the population means were 50 and 35 Hz, respectively. For awake AI cells, the rBMF tended to be somewhat higher than the tBMF (data not shown; paired t test, one-tailed, p = 0.0265; n = 49), but both numbers (means, 6.4 and 1.9 Hz, respectively) were low relative to those of IC neurons, as expected. Interestingly, in the anesthetized AI, rBMFs were slightly higher than in awake AI, mirroring the shift in synchrony limits (Mann–Whitney U test, two-tailed, p = 0.0425; n = 78; medians, 3.0 Hz anesthetized and 2.0 Hz awake AI). For the marmoset, it has been suggested that AI cells that fail to respond synchronously to modulating stimuli may nonetheless represent them with a rate code (Lu et al., 2001
Discussion
In awake animals, AI cells display higher variability than IC cells in signaling the beginning of a new stimulus or a new cycle in an ongoing modulation. Anesthetics significantly alter the temporal response profiles of AI cells to static as well as modulated stimuli but produce minor effects in IC. Data obtained from anesthetized preparations suggest an IC–AI coding transformation toward temporally precise, binary-like responses signaling the onsets of new stimuli or stimulus cycles; in contrast, recordings in the awake state suggest a quantitative rather than qualitative difference in response timing variability, adaptation kinetics, and envelope-tracking limits between IC and AI.Temporal coding in awake IC and AI
Although temporally precise onset spikes have frequently been viewed as a critical feature of cortical coding (Furukawa and Middlebrooks, 2002We show that AI responses to long, continuous stimuli exhibit substantially lower initial amplitudes, more rapid decay kinetics, and a lower steady-state firing level than those of IC cells. Although little systematic information is available on response adaptation kinetics in unanesthetized IC and AI, our results are consistent with two previous studies. The first (Goldstein et al., 1968
A striking observation is the similarity in the temporal profiles of responses to long-duration tones, noise, and SAM within each structure. This suggests a slow, stimulus-invariant temporal filter, with faster kinetics and more extensive filtering in AI (median time constants, 257 ms in IC and 73 ms in AI). This filter may gate the appearance of spikes to stimulus features occurring on a faster timescale, such as amplitude modulations in 20 Hz SAM, which IC neurons track with synchronous spikes.
In addition to a slow filter controlling response adaptation, our findings indicate a filtering process operating on a more rapid timescale. Responses to SAM suggest that IC can temporally track stimulus changes occurring at a rate of up to 190 Hz, whereas AI can do so up to only 7 Hz. These limits are broadly consistent with those reported previously for anesthetized and awake IC (Batra et al., 1989
Anesthetic effects on temporal coding
The barbiturate–ketamine anesthetic regimen in this study was chosen as representative of previous investigations in auditory cortical and collicular physiology. Pentobarbital prolongs the open time of GABA-activated chloride channels (Nicoll et al., 1975A difference in minimum response latency between anesthetized and unanesthetized cortical neurons has not been noticed previously, but our results are consistent with two previous reports on gerbil auditory cortex. Single and multiunit response latencies in anesthetized gerbil AI reportedly range between 10 and 25 ms for AI and the anterior auditory field (AAF) (Thomas et al., 1993
One potential explanation for this phenomenon is that different neural populations are sampled in recordings from anesthetized and unanesthetized animals. However, our distributions of BFs and thresholds indicate that the two populations are closely matched.
Another possibility is that an anesthesia-sensitive inhibitory mechanism ordinarily blocks depolarization and prevents early spikes in unanesthetized cortex. The disappearance of early inhibition under anesthesia may be attributable to pentobarbital-mediated GABAA receptor desensitization (Brownell et al., 1979
A final possibility is that the latency difference between anesthetized and unanesthetized animals arises subcortically but above the level of the inferior colliculus, and thus its mechanism could not be observed in this preparation.
The relatively higher limits of response synchronization to SAM in the anesthetized cortex are consistent with the shift toward shorter latencies. A similar relationship between response latency and synchronization is evident for trains of repeating tones in rat auditory cortex (Kilgard and Merzenich, 1999
In conclusion, cortical neurons are ideally suited to represent biologically relevant sounds. They temporally encode low-frequency modulations that predominate in natural sounds, including speech (Singh and Theunissen, 2003
Footnotes
Received Nov. 7, 2006; revised April 27, 2007; accepted April 28, 2007.This work was supported by National Institutes of Health Grant DC006864 (D.H.S.) and a grant from New York University (M.N.S.). We thank Dr. Shigeyuki Kuwada for helpful advice concerning the unanesthetized recording preparation and Kuei-Chu Chen for technical assistance.
Correspondence should be addressed to Malcolm N. Semple, Center for Neural Science, New York University, 4 Washington Place, Room 809, New York, NY 10003. Email: mal.semple{at}nyu.edu
Copyright © 2007 Society for Neuroscience 0270-6474/07/276091-12$15.00/0
References
Astl J, Popelar J, Kvasnak E, Syka J (1996) Comparison of response properties of neurons in the inferior colliculus of guinea pigs under different anesthetics. Audiology 35:335–345.[Web of Science][Medline]
Batra R, Kuwada S, Stanford TR (1989) Temporal coding of envelopes and their interaural delays in the inferior colliculus of the unanesthetized rabbit. J Neurophysiol 61:257–268.
[Abstract/Free Full Text] Brownell WE, Manis PB, Ritz LA (1979) Ipsilateral inhibitory responses in the cat lateral superior olive. Brain Res 177:189–193.[CrossRef][Web of Science][Medline]
Chase SM, Young ED (2006) Spike-timing codes enhance the representation of multiple simultaneous sound-localization cues in the inferior colliculus. J Neurosci 26:3889–3898.
[Abstract/Free Full Text] Chimoto S, Kitama T, Qin L, Sakayori S, Sato Y (2002) Tonal response patterns of primary auditory cortex neurons in alert cats. Brain Res 934:34–42.[CrossRef][Web of Science][Medline]
Creutzfeldt O, Hellweg FC, Schreiner C (1980) Thalamocortical transformation of responses to complex auditory stimuli. Exp Brain Res 39:87–104.[Web of Science][Medline]
DeWeese MR, Wehr M, Zador AM (2003) Binary spiking in auditory cortex. J Neurosci 23:7940–7949.
[Abstract/Free Full Text] Drullman R (1995) Temporal envelope and fine structure cues for speech intelligibility. J Acoust Soc Am 97:585–592.[CrossRef][Web of Science][Medline]
Eggermont JJ (1995) Representation of a voice onset time continuum in primary auditory cortex of the cat. J Acoust Soc Am 98:911–920.[CrossRef][Web of Science][Medline]
Feng HJ, Bianchi MT, Macdonald RL (2004) Pentobarbital differentially modulates alpha1beta3delta and alpha1beta3gamma2L GABAA receptor currents. Mol Pharmacol 66:988–1003.
[Abstract/Free Full Text] Franks NP, Lieb WR (1994) Molecular and cellular mechanisms of general anaesthesia. Nature 367:607–614.[CrossRef][Medline]
Furukawa S, Middlebrooks JC (2002) Cortical representation of auditory space: information-bearing features of spike patterns. J Neurophysiol 87:1749–1762.
[Abstract/Free Full Text] Gaese BH, Ostwald J (2001) Anesthesia changes frequency tuning of neurons in the rat primary auditory cortex. J Neurophysiol 86:1062–1066.
[Abstract/Free Full Text] Goldstein MH Jr, Hall JL II, Butterfield BO (1968) Single-unit activity in the primary auditory cortex of unanesthetized cats. J Acoust Soc Am 43:444–455.[CrossRef][Web of Science][Medline]
Goswami U, Thomson J, Richardson U, Stainthorp R, Hughes D, Rosen S, Scott SK (2002) Amplitude envelope onsets and developmental dyslexia: a new hypothesis. Proc Natl Acad Sci USA 99:10911–10916.
[Abstract/Free Full Text] Hefti BJ, Smith PH (2000) Anatomy, physiology, and synaptic responses of rat layer V auditory cortical cells and effects of intracellular GABA(A) blockade. J Neurophysiol 83:2626–2638.
[Abstract/Free Full Text] Hefti BJ, Smith PH (2003) Distribution and kinetic properties of GABAergic inputs to layer V pyramidal cells in rat auditory cortex. J Assoc Res Otolaryngol 4:106–121.[CrossRef][Medline]
Heil P (2004) First-spike latency of auditory neurons revisited. Curr Opin Neurobiol 14:461–467.[CrossRef][Web of Science][Medline]
Heil P, Irvine DR (1997) First-spike timing of auditory-nerve fibers and comparison with auditory cortex. J Neurophysiol 78:2438–2454.
[Abstract/Free Full Text] Houtgast T, Steeneken HJM (1985) A review of the MTF concept in room acoustics and its use for estimating speech intelligibility in auditoria. J Acoust Soc Am 77:1069–1077.[CrossRef][Web of Science]
Kilgard MP, Merzenich MM (1999) Distributed representation of spectral and temporal information in rat primary auditory cortex. Hear Res 134:16–28.[CrossRef][Web of Science][Medline]
Kong YY, Zeng FG (2006) Temporal and spectral cues in Mandarin tone recognition. J Acoust Soc Am 120:2830–2840.[CrossRef][Web of Science][Medline]
Krishna BS, Semple MN (2000) Auditory temporal processing: responses to sinusoidally amplitude-modulated tones in the inferior colliculus. J Neurophysiol 84:255–273.
[Abstract/Free Full Text] Kuwada S, Batra R, Stanford TR (1989) Monaural and binaural response properties of neurons in the inferior colliculus of the rabbit: effects of sodium pentobarbital. J Neurophysiol 61:269–282.
[Abstract/Free Full Text] Leong D, Puil E, Schwarz D (2004) Ketamine blocks non-N-methyl-D-aspartate receptor channels attenuating glutamatergic transmission in the auditory cortex. Acta Otolaryngol 124:454–458.[CrossRef][Medline]
Liang L, Lu T, Wang X (2002) Neural representations of sinusoidal amplitude and frequency modulations in the primary auditory cortex of awake primates. J Neurophysiol 87:2237–2261.
[Abstract/Free Full Text] Lu T, Wang X (2004) Information content of auditory cortical responses to time-varying acoustic stimuli. J Neurophysiol 91:301–313.
[Abstract/Free Full Text] Lu T, Liang L, Wang X (2001) Temporal and rate representations of time-varying signals in the auditory cortex of awake primates. Nat Neurosci 4:1131–1138.[CrossRef][Web of Science][Medline]
MacDonald RL, Rogers CJ, Twyman RE (1989) Barbiturate regulation of kinetic properties of the GABAA receptor channel of mouse spinal neurones in culture. J Physiol (Lond) 417:483–500.
[Abstract/Free Full Text] Malone BJ, Semple MN (2001) Effects of auditory stimulus context on the representation of frequency in the gerbil inferior colliculus. J Neurophysiol 86:1113–1130.
[Abstract/Free Full Text] Malone BJ, Scott BH, Semple MN (2000) Processing of sinusoidal modulations of amplitude and frequency in the auditory cortex of alert rhesus macaques. Soc Neurosci Abstr 26:358–18.
Mickey BJ, Middlebrooks JC (2003) Representation of auditory space by cortical neurons in awake cats. J Neurosci 23:8649–8663.
[Abstract/Free Full Text] Mitani A, Shimokouchi M, Itoh K, Nomura S, Kudo M, Mizuno N (1985) Morphology and laminar organization of electrophysiologically identified neurons in the primary auditory cortex in the cat. J Comp Neurol 235:430–447.[CrossRef][Web of Science][Medline]
Nicoll RA, Eccles JC, Oshima T, Rubia F (1975) Prolongation of hippocampal inhibitory postsynaptic potentials by barbiturates. Nature 258:625–627.[CrossRef][Medline]
Phillips DP, Farmer ME (1990) Acquired word deafness, and the temporal grain of sound representation in the primary auditory cortex. Behav Brain Res 40:85–94.[CrossRef][Web of Science][Medline]
Phillips DP, Hall SE (1990) Response timing constraints on the cortical representation of sound time structure. J Acoust Soc Am 88:1403–1411.[CrossRef][Web of Science][Medline]
Rose HJ, Metherate R (2005) Auditory thalamocortical transmission is reliable and temporally precise. J Neurophysiol 94:2019–2030.
[Abstract/Free Full Text] Ruotsalainen S, Haapalinna A, Riekkinen PJ Sr, Sirvio J (1997) Dexmedetomidine reduces response tendency, but not accuracy of rats in attention and short-term memory tasks. Pharmacol Biochem Behav 56:31–40.[CrossRef][Web of Science][Medline]
Schulze H, Ohl FW, Heil P, Scheich H (1997) Field-specific responses in the auditory cortex of the unanaesthetized Mongolian gerbil to tones and slow frequency modulations. J Comp Physiol A Neuroethol Sens Neural Behav Physiol 181:573–589.[CrossRef][Web of Science][Medline]
Shannon RV, Zeng FG, Kamath V, Wygonski J, Ekelid M (1995) Speech recognition with primarily temporal cues. Science 270:303–304.
[Abstract/Free Full Text] Singh NC, Theunissen FE (2003) Modulation spectra of natural sounds and ethological theories of auditory processing. J Acoust Soc Am 114:3394–3411.[CrossRef][Web of Science][Medline]
Spitzer MW, Semple MN (1993) Responses of inferior colliculus neurons to time-varying interaural phase disparity: effects of shifting the locus of virtual motion. J Neurophysiol 69:1245–1263.
[Abstract/Free Full Text] Stecker GC, Middlebrooks JC (2003) Distributed coding of sound locations in the auditory cortex. Biol Cybern 89:341–349.[CrossRef][Web of Science][Medline]
Thomas H, Tillein J, Heil P, Scheich H (1993) Functional organization of auditory cortex in the mongolian gerbil (Meriones unguiculatus). I. Electrophysiological mapping of frequency representation and distinction of fields. Eur J Neurosci 5:882–897.[CrossRef][Web of Science][Medline]
Tollin DJ, Populin LC, Yin TC (2004) Neural correlates of the precedence effect in the inferior colliculus of behaving cats. J Neurophysiol 92:3286–3297.
[Abstract/Free Full Text] Wang X, Lu T, Snider RK, Liang L (2005) Sustained firing in auditory cortex evoked by preferred stimuli. Nature 435:341–346.[CrossRef][Medline]
Wehr M, Zador AM (2003) Balanced inhibition underlies tuning and sharpens spike timing in auditory cortex. Nature 426:442–446.[CrossRef][Medline]
Wehr M, Zador AM (2005) Synaptic mechanisms of forward suppression in rat auditory cortex. Neuron 47:437–445.[CrossRef][Web of Science][Medline]
Wu SH, Kelly JB (1994) Physiological evidence for ipsilateral inhibition in the lateral superior olive: synaptic responses in mouse brain slice. Hear Res 73:57–64.[CrossRef][Web of Science][Medline]
Wu SH, Oertel D (1986) Inhibitory circuitry in the ventral cochlear nucleus is probably mediated by glycine. J Neurosci 6:2691–2706.[Abstract]
Zeng FG, Nie K, Stickney GS, Kong YY, Vongphoe M, Bhargave A, Wei C, Cao K (2005) Speech recognition with amplitude and frequency modulations. Proc Natl Acad Sci USA 102:2293–2298.
[Abstract/Free Full Text]
Related articles in J. Neurosci.:
- This Week in The Journal
J. Neurosci. 2007 27: i.[Full Text]
This article has been cited by other articles:
S. M. N. Woolley, P. R. Gill, T. Fremouw, and F. E. Theunissen
Functional Groups in the Avian Auditory System
J. Neurosci., March 4, 2009; 29(9): 2780 - 2793.
[Abstract] [Full Text] [PDF]
E. B. Issa and X. Wang
Sensory Responses during Sleep in Primate Primary and Secondary Auditory Cortex
J. Neurosci., December 31, 2008; 28(53): 14467 - 14480.
[Abstract] [Full Text] [PDF]
Y. Zheng and M. A. Escabi
Distinct Roles for Onset and Sustained Activity in the Neuronal Code for Temporal Periodicity and Acoustic Envelope Shape
J. Neurosci., December 24, 2008; 28(52): 14230 - 14244.
[Abstract] [Full Text] [PDF]
K. A. Razak and Z. M. Fuzessery
Facilitatory Mechanisms Underlying Selectivity for the Direction and Rate of Frequency Modulated Sweeps in the Auditory Cortex
J. Neurosci., September 24, 2008; 28(39): 9806 - 9816.
[Abstract] [Full Text] [PDF]
B. Krebs, N. A. Lesica, and B. Grothe
The Representation of Amplitude Modulations in the Mammalian Auditory Midbrain
J Neurophysiol, September 1, 2008; 100(3): 1602 - 1609.
[Abstract] [Full Text] [PDF]
D. Bendor and X. Wang
Neural Response Properties of Primary, Rostral, and Rostrotemporal Core Fields in the Auditory Cortex of Marmoset Monkeys
J Neurophysiol, August 1, 2008; 100(2): 888 - 906.
[Abstract] [Full Text] [PDF]
M. Pecka, A. Brand, O. Behrend, and B. Grothe
Interaural Time Difference Processing in the Mammalian Medial Superior Olive: The Role of Glycinergic Inhibition
J. Neurosci., July 2, 2008; 28(27): 6914 - 6925.
[Abstract] [Full Text] [PDF]
J. C. Middlebrooks
Auditory Cortex Phase Locking to Amplitude-Modulated Cochlear Implant Pulse Trains
J Neurophysiol, July 1, 2008; 100(1): 76 - 91.
[Abstract] [Full Text] [PDF]
H. Xu, V. C. Kotak, and D. H. Sanes
Conductive Hearing Loss Disrupts Synaptic and Spike Adaptation in Developing Auditory Cortex
J. Neurosci., August 29, 2007; 27(35): 9417 - 9426.
[Abstract] [Full Text] [PDF]
This Article Abstract 
Full Text (PDF) Submit an eLetter Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Citation Map Services Email this article to a friend Related articles in J. Neurosci. Similar articles in this journal Similar articles in ISI Web of Science Similar articles in PubMed Alert me to new issues of the journal Download to citation manager 
Citing Articles Citing Articles via HighWire Citing Articles via ISI Web of Science (3) Citing Articles via Google Scholar Google Scholar Articles by Ter-Mikaelian, M. Articles by Semple, M. N. Search for Related Content PubMed PubMed Citation Articles by Ter-Mikaelian, M. Articles by Semple, M. N.
|
|
|
|
 |
|