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The Journal of Neuroscience, November 15, 1998, 18(22):9500-9516
The Functional Influence of Burst and Tonic Firing Mode on Synaptic Interactions in the Thalamus
Uhnoh Kim and David A. McCormick Section of Neurobiology, Yale University School of Medicine, 333 Cedar Street, New Haven, Connecticut 06510
ABSTRACT
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Abstract
Introduction
Thalamocortical and perigeniculate (PGN) neurons can generate action potentials either as Ca2+ spike-mediated high-frequency bursts or as tonic trains. Using dual intracellular recordings in vitro in monosynaptically connected pairs of PGN and dorsal lateral geniculate nucleus (LGNd) neurons, we found that the functional effect of synaptic transmission between these cell types was strongly influenced by the membrane potential and hence the firing mode of both the pre- and postsynaptic neurons. Activation of single action potentials or low-frequency spike trains in PGN or thalamocortical neurons resulted in the generation of PSPs that were 0.5-2.0 mV in amplitude. In contrast, the generation of Ca2+ spike-mediated bursts of action potentials in the presynaptic cell increased these PSPs to an average of 4.4 mV for the IPSP and 3.0 mV for the EPSP barrage, because of temporal summation and/or facilitation. If the postsynaptic neuron was at a resting membrane potential (e.g.,
65 mV), these PSP barrages could result in the activation of a low-threshold Ca2+ spike and burst of action potentials. These results demonstrate that the burst firing mode of action potential generation is a particularly effective means by which perigeniculate and thalamocortical neurons may influence one another. We propose that the activation of burst discharges in these cell types is essential for the generation of some forms of synchronized rhythmic oscillations of sleep and of epileptic seizures.
Key words: inhibition; excitation; perigeniculate; thalamocortical; thalamic reticular; spindle waves
INTRODUCTION
Thalamocortical and thalamic reticular (perigeniculate) neurons exhibit two distinct modes of action potential generation. During periods of slow wave sleep, rhythmic burst firing mediated by the activation of low-threshold Ca2+ spikes is prevalent, whereas during waking, activity in both cell types is dominated by the occurrence of trains of action potentials (Mukhametov et al., 1970a
,b
The interactions between the GABAergic neurons of the thalamic reticular or perigeniculate nuclei and the thalamocortical cells during the waking, or tonic discharge, state are less well understood. In the dorsal lateral geniculate nucleus, these interactions have been suggested to contribute to feedforward and feedback, as well as binocular and far-field, inhibition within the LGNd (Lindström, 1982
Intracellular and extracellular recordings from numerous cell types in varying regions of the mammalian brain, including the neocortex, hippocampus, superior colliculus, and brainstem, indicate that neurons that generate either burst, tonic, or both types of activity are relatively common (e.g., Kandel and Spencer, 1961
Intracellular studies of neurons maintained in the ferret LGNd and PGN slice provide a unique opportunity to examine the properties of these two modes of action potential generation on synaptic transmission in the mammalian brain, because this preparation functionally maintains the extensive connections between the excitatory thalamocortical and inhibitory PGN neurons (e.g., Bal et al., 1995a
MATERIALS AND METHODS
Sagittal slices of the ferret LGNd and PGN were formed as described previously and were maintained at 35°C in an interface style recording chamber (Bal et al., 1995a
Intracellular recording electrodes were formed on a Sutter Instruments P-80 micropipette puller from medium-walled glass (1BF100; WPI) and were beveled on a Sutter Instruments beveler. Micropipettes were filled with 1.2 M potassium acetate and 2% biocytin for intracellular labeling of recorded neurons and had resistances of between 60 and 100 M
. Biocytin-filled neurons were visualized via the standard avidin-biotin-horseradish peroxidase reaction with diaminobenzidine (Horikawa and Armstrong, 1988
Some portions of the data obtained from the 41 pairs of PGN to LGNd cells have been published elsewhere (Kim et al., 1997
RESULTS
Dual intracellular recordings were obtained from 45 pairs of monosynaptically connected PGN and thalamocortical (LGNd) neurons in the ferret geniculate slice maintained in vitro (40 pairs, PGN to LGNd; 4 pairs, LGNd to PGN; and 1 pair, both directions). The properties of synaptic transmission between these two types of neuron were examined via the injection of depolarizing and hyperpolarizing current pulses in the presynaptic neuron to activate tonic trains or bursts of action potentials. In addition, the membrane potential of the pre- and postsynaptic neurons was manipulated via the intracellular injection of DC.
The properties of synaptic transmission between PGN and thalamocortical cells are summarized in Figure 1. Single action potentials in PGN neurons evoked monosynaptic IPSPs that were 0.5-1.9 mV in amplitude in thalamocortical cells (Fig. 1B), whereas single action potentials in thalamocortical cells evoked EPSPs that were 0.7-2.0 mV in amplitude in PGN cells (Fig. 1G). The activation of prolonged trains of action potentials in PGN or thalamocortical neurons resulted in trains of IPSPs or EPSPs, respectively, that exhibited temporal summation in the postsynaptic neuron (Fig. 1C,H). Activation of a low-threshold Ca2+ spike-mediated burst in the presynaptic neuron resulted in a large summated IPSP or EPSP barrage in the postsynaptic cell (Fig. 1D,I). Functionally, the activation of an IPSP by the burst discharge of a single PGN cell could result in the generation of a rebound low-threshold Ca2+ spike in the thalamocortical cell (Fig. 1E), and the activation of an EPSP barrage by a burst of action potentials in the thalamocortical cell could activate a low-threshold Ca2+ spike and burst of action potentials in the PGN neuron (Fig. 1J).
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Figure 1. Properties of synaptic connections between PGN and thalamocortical neurons. A, Schematic diagram of the recording arrangement for recordings in B-E is shown. The PGN neuron was activated via the intracellular injection of a depolarizing current pulse while recording from a recipient thalamocortical neuron in lamina A of the LGNd. B, Low-frequency (20-50 Hz) tonic firing in the PGN neuron activates small (0.5-1.9 mV) IPSPs in the thalamocortical cell (arrows). C, Increasing the frequency of discharge of the PGN neuron to an average of 170 Hz results in temporal summation of the IPSPs. D, Activation of a burst discharge in the PGN neuron results in a larger summated IPSP in the postsynaptic thalamocortical cell. E, Activation of a presynaptic burst in a PGN neuron could activate a rebound Ca2+ spike and burst in a thalamocortical cell. F, Schematic diagram of the recording arrangement for recordings in G-J is shown. The thalamocortical cell was activated with the intracellular injection of current. G, Low-frequency (10-30 Hz) firing in the thalamocortical neuron resulted in 0.7-2.0 mV EPSPs in the PGN cell. H, Increasing the discharge of the thalamocortical cell to an average of 80 Hz results in temporal summation of the EPSPs. I, A presynaptic burst of action potentials in the thalamocortical cell results in a summated barrage of EPSPs in the PGN neuron. J, Activation of a presynaptic burst in a thalamocortical cell could activate a burst in a PGN neuron, which then could activate a barrage of IPSPs in the thalamocortical cell. The upward- and downward-pointing arrows indicate temporal correlation between burst of action potentials and the activation of postsynaptic potentials. Data are from four different cell pairs (B-D, E, G-I, J).
Perigeniculate inhibition of thalamocortical neurons: single-spike and tonic activity
The generation of action potentials at low frequencies (~1 Hz) in PGN neurons that were monosynaptically connected with a simultaneously recorded LGNd cell resulted in IPSPs with a relatively fixed latency of ~1 msec. The mean amplitude of these single IPSPs varied considerably among different pairs of cells, ranging from just above the noise level (0.1-0.2 mV) to 1.01 ± 0.30 mV in the most strongly connected pair in our sample (n = 15 pairs analyzed). Single-spike-evoked IPSPs reached their peak amplitude within 2-5 msec from onset and exhibited a duration at half-amplitude of 10-50 msec (Fig. 2A,B), which was similar to the membrane time constants (14-37 msec; n = 6 pairs), measured from a 5 to 10 mV change in membrane potential in response to the injection of a hyperpolarizing current pulse.
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Figure 2. Properties of synaptic transmission from PGN to thalamocortical cells at low frequencies. A, Activation of single action potentials at ~1 Hz in the PGN cell with the intracellular injection of depolarizing current results in single IPSPs in the postsynaptic thalamocortical neuron. B, Overlap of 20 single IPSPs is shown. The single IPSPs range from 0.6 to 1.2 mV in amplitude. C, Examples of the increase and decrease in the size of the second IPSPs activated at interspike frequencies of 5-80 Hz are shown. Da-Dc, Plots of sizes of the first versus the second IPSPs that are activated in the frequency range of 5-80 Hz in four different pairs are shown. The mean sizes of the first IPSPs in these pairs were 0.53, 0.80, 0.95, and 0.88 mV, whereas those of the second IPSPs were 0.53, 0.73, 0.75, and 0.78 mV, respectively. The diagonal lines indicate no change in amplitude between the first and second IPSPs. The vertical dotted lines indicate the mean sizes of the first IPSPs. E, In pairs 1 and 2, the sizes of the second IPSPs are not significantly different from those of the first IPSPs, whereas in pair 3, the second IPSPs are consistently depressed in amplitude. In pair 4, the amplitude of the second IPSPs decreased if the first IPSP was larger than average.
The relationship between the frequency of action potential activity in the PGN cell and the amplitude of the resulting postsynaptic IPSPs was systematically examined. When a train of two to five action potentials was evoked in the PGN cell in the frequency range of 5-80 Hz (n = 5 pairs analyzed), the activation of the first IPSP either had little effect or resulted in the depression of the second IPSP. For example, in three connected pairs (see Fig. 2Da,Db,E, pairs 1 and 2), the sizes of the second IPSPs varied independently of that of the first, and the mean sizes of the first and second IPSPs were not significantly different. However, in pair 3 (Fig. 2Dc,E), the second IPSP was consistently depressed in amplitude, as was evident in the significantly smaller mean size of the second IPSPs (0.75 ± 0.27 mV) compared with that of the first (0.95 ± 0.19 mV; paired t test, p = 0.003). In pair 4 (Fig. 2Dc,Dd,E), the depression of the second IPSP occurred in association with the activation of a large first IPSP. The mean size of the second IPSP, given that the first IPSP was larger than average, was 0.67 ± 0.09 mV and was significantly smaller than the average of the first IPSPs in all trials (0.88 ± 0.31 mV; p = 0.03). In contrast, the mean size of the second IPSP after a first IPSP that was smaller than average was 0.85 ± 0.13 mV and, therefore, was not significantly different from the average of the first IPSPs.
The generation of repetitive trains of action potentials at frequencies greater than ~20-50 Hz resulted in temporal summation of postsynaptic IPSPs (Fig. 3). There were two phases in this summation. During the initial 30-50 msec, the IPSPs summated markedly, depending on the frequency of presynaptic activity (Fig. 3Ba,Bb). However, after this time period, the individual IPSPs decreased in amplitude as did the compound IPSP (Fig. 3A,D).
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Figure 3. High-frequency discharge results in summation and facilitation in PGN to LGNd synaptic transmission. A, When action potentials are generated at >100 Hz in frequency, the amplitudes of the first four to six IPSPs (arrows) progressively increase, followed by individual IPSPs of diminished amplitude. The number above each trace is the average frequency of action potential discharge. Ba, The number of single-spike IPSPs that contribute to the peak amplitude increases with increasing rate of presynaptic action potential generation. Bb, The peak amplitude of summated IPSPs increases with increasing rate of action potential generation. Bc, The averaged amplitude per single-spike IPSP (peak amplitude of summated IPSPs/number of action potentials) also grows with increasing rate of action potential generation and is larger than the mean of single IPSPs activated at an interspike frequency of ~1 Hz (horizontal dashed line), indicating facilitation in synaptic transmission during the high-frequency action potential generation. C, Amplitude of facilitation in the initial IPSPs is frequency dependent. Ca, Plot of amplitudes of the second and third individual IPSPs versus the first activated by a train of presynaptic action potentials at 150-300 Hz are shown. The diagonal line indicates no change in the amplitude. Cb, Plots of amplitude ratios of the second and third IPSPs to the first as a function of discharge rate of the presynaptic PGN cell are shown. The ratios increase with increasing rate of the action potential generation. The horizontal line indicates no change in the amplitude between the first and the second or third IPSPs. The diagonal lines represent the best-fit linear regression, exhibiting that the magnitude of facilitation is larger in the third IPSP in comparison with the second. D, Despite maintained discharge of the PGN cell at high frequency, the summated IPSPs reach a peak and then decline gradually in amplitude to a steady state level. Data in A-C are from one cell pair and in D are from another.
In part because of temporal summation, the peak amplitude of the compound IPSP increased relatively linearly with increasing rate of presynaptic action potential generation (Fig. 3Bb). However, at higher frequencies of activation (>100 Hz), the amplitude of the compound IPSP was substantially larger than expected, given the amplitude of the single-spike IPSPs. Under these circumstances, the average amplitude of the single-spike IPSPs during the tonic train of action potentials increased with increasing discharge rate of the PGN cell and was larger than was the mean amplitude of single IPSPs activated at ~1 Hz (Fig. 3Bc).
Facilitation during the first three IPSPs generated at higher frequencies (>100 Hz) was examined more closely. Plots of amplitudes of the first versus second or third IPSPs activated during a train of presynaptic action potentials at 150-300 Hz revealed that the second and third IPSPs were consistently larger than was the first irrespective of the amplitude of the first IPSPs (Fig. 3Ca). The facilitation in single-spike IPSP amplitude was greater for the third IPSP than for the second. The mean size of the second IPSPs was 1.4-1.6 times larger than was that of the first IPSP, whereas the mean amplitude of the third IPSP was 1.8-2.1 times larger (n = 6 pairs). The degree of facilitation increased with increasing rate of discharge of the presynaptic PGN cell (Fig. 3Cb).
Perigeniculate inhibition of thalamocortical neurons: burst discharge
The generation of bursts of action potentials in PGN cells, via the activation of a low-threshold Ca2+ spike, resulted in a 350-550 Hz barrage of IPSPs in the postsynaptic cell (Fig. 4A,B), the temporal summation and facilitation of which resulted in compound IPSPs that were up to 11.06 ± 0.78 mV in amplitude in the most strongly connected pair of cells from our sample. Because the time-to-peak of single IPSPs ranged from 2.5 to 3.2 msec on average among pairs of cells (n = 15 pairs), the single-spike IPSPs activated during the burst discharge of action potentials at 350-550 Hz presumably overlapped in their temporal development, and therefore it was not possible to measure the true amplitude of individual IPSPs during the burst. For this reason, we calculated the average amplitude per single-spike IPSPs by dividing the peak amplitude of the postsynaptic compound IPSPs by the number of action potentials generated in the burst.
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Figure 4. Burst discharges are associated with summation and facilitation of IPSPs from the PGN to LGNd. A, A burst discharge of action potentials results in the summated IPSPs that increase in peak amplitude with increasing rate of presynaptic action potential generation. Note that each action potential, even at 450 Hz, results in a postsynaptic IPSP. The frequency of action potentials is an average during the burst. B, Overlap of the summated IPSPs in A is shown. C, The averaged amplitude per single-spike IPSP grows progressively above the mean size of single IPSPs activated at 1 Hz (horizontal dashed line) with increasing rate of action potential generation. Da, The averaged amplitude per single-spike IPSP is plotted as a function of the mean size of single IPSPs at 1 Hz in 11 different pairs. In each pair, the mean size of single IPSPs at 1 Hz was calculated over 30-60 trials, whereas the averaged amplitude per single-spike IPSP during burst generation was derived from averaging 10-20 bursts of action potentials at 450-550 Hz. In every pair, the averaged amplitude per single-spike IPSP during a burst is larger than is the mean size of single IPSPs activated at low frequencies. These results are indicative of facilitation in synaptic transmission during the burst of high-frequency action potentials. The diagonal line indicates no change in amplitude. Each point represents the average from a single pair. Db, The ratio of the average amplitude per single-spike IPSP during a burst to the mean amplitude of low-frequency single IPSPs was plotted as a function of the mean size of single IPSPs. The amplitude ratio shows a tendency to decrease in pairs of larger mean sizes of single IPSPs, although this result does not reach statistical significance. E, F, Relationship between the amplitude of the compound IPSP after four (E) or six (F) action potentials and the frequency of action potential generation in the tonic and burst firing mode in two cell pairs are shown.
The average single-spike IPSP amplitude was larger during presynaptic burst discharge than was the mean amplitude of single IPSPs activated at interspike frequencies of ~1 Hz in all pairs tested (n = 11). These results confirm the presence of facilitation in the efficacy of the synaptic transmission from PGN to LGNd during high-frequency discharge (Fig. 4C,Da). The facilitation in the transmission by the burst discharge was again a function of the rate of action potential generation in that the average single-spike IPSP amplitude increased progressively with increasing rate of action potential generation (Fig. 4C). Even in one connected pair of cells in which single IPSPs after presynaptic action potentials at 1 Hz were barely detectable (0.1-0.2 mV), the burst discharge of a presynaptic PGN cell evoked compound IPSPs of ~3 mV, from which was calculated an average IPSP amplitude per single spike of 0.51 mV (data not shown).
There was a weak (r =
Changing the membrane potential of the thalamocortical neuron had significant effects on the response of these cells to the IPSP barrage (Fig. 5). At relatively hyperpolarized membrane potentials (e.g., Fig. 5A,
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Figure 5. Membrane potential of the thalamocortical cell determines the functional effect of presynaptic bursts in a PGN cell. A, B, Depolarization of the thalamocortical cell by only 3 mV results in abolition of rebound burst firing [
Single PGN cells can activate both GABAA and GABAB receptor-mediated IPSPs
We have demonstrated previously that activation of single PGN cells can activate both GABAA and GABAB receptor-mediated IPSPs in thalamocortical cells, depending on the pattern of presynaptic action potential generation (Fig. 6) (see Kim et al., 1997
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Figure 6. The progressive block of GABAA receptors reveals the contribution of GABAB receptor activation. A, In control, the burst discharge of the presynaptic PGN cell results in a large IPSP and the activation of a rebound low-threshold calcium spike. The temporal development of this rebound calcium spike overlaps and conceals the activation of the GABAB receptor-mediated IPSP. The bath infusion of bicuculline methiodide (100 µM) gradually blocks the fast, GABAA receptor-mediated component of the evoked IPSP, and this also results in a loss of the rebound low-threshold Ca2+ spike. After 20-25 min, both GABAA and GABAB receptor-mediated IPSPs are activated after a single burst in the PGN cell. After 40 min, bicuculline infusion completely blocks the GABAA receptor-mediated IPSP and unveils the pure GABAB receptor-mediated IPSPs. B, Overlap of the responses in A is shown. Note that the number of action potentials generated by the PGN cell also increased in the presence of bicuculline.
The convergence and divergence of connections between populations of PGN and LGNd cells underlie the propagation and synchronization of spontaneous spindle waves in ferret LGNd slices in vitro (Kim et al., 1995
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Figure 7. Degree of convergence of PGN neurons onto single thalamocortical cells. A, Induction of a burst discharge in presynaptic PGN cells in two connected pairs ~1-2 sec before the arrival of a spindle wave initiated three cycles of IPSPs in the recipient thalamocortical cell via divergent and convergent connections between the two population of neurons. During the generation of a spindle wave, the same thalamocortical cells received a barrage of IPSPs that grew in amplitude, resulting from recruitment of convergent PGN cells into the oscillation. B, Overlay of a summated IPSP from the burst discharge of a single presynaptic PGN cell with the peak IPSP (* in A) generated during spindle oscillation reveals a three- to fourfold increase in IPSP amplitude during the spindle oscillation. Because of the nonlinear nature of the summation of IPSPs from a population of convergent PGN cells, especially as summated IPSPs reach the reversal potential, this ratio will underestimate the degree of convergence. Data obtained from two different cell pairs are shown. Pairs in Aa and Ab are shown in Ba and Bb.
Whereas the induction of a single burst in a presynaptic PGN cell activated postsynaptic IPSPs of ~2-11 mV in amplitude, the same postsynaptic LGNd cell received barrages of IPSPs of ~9-24 mV in amplitude during spontaneous generation of spindle oscillations. The average amplitude of IPSPs induced by burst firing in PGN cells was 4.4 ± 2.5 mV, whereas the average peak amplitude of IPSPs in the same thalamocortical neurons during spindle wave generation was 15.5 ± 3.6 mV (n = 30 pairs).
During the generation of spindle oscillations, PGN cells generate repetitive burst discharges of action potentials at an interburst frequency of 6-10 Hz. Here we examined how this repetitive burst discharge may affect synaptic transmission between PGN and LGNd cells. When PGN cells were induced to generate repetitive bursts of action potentials at interburst frequencies >1 Hz, the second barrage of IPSPs decreased in amplitude in comparison with the first, whereas relatively little change in amplitude was observed between the second and the subsequent barrages of IPSPs whether they were mediated by GABAA (Fig. 8A; n = 4 pairs) or GABAB (Fig. 8B) receptors.
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Figure 8. Effects of repetitive discharge of the presynaptic neuron on synaptic transmission between thalamocortical and PGN neurons. A, Repetitive burst discharges in a PGN neuron result in IPSP barrages that decrease in amplitude, particularly between the first and second barrages, despite increases in the number of action potentials generated by the presynaptic neuron. The depression in amplitude of the second barrage of IPSPs begins to occur at interburst frequencies >1 Hz, with the amplitude reduced by one-half at ~5 Hz. B, In the presence of bicuculline, GABAB receptor-mediated IPSPs also exhibit decrements in amplitude between the first and second slow IPSPs. C, Repetitive burst firing in a thalamocortical cell, induced by the intracellular injection of hyperpolarizing current pulses, results in barrages of EPSPs in a PGN neuron. These EPSP barrages do not change markedly in peak amplitude with repetitive activation. D, Overlap of the indicated IPSP and EPSP barrages is illustrated. Sharp, spike-like events above the EPSP barrages are capacitance-coupling artifacts.
Thalamocortical excitation of perigeniculate neurons
The probability of obtaining monosynaptic connections from a thalamocortical neuron to a PGN cell was significantly less than that in the other direction, presumably because of the markedly less dense axon collaterals formed in the PGN by thalamocortical cells in comparison with those formed in the LGNd by PGN cells (Ferster and LeVay, 1978
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Figure 9. Properties of monosynaptic connections between thalamocortical neurons and recipient PGN cells. A, Activation of tonic firing in a thalamocortical neuron results in a train of EPSPs in the PGN neuron. Increasing the frequency of action potential generation in the thalamocortical neuron results in temporal summation of these EPSP barrages. Note that the EPSP barrages reach a plateau and do not show facilitation. B, Activation of bursts of action potentials in the thalamocortical neuron results in summated barrages of EPSPs in the PGN cell. C, Overlays of postsynaptic recordings in A and B are shown. D, Changing the membrane potential of the postsynaptic neuron alters the functional effect of the EPSP barrage. Depolarization of the PGN neuron from
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Figure 10. The amplitude of single-spike EPSPs in the postsynaptic PGN cell decreases during the generation of a high-frequency train of action potentials in the presynaptic thalamocortical cell. A, At low-frequency discharge rates (70-90 Hz), EPSP amplitudes are relatively stable. B, At higher frequency (100-150 Hz) rates of presynaptic discharge, the EPSPs exhibit a steady decrement in amplitude. C, The EPSPs during an increased intensity of presynaptic discharge (210 Hz) decrease markedly after the first EPSP.
The activation of a burst-induced barrage of EPSPs in a PGN neuron at a membrane potential of
During the generation of spindle waves, each PGN cell received from a population of thalamocortical cells EPSP barrages that grew in amplitude eventually to activate low-threshold calcium-mediated burst discharges (Fig. 11A). The peak amplitude of these EPSP barrages reached 16-24 mV. Single-burst discharges of presynaptic thalamocortical cells activated EPSP barrages that were an average of 3.0 ± 1.0 mV (n = 4) in recipient PGN cells, suggesting a five- to eightfold increase in the peak amplitude of EPSP barrages during spindle oscillation, because of the synchronized discharge of convergent thalamocortical cells onto single PGN cells (Fig. 11).
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Figure 11. Evidence of convergence of multiple thalamocortical cells onto single PGN cells. A, Injection of hyperpolarizing current pulses into thalamocortical cells in two different pairs induces burst discharges that then generate EPSPs in the postsynaptic PGN cells. During spindle waves, the same PGN cells receive barrages of EPSPs that grow in amplitude during successive cycles of oscillation and that activate low-threshold calcium spikes and plateau potentials. B, Comparing the amplitude of single-burst EPSPs with that of the peak subthreshold EPSPs (* in A) during spindle oscillation illustrates the convergence of multiple thalamocortical cells onto the single PGN cells. Because EPSPs from a population of presynaptic LGNd cells are likely to summate in a nonlinear manner, the amplitude ratio between the two will underestimate the degree of convergence. Pairs in Aa and Ab are shown in Ba and Bb.
Repetitive activation of burst discharges at 5-9 Hz resulted in the generation of repetitive barrages of EPSPs in PGN neurons (Fig. 8C). In contrast to IPSP barrages between PGN and thalamocortical cells, these EPSP barrages did not exhibit significant decreases in peak amplitude with repetitive activation (Fig. 8C,D).
DISCUSSION
Our results demonstrate that synaptic transmission from PGN to LGNd cells is highly dynamic, depending on the pattern of activity in the presynaptic PGN cell. The amplitude of individual IPSPs generated by action potentials in the PGN cell may be either larger or smaller than that of the previous IPSPs, depending on the frequency of action potential activity and the number of action potentials generated in the immediate past. Recent investigations of synaptic transmission between hippocampal pyramidal cells have demonstrated that the probability of transmitter release is dependent on whether or not the preceding action potential in the train results in the release of neurotransmitter (Dobrunz and Stevens, 1997
The generation of action potentials in PGN cells at frequencies greater than ~100 Hz resulted in the strong facilitation of synaptic transmission during the initial three to five IPSPs (Figs. 1, 3, 4). Presumably, this increase in IPSP amplitude resulted from an increase in release of transmitter, perhaps via a Ca2+-dependent mechanism (e.g., Magleby, 1987
In addition to short-term facilitation and depression, the repetitive activation of bursts in PGN cells also exhibited depression of synaptic transmission between the first and second response that occurred at frequencies between 1 and 8 Hz and that persisted for ~1 sec (Fig. 8A,B). A similar frequency-dependent depression of GABAergic synaptic transmission has been demonstrated in pyramidal cells of the hippocampus and cerebral cortex (Deisz and Prince, 1989
Properties of thalamocortical synapses onto PGN cells
Activation of an action potential in a single thalamocortical cell resulted in EPSPs that are 0.7-2.0 mV in amplitude in the postsynaptic PGN neuron. This EPSP amplitude is similar to that for the influence of pyramidal cells in the hippocampus and cerebral cortex onto local interneurons (Miles, 1990
In contrast to our observations on the PGN to thalamocortical cell synapse, we did not observe facilitation in the postsynaptic EPSPs generated by thalamocortical cells in PGN neurons, even at high frequencies. With repetitive activation, thalamocortical EPSPs exhibited pronounced decrements in amplitude (Figs. 9, 10), which may result from both pre- and postsynaptic influences such as the saturation of postsynaptic receptors (Tang et al., 1994
Functional properties of burst and tonic mode
The burst and lower frequency tonic firing modes of action potential generation seem to differ in their effects on synaptic transmission in the thalamus attributable in part to the temporal summation of PSPs, to the temporally isolated nature of burst discharges, and, in the case of PGN to thalamocortical cell synapses, to facilitation at high frequencies. The first and last differences result from the high frequencies (300-500 Hz) of action potential discharge associated with burst discharges. Thus, if a quiescent PGN neuron were to generate action potentials in the tonic firing mode at a rate that was comparable with that of burst discharges, then similar levels of summation and facilitation are expected to occur in the postsynaptic response. Presumably, the presynaptic terminals formed by PGN axons experience only the pattern of action potential generation arriving at these terminals and are not influenced by the mechanisms by which these action potential patterns are generated at the soma (e.g., via a low threshold Ca2+ spike or tonic discharge). However, if the PGN neuron generates a high-frequency tonic discharge in the midst of ongoing tonic activity, then the resulting IPSP should be smaller than that during an isolated burst discharge because of large decreases in synaptic facilitation (e.g., Fig. 3) and postsynaptic response (Fig. 8A,B). Therefore, isolated, high-frequency burst discharges are particularly effective in activating large IPSPs in postsynaptic thalamocortical cells. Although it has not been specifically addressed, it is widely assumed that PGN neurons generate high-frequency discharges primarily, or exclusively, via the activation of low-threshold Ca2+ spikes and that the tonic mode of action potential generation is associated with activity in the frequency range of 0-200 Hz (Mukhametov et al., 1970a
As we have reported previously for spindle wave-associated IPSPs, the IPSPs activated by single PGN cells seem to be mediated almost entirely via the activation of GABAA receptors. After the block of GABAA receptors and strong activation of the PGN cell, we found a small (1-3 mV) residual slow IPSP that is mediated by GABAB receptors (e.g., Fig. 6) (see also Kim et al., 1997
conductances through GABAA receptors (Sodickson and Bean, 1996
The generation of prolonged trains of action potentials in PGN cells resulted in postsynaptic IPSPs that increased and then decreased in amplitude. The reduction in IPSP amplitude may contribute to the "waning" of spindle waves or the antagonism of synchronized oscillations, although this influence is most likely minor, because block of GABAB receptors, which generally reduces or blocks reduction of IPSP amplitude during repetitive stimulation (see Thompson et al., 1993
As with the PGN input onto thalamocortical cells, burst firing in thalamocortical neurons was especially effective in activating hyperpolarized PGN cells, because of temporal summation of the EPSPs during the burst. Interestingly, we did not observe any noticeable changes in the amplitude of these EPSP barrages with repetitive burst firing, indicating that decrement of this synaptic connection is also unlikely to contribute to the waning of spindle waves.
With the PGN in the tonic firing mode, barrages of EPSPs generated by burst firing in thalamocortical cells were only effective in activating an extra action potential in the PGN neuron. Presumably this results from the large currents involved in the generation of action potentials overriding the relatively small currents generated by EPSPs arriving from a single thalamocortical neuron. However, when the PGN cells are hyperpolarized, the EPSP barrages can trigger the low-threshold Ca2+ current and therefore generate a high-frequency burst discharge. The findings that burst firing in PGN cells is essential to the generation of IPSPs that are large enough in amplitude to result in the generation of rebound burst firing in thalamocortical cells and that thalamocortical cells need to be hyperpolarized for this to occur suggest that the generation of synchronized slow oscillations such as spindle waves (and some forms of spike-and-wave seizure) may require that both PGN and thalamocortical cells be in the hyperpolarized state. Indeed, we have shown previously that depolarization of either thalamocortical cells or PGN neurons into the tonic firing mode with the application of various neurotransmitters results in an abolition of spindle wave generation (Lee and McCormick, 1996
Summary
Thalamocortical activity exhibits at least three distinct states in vivo: tonic activity during waking and REM sleep, repetitive burst firing during non-REM sleep, and high-frequency, prolonged burst firing during some forms of generalized seizures (Steriade et al., 1986
FOOTNOTES Received Feb. 11, 1998; revised Aug. 25, 1998; accepted Aug. 28, 1998.
This research was supported by grants from the National Institutes of Health, the Klingenstein Fund, the McKnight Foundation, and the Human Frontiers Science Program. Additional information about these and related findings may be obtained at http://info.med.yale.edu/neurobio/mccormick/mccormick.html.
Correspondence should be addressed to Dr. David A. McCormick, Section of Neurobiology, Yale University School of Medicine, 333 Cedar Street, New Haven, CT 06510.
APPENDIX Our present physiological recordings, together with previous anatomical results (Kim et al., 1997
Convergence from perigeniculate to thalamocortical neurons
Our physiological and morphological results indicate that each PGN cell gives rise to a relatively strong connection to at least a subset of thalamocortical cells. In the five examples that we examined, we identified 11, 60, 62, 69, and 69 putative synaptic contacts from a single PGN cell onto a postsynaptic thalamocortical cell (Kim et al., 1997Divergence from perigeniculate to thalamocortical neurons
In four cells we estimated the number of putative synaptic contacts formed by perigeniculate cells in the LGNd by counting the number of beads or swellings formed by the axons of these cells. These counts ranged from ~3000 to 5000 synaptic contacts, which is similar to that estimated previously in the cat LGNd (Uhlrich et al., 1991Convergence of thalamocortical to PGN cells
Although we have not yet determined the number of contacts from a thalamocortical cell onto a single PGN cell, these are likely to be relatively low. The axon collaterals formed by single thalamocortical cells in the PGN typically do not bifurcate extensively nor give rise to dense synaptic plexuses (Ferster and LeVay, 1978
REFERENCES
- Ahlsen G, Lindström S, Lo FS (1985) Interaction between inhibitory pathways to principal cells in the lateral geniculate nucleus of the cat. Exp Brain Res 58:134-143[ISI][Medline].
- Avoli M, Gloor P, Kostopoulos G, Naquet R (1990) In: Generalized epilepsy. Neurobiological approaches. Boston: Birkhauser.
- Bal T, McCormick DA (1996) What stops synchronized thalamocortical oscillations? Neuron 17:297-308[ISI][Medline].
- Bal T, von Krosigk M, McCormick DA (1995a) Synaptic and membrane mechanisms underlying synchronized oscillations in the ferret LGNd in vitro. J Physiol (Lond) 483:641-663[ISI][Medline].
- Bal T, von Krosigk M, McCormick DA (1995b) Role of the ferret perigeniculate nucleus in the generation of synchronized oscillations in vitro. J Physiol (Lond) 483:665-685[ISI][Medline].
- Buhl EH, Halasy K, Somogyi P (1994) Diverse sources of hippocampal unitary inhibitory postsynaptic potentials and the number of synaptic release sites. Nature 368:823-828[Medline].
- Colquhoun D, Jonas P, Sakmann B (1992) Action of brief pulses of glutamate on AMPA/kainate receptors in patches from different neurones of rat hippocampal slices. J Physiol (Lond) 458:261-287
[Abstract/Free Full Text] .- Contreras D, Steriade M (1995) Cellular basis of EEG slow rhythm: a study of dynamic corticothalamic relationships. J Neurosci 15:604-622[Abstract].
- Davies CH, Collingridge GL (1993) The physiological regulation of synaptic inhibition by GABAB autoreceptors in rat hippocampus. J Physiol (Lond) 472:245-265
[Abstract/Free Full Text] .- Debanne D, Guerineau NC, Gahwiler BH, Thompson SM (1995) Physiology and pharmacology of unitary synaptic connections between pairs of cells in areas CA3 and CA1 of rat hippocampal slice cultures. J Neurophysiol 73:1282-1294
[Abstract/Free Full Text] .- Deisz RA, Prince DA (1989) Frequency-dependent depression of inhibition in guinea-pig neocortex in vitro by GABAB receptor feed-back on GABA release. J Physiol (Lond) 412:513-541
[Abstract/Free Full Text] .- Destexhe A, Sejnowski TJ (1995) G-protein activation kinetics and spillover of gamma-aminobutyric acid may account for differences between inhibitory responses in the hippocampus and thalamus. Proc Natl Acad Sci USA 92:9515-9519
[Abstract/Free Full Text] .- Dobrunz LE, Stevens CF (1997) Heterogeneity of release probability, facilitation, and depletion at central synapses. Neuron 18:995-1008[ISI][Medline].
- Domich L, Oakson G, Steriade M (1986) Thalamic burst patterns in the naturally sleeping cat: a comparison between cortically projecting and reticularis neurones. J Physiol (Lond) 379:429-449
[Abstract/Free Full Text] .- Dutar P, Nicoll RA (1988a) A physiological role for GABAB receptors in the central nervous system. Nature 332:156-158[Medline].
- Dutar P, Nicoll RA (1988b) Pre- and postsynaptic GABAB receptors in the hippocampus have different pharmacological properties. Neuron 1:585-591[ISI]
