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The Journal of Neuroscience, April 15, 2002, 22(8):3277-3284
Midline Thalamic Region: Widespread Excitatory Input to the Entorhinal Cortex and Amygdala
D. X. Zhang and E. H. Bertram Department of Neurology, University of Virginia Health Science Center, Charlottesville, Virginia 22908
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
The midline thalamus has a role in memory formation and has well described projections to multiple limbic sites including the hippocampus, amygdala, and entorhinal cortex. Stimulation of this region evokes excitatory responses in the CA1 region of the hippocampus, but nothing is known about the nature of thalamic influence on other limbic sites such as the entorhinal cortex and the amygdala. In this study we electrically stimulated the midline thalamus in anesthetized rats to determine whether responses could be evoked in the amygdala or entorhinal cortex. In addition we examined the distribution of the responses within the target regions as well as the effect of short interval paired or high-frequency tetanizing stimulation. We found reproducible responses in the entorhinal cortex and the amygdala with a distribution of responses that matched the described synaptic input from the thalamus. In addition, high-frequency stimulation induced a consistent long-term potentiation in the two sites. Paired stimulation resulted in depression of the test response in the amygdala, but a facilitation in the entorhinal cortex. These findings indicate that the midline has a significant monosynaptic excitatory influence in the amygdala and the entorhinal cortex. Combined with the previous work in the hippocampus, this study suggests that the midline thalamus plays a significant role in limbic physiology and may serve to synchronize activity in this system.
Key words: thalamus; amygdala; entorhinal cortex; physiology; long-term potentiation; thalamolimbic regional interactions; limbic system
INTRODUCTION
The midline thalamus, including the medial dorsal nucleus, may play a significant role in certain types memory formation (Parker et al., 1997
; Aggleton and Brown, 1999
Early reports of thalamic influence on the cortex (Morison and Dempsey, 1942
The reciprocal anatomic connections between the midline thalamic region and multiple limbic sites such as the hippocampus, entorhinal cortex, and the amygdala(Aggleton and Mishkin, 1984
MATERIALS AND METHODS
Animal preparation. The major methods are similar to our previous paper describing the hippocampal response to thalamic stimulation (Bertram and Zhang, 1999
The electrodes were inserted into the brain stereotactically using target coordinates from a standard atlas (Paxinos and Watson, 1986
3.3 mm. A thalamic twisted pair bipolar stainless steel stimulating electrode insulated with a Teflon coating with only the cut ends exposed (wire diameter, 0.125 mm; tip separation, 1.0 mm) was placed in the midline thalamus (1.8-2.3 mm posterior to bregma, lateral 0.4-0.8 mm to the midline, 5.5-6.3 mm below the dura, with a 5° arm angle from vertical axis for the entorhinal cortex experiments and a 0° angle for the amygdala experiments). This position was in the lower aspect of the medial dorsal nucleus or just above the rhomboid and reuniens nuclei. The recording electrodes were glass micropipettes filled with 0.9% NaCl and 1% Fast Green. To help position the thalamic stimulating electrode, an additional recording electrode was placed into the CA1 pyramidal cell layer (5.4-5.6 mm posterior to bregma, 4.8-5.0 mm lateral to the midline, and 2.3-2.5 mm below the dura) to record the maximal thalamic induced CA1 response after adjusting thalamic stimulating and CA1 recording electrode depths. The intensity of thalamic stimulation (duration, 0.2 msec; monophasic) inducing a maximal CA1 response was used as the initial stimulating intensity of the thalamic projection to entorhinal cortex and the amygdala.
Basic characteristics and topography of responses. The purpose of this series of experiments was to define the basic parameters of the responses in the entorhinal cortex and the amygdala at defined anteroposterior and mediolateral positions. The characteristics under examination included the presence of a response, the presence of a population spike, and the latencies to the peaks of significant early responses. These observations were compared with the responses obtained in CA1 after thalamic stimulation. In some animals the responses were recorded from a minimum of two anteroposterior planes separated by at least 0.5 mm. In the entorhinal cortex the nominal anteroposterior placements were (relative to bregma)
The nominal placements for the amygdala recording electrodes were
Each collected response is an average of five consecutive responses induced by stimuli delivered once every 10 sec. Responses were evaluated, as noted above, for latency and maximal amplitude, as well as for the presence of a population spike. In each anteroposterior plane, the relative position of the response with the shortest latencies and maximal amplitudes (as determined by the maximal amplitude negative responses) was noted.
Long-term potentiation. LTP is generally considered to be a monosynaptic process that is induced by several brief, high-frequency stimuli (Schwartzkroin and Wester, 1975
The conditioning stimulus consisted of two trains (separated by 10 sec) of 100 pulses delivered at 100 Hz. The intensity for the conditioning stimulus was the same as for the baseline and test stimulus single pulses. The intensity for the single stimuli were set to provide a response that was approximately half of the maximal amplitude so that there was potential for a potentiation of the response. The responses were evaluated by amplitude and peak latency of the largest negative response (Fig. 1, N2), and after the conditioning trains, these characteristics were compared with the baseline responses as percentage of change.
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Figure 1. Basic field responses. A, Typical EC and amygdala responses to midline thalamic stimulation. Most early responses were an initial positive deflection (P1) followed by a larger negative wave (N2). After the stimulus there was a variable initial negative potential that was not included in the evaluation. B, Bilateral response in EC with superimposed population spike after stimulation at a single point in the midline thalamus. For some of the evoked responses, there was a well developed spike discharge mixed in with or superimposed on the N2 wave (arrow). This latter response was not seen consistently in all animals. When recorded bilaterally, similar responses were found ipsilateral and contralateral to stimulation. In each trace there is an initial positive 5 mV calibration pulse followed several milliseconds later by a lower amplitude stimulation artifact that is partially blanked.
Paired-pulse studies. Paired stimuli given at short intervals (e.g., 20 msec) in the hippocampus are a synaptic response that results in a second (or test) response that is typically smaller than the first (an observation usually called paired-pulse inhibition or depression). We had previously found that thalamic stimulation of sufficient intensity could induce paired-pulse depression in the CA1 region of the hippocampus, although this depression was less than usually observed after contralateral CA3 stimulation (Bertram and Zhang, 1999
Stimulation at 20 msec interval was used to determine whether there was any difference in the responses to thalamic stimulation between CA1 pyramidal cell layer and entorhinal cortex or amygdala. Before the recording electrode was placed into entorhinal cortex or amygdala, the CA1 responses to paired-pulse thalamic stimulation were recorded. After the recording electrode was placed into entorhinal cortex or amygdala, the responses to paired-pulse thalamic stimulation were recorded again. These responses were obtained in the region of each AP plane that provided the maximal response after thalamic stimulation. The intensities of test and conditioning stimulation were set at levels sufficient to induce a maximum conditioning response, because we have found that this intensity provides the most consistent and reliable results. Responses were evaluated for change in amplitude of the primary negative potential (Fig. 1A, N2). We chose a standardized AP plane for this analysis for the entorhinal cortex (EC) (bregma
Histology. At the end of each experiment, the electrode positions were marked for histological confirmation. The Fast Green in the recording electrode was iontophoresed into the surrounding tissue by using negative direct current (20-50 µA; 5-10 min) at the end of the experiment. The positions of the recording electrode in that AP plane were extrapolated from this one position. Positive direct current (10 V for 5-10 sec) was passed through the negative tip (lower) of the stimulating electrodes to deposit iron from the electrode into the surrounding tissue. The animals were decapitated while still under anesthesia, and the brains were removed and placed into fixative consisting of 1% potassium ferrocyanide and 4% formaldehyde. The fixed brains were frozen and sectioned at 40 µm. The sections were stained for Nissl with thionine. The electrode positions with the maximal response were determined by the position of the iontophoresed Fast Green, and the other electrode positions more were determined by extrapolation based on the distance moved between recording positions. Each position was plotted on a standard diagram for each AP plane of study, and the responses recorded were correlated to each position (Paxinos and Watson, 1997
Statistical evaluation. All data are presented as means ± SEM. Quantitative comparisons were made in the paired-pulse and long-term potentiation experiments. For the paired-pulse data, the percentage of change in amplitude of the second or test response was compared between either the amygdala or entorhinal cortex and the hippocampal CA1 response. The percentage of change was determined for each individual response, and the two groups (either CA1 and amygdala or CA1 and entrorhinal cortex) were compared with a t test.
For the LTP experiments data after the conditioning stimulation (percentage of change in amplitude or latency) were compared with the normalized values obtained immediately before conditioning with a one-way ANOVA with repeated measures (ANOVA-RM). Post hoc pairwise comparisons between the last baseline value and each of the postconditioning points were made with a Student-Newman-Keuls test. For all comparisons significance was set at a level of p < 0.05.
RESULTS
Basic response characteristics
Responses were obtained throughout the EC and the amygdala. Although there was some variation in the qualitative features of the field response, the overall morphology of the maximal amplitude responses in the amygdala and EC was quite similar. For some responses there was an initial low-amplitude negative response (N1) that was quite variable in its presence and appearance, but was found in the amygdala and EC without predilection for a particular region or site within a region. The first consistent response across animals and sites was a positive response (P1) (Fig. 1A). This response was followed by a higher amplitude negative wave (N2). The responses increased in amplitude with increasing stimulus intensity (Fig. 2A,B). On occasion, negative spikes or multiple spikes were superimposed on N2 (for examples, see Figs. 1B, 2A), and in general these spikes were only seen when N2 was at or near maximal amplitude (Fig. 2A).
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Figure 2. Basic depth profile of EC and amygdala response. A, EC responses recorded at
In comparing the latency and amplitudes of the EC and amygdala responses to the CA1 response in the hippocampus the latency to onset of the response was similar, but the peak latencies for N2 are longer. The N2 response was also longer in duration and lower in amplitude in EC and amygdala compared with CA1 (see Table 1 for latency and amplitude data).
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Table 1. Latencies and amplitudes of primary responses in CA1, EC and amygdala The responses were seen throughout the EC and amygdala, but there was usually an area of maximal amplitude and shortest latency in each AP plane examined. For the EC the responses tended to be higher in amplitude in the more lateral areas of layers II and III. There was a clear phase reversal as the electrode moved into the superficial portions of layer II and layer I. (Figs. 2A, 3). For the amygdala the responses were of highest amplitude and shortest latency in the area around the basal nucleus (lateral mid to ventral aspect of the amygdala) (Figs. 2B, 3). The mediolateral differences in response were less pronounced in EC than in amygdala (Fig. 3). As noted above there was a clearly graded response to increasing stimulus intensity, with a likely postsynaptic response that evolves to a higher amplitude response with occasional superimposed spike discharges (Fig. 2A,B). As seen in Table 2 the responses were seen with similar latencies and amplitudes throughout the anteroposterior extent of the EC and amygdala.
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Figure 3. Mediolateral distribution of EC and amygdala responses. Responses to thalamic stimulation recorded ~0.5 mm posterior to responses shown in Figure 2. Responses are obtained at depth that gives approximately the greatest amplitude response. There is little shift in EC amplitude in the three mediolateral positions, but for the amygdala the greatest amplitude is consistently in the more lateral positions. Brain diagrams from Paxinos and Watson (1997)
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Table 2. Amplitudes and latencies from different anterior posterior planes Within the midline thalamus there was a region that clearly elicited the maximal responses in EC and amygdala when stimulated. As shown in Figure 4 this region corresponded to the ventral aspects of the MD, with some extension into the upper rhomboid nucleus. This thalamic region was similar to the midline thalamic region that elicited the maximal response in CA1. When the stimulating electrode was placed 2 mm laterally from the midline and moved ventrally through the lateral dorsal and ventrolateral nuclei, we could not evoke responses in EC and amygdala (data not shown).
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Figure 4. EC and amygdala responses to different midline thalamic stimulation positions. The numbers next to the responses are the approximate positions of the negative (bottom) tip of the stimulating electrode. The extent of the stimulating electrode trajectory was confirmed histologically. The recording electrodes were kept at the indicated positions as the stimulating electrode was moved through the thalamus. These observations indicate that the midline site for eliciting responses in the EC (n = 4) and amygdala (n = 3) is restricted to a narrow area. Brain diagrams from Paxinos and Watson (1997)
In a small number of animals we recorded in the EC and amygdala on both sides (ipsilateral and contralateral to stimulation). We found responses that were essentially identical on the two sides. See Figure 1B for responses in the EC ipsilateral and contralateral to stimulation.
Paired-pulse studies
Short-interval paired stimulation evoked opposite responses in the EC and the amygdala. The amygdala responded like CA1 with a significant suppression of N2 (p < 0.05; t test). On the other hand, EC had a significant facilitation of the response (p < 0.001; t test). (Fig. 5, Table 3). These responses were obtained at a maximal conditioning response and were the same throughout the EC and amygdala. The data displayed are from a standardized site in one AP plane for the EC and amygdala, but the relative nature of the paired response was similar throughout each region.
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Figure 5. Short-interval (20 msec) paired-pulse stimulation. Stimulus intensities were adjusted to achieve maximal response by midline thalamic stimulation. The evoked CA1 responses show the well described depression of the test response to thalamic stimulation. In comparison, the test EC response by the same thalamic stimulation shows a significant facilitation. Like the CA1 response, the amygdala shows a significant suppression of the test response. The data for these responses are shown in Table 3.
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Table 3. Short-interval paired-pulse response amplitude changes Long-term potentiation
LTP was induced in the EC and amygdala (Fig. 6). For the amygdala (n = 5) the baseline amplitude for the N2 response was 2.95 ± 0.69 mV, and the latency was 18.22 ± 0.12 msec. There was a significant increase in the amplitude (p < 0.001; F = 11.295; between group df = 7) and a significant decrease in the latency (p < 0.001; F = 36.772; between group df = 7). Post hoc pairwise comparison (Student-Newman-Keuls) between baseline and each of the points after conditioning reveal that each amplitude and latency measure after conditioning was significantly different from baseline (p < 0.001 for all points, amplitude and latency).
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Figure 6. Long-term potentiation. A, Long-term potentiation in the EC and amygdala. After the conditioning stimuli, there is a significant and sustained (at least 30 min after conditioning) increase in amplitude of the EC and amygdala response (filled circles). There is also a significant shortening of the latency in the amygdalar response, whereas there is only a slight decrease in latency in the EC (open circles). B, Means of amplitudes and latencies for EC (n = 7) and amygdala (n = 5), reflecting the changes after the conditioning stimuli. Bars indicate SEM. For the amygdala there was a significant shortening of the duration and an increase in the amplitude (p < 0.001 ANOVA-RM for the two measures). For the EC there was a significant increase in amplitude (p = 0.004 ANOVA-RM) and a significant decrease in peak latency (p = 0.01 ANOVA-RM).
For the EC (n = 7) the baseline amplitude was 2.30 ± 0.28 mV, and the latency was 13.00 ± 0.72 msec. There was also a significant increase in amplitude of the response after conditioning (p = 0.004, F = 3.686, between group df = 7) and a significant decrease in latency (p = 0.01, F = 3.166, between group df = 7). Post hoc Student-Newman-Keuls testing showed that all postconditioning latency changes were significantly less than baseline (p < 0.04 for all points). For amplitude, the post hoc pairwise comparison indicated that the first three points and the last measured point after conditioning were significantly greater than baseline (p < 0.04 for these four points).
DISCUSSION
The major finding of this study is the excitatory response in the amygdala and the entorhinal cortex that follow midline thalamic stimulation. This finding, together with our previous description of similar excitatory responses in the CA1 region of the hippocampus, suggests that the midline thalamic nuclei can play a significant role in the physiology of these major limbic regions. The circuitry within and between each region is complex. The interactions between several regions (e.g., the hippocampus and entorhinal cortex) are well described, and these observations raise the possibility that the recorded responses are polysynaptic (e.g., a thalamically induced CA1 response that subsequently evokes an EC response). However, the LTP studies, which demonstrated potentiation in the EC and amygdala, suggest that the primary responses that we recorded were monosynaptic (Schwartzkroin and Wester, 1975
The efferents from the midline thalamus to the limbic system are widespread, but within each region there are areas that receive a greater proportion of terminals from the thalamus, as assessed by tract tracing studies. In the hippocampus, the majority of the thalamic afferents are found in apical dendrites of CA1, as well as in the subiculum (with the subiculum sending axons back to the medial dorsal thalamic nucleus) (Herkenham, 1978
The projection neurons within the midline, on the basis of retrograde tract tracing studies, have predominantly unilateral projections with only minimal crossing of midline (Su and Bentivoglio, 1990
It is of some note that the stimulus intensity to elicit maximal responses was somewhat higher than is seen for evoking responses in the hippocampus when stimulating locally, as we have seen in previous studies (Bertram and Zhang, 1999
The relatively high stimulus intensities necessary to evoke responses in the target site may raise concerns that the responses were the result of the inadvertent stimulation of a site adjacent to the midline thalamic region or of fibers that traversed the stimulated region. These concerns may be partially ameliorated by the observations that were made in Figure 4: there was a narrow window in the midline region for eliciting these responses. Although we show data for midline electrode positions, we also found that electrodes placed 2 mm lateral to the midline failed to elicit responses. We cannot completely exclude the possibility that some fibers of passage might be inadvertently stimulated, but there are no such fibers, to our knowledge, in the region of the thalamus that elicits maximal response. Even if there were, the observation that stimulation in a single central site evokes excitatory responses from the three separate limbic sites is unique and emphasizes the potential role this region has in limbic system function.
There may also be concerns about the regions in the EC and amygdala that generate the responses, that what we are recording are far field responses generated by neighboring structures. It is difficult to determine a well defined point of maximal response. That difficulty may be related, in part, to the rather diffuse and widespread pattern of thalamic axon terminals seen throughout the EC and amygdala as well as the more widely distributed neuronal populations in these two regions, compared with the more tightly distributed pyramidal cells of CA1. The observation of reversals of polarity as the recording electrode was moved through the EC and amygdala (Figs. 2, 3). supports the hypothesis that the responses are generated locally in the two regions.
The primary observation of this study that there is a significant monosynaptic excitatory input from the thalamus to the entorhinal cortex and amygdala, combined with the previous studies of thalamic excitation of the hippocampus, suggests that the thalamus plays a significant role in the physiology of the limbic system. Because it has widespread connections to the limbic as well as cortical and subcortical structures, the midline thalamic region may have a powerful synchronizing role. Much work needs to be performed in follow up to this initial study with regard to the nature of these synapses, their location, and their pharmacology. There also needs to be an understanding of the thalamolimbic circuit, because, as with the thalamocortical circuit, there are major projections from these limbic sites back to the thalamus. Additional work examining the nature of the regional interactions within the thalamus is also necessary. An understanding of these pathways and circuits will no doubt give us a better understanding of the functions associated with these structures, including memory and limbic epilepsy.
FOOTNOTES Received Oct. 23, 2001; revised Jan. 29, 2002; accepted Feb. 7, 2002.
This study was supported by National Institutes of Health, National Institute of Neurological Disorders and Stroke Grant NS 25605. We thank John Williamson for his technical expertise.
Correspondence should be addressed to Edward H. Bertram, P. O. Box 800394, University of Virginia, Department of Neurology, Charlottesville, VA 22908-0394. E-mail: ehb2z{at}virginia.edu.
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