Department of Neurobiology, Duke University Medical Center, Durham, North Carolina 27710
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ABSTRACT |
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Özen, Gülden, George J. Augustine, and William C. Hall. Contribution of Superficial Layer Neurons to Premotor Bursts in the Superior Colliculus. J. Neurophysiol. 84: 460-471, 2000. In vitro whole-cell patch-clamp methods were used to examine the contribution of one component of intracollicular circuitry, the superficial gray layer, to the generation of bursts of action potentials that occur in the intermediate layer and that command head and eye movements in vivo. Applying a single brief (0.5 ms) pulse of current to the superficial layer of rat collicular slices evoked prolonged bursts of excitatory postsynaptic currents (EPSCs) in the cells of the intermediate layer. The EPSCs were sufficient to elicit bursts of action potentials that lasted as long as 300 ms and resembled presaccadic command bursts. To examine the contribution of neurons within the superficial layer to the production of these bursts, we determined how superficial neurons respond to the same current pulses that evoke bursts in the intermediate layer. Recordings from 61 superficial layer cells revealed 19 neurons that produced multiple action potentials following stimulation. Nine of these 19 neurons were wide- and narrow-field vertical cells, which are known to project to the intermediate layer and could contribute to producing the EPSC bursts. The remaining cells (n = 42) did not generate trains of action potentials and 21 of these showed only subthreshold potential changes in response to the stimulus. Our results indicate that most superficial cells do not directly contribute to production of the EPSC bursts, but a small number do have the properties necessary to provide a prolonged excitatory drive to the premotor neurons.
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INTRODUCTION |
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The superior
colliculus is composed of layers with sensory and motor functions,
which provides an opportunity to address the fundamental problem of how
sensory signals are translated into the command signals for movements.
Recent in vitro experiments demonstrated a strong functional link
between the superficial visuosensory and intermediate premotor layers
of the superior colliculus in the tree shrew and rat (Isa et al.
1998; Lee et al. 1997
). Of particular interest
was the observation, in tree shrew, that applying single, brief
electrical stimuli to the superficial layer of the superior colliculus
evokes strong and prolonged synaptic excitation of intermediate layer
premotor neurons (Lee et al. 1997
). These prolonged
responses may be generated by the same collicular circuitry responsible
for producing the bursts of action potentials that command saccadic
head and/or eye movements in vivo (Goldberg and Wurtz
1972
; Munoz and Guitton 1986
; Munoz et al. 1991
; Sparks 1978
; Sparks and Nelson
1987
; Wurtz and Albano 1980
; Wurtz and
Goldberg 1972
; Wurtz and Mohler 1976
).
The present experiments examined the circuitry responsible for
the excitatory postsynaptic current (EPSC) bursts that are generated in
the intermediate layer. One possibility is that these prolonged
synaptic responses are produced by trains of action potentials
generated by neurons within the superficial layer itself. Although the
superficial layer contains distinct types of neurons (Hall and
Lee 1993; Isa et al. 1998
; Langer and
Lund 1974
; Lee and Hall 1995
; Lund and
Lund 1972
; Mooney et al. 1988
;
Moschovakis et al. 1988
; Shi et al. 1997
;
Sterling 1971
; Warton and Jones 1985
;
Warton et al. 1990
), not enough is known about their
synaptic connectivity or physiological properties to predict whether
bursts could arise in the superficial layer itself. Thus it is not
clear whether the electrical stimuli that evoke prolonged EPSC bursts in the premotor neurons do so by evoking bursts of action potentials in
superficial neurons. Alternatively, recurrent axonal collaterals arising from cells in the underlying optic and/or intermediate layers
of the colliculus (Hall and Lee 1997
; Lee and
Hall 1995
; Mooney et al. 1988
;
Moschovakis et al. 1988
) might give rise to positive
feedback that prolongs and strengthens transient signals that arrive
from the superficial layer (Arai et al. 1994
;
Pettit et al. 1999
).
In the present study, we examined the origins of
intermediate-layer EPSC bursts in the rat superior colliculus. First,
we confirmed that rat intermediate layer neurons produce prolonged bursts of EPSCs that resemble those reported in the tree shrew (Lee et al. 1997). Second, we demonstrated that these
responses are capable of generating prolonged bursts of action
potentials in the intermediate layer neurons. This result suggests that
one function of intracollicular circuitry may be to generate command bursts. Finally, we recorded the responses of many superficial layer
neurons to the same brief stimuli and found that while most of these
neurons do not produce prolonged responses, a few produce multiple
action potentials and also project to the intermediate layer. Signals
transmitted to the intermediate layer by this subset of visuosensory
neurons may play a direct role in generating the bursts of action
potentials that command saccadic orienting movements of the head and eyes.
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METHODS |
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Forty-one Sprague-Dawley rats were used for this study. All experimental protocols were approved by Duke University Institutional Animal Care and Use Committee Protocol and complied with the guidelines of the Public Health Service policy on Humane Care and Use of Laboratory Animals.
Physiology
The experimental procedures that we used are described in
Lee et al. (1997). Coronal slices were cut from the
superior colliculus (SC) of Sprague-Dawley rats [age, postnatal day
11-19 (P11-P19)] that were anesthetized with pentobarbital sodium.
Slices 300 µm thick were incubated at 37°C for 1 h and then
stored at 25°C on a membrane interface until transfer to the
recording chamber. Whole-cell patch-clamp recordings (Edwards et
al. 1989
) were obtained from individual collicular neurons
using 3-8 M
recording pipettes. The internal solution for the
recording electrodes was composed of (in mM) 130 K-gluconate, 2 NaCl,
20 HEPES (pH 7.3), 4 MgCl2, 4 Na2ATP, 0.4 Na-GTP, 0.5 EGTA, and 0.3-0.5%
biocytin. The liquid-junction potential between the electrode solution
and the bath was calculated to be
10 mV and the membrane potential
measurements presented in the present study were corrected to take this
into account.
The external solution contained (in mM) 123 NaCl, 2.5 KCl, 1 NaH2PO4, 1.3 MgSO4, 26.2 NaHCO3, 11 D-glucose, and 2.5 CaCl2. The drugs bicuculline methiodide (Sigma) and/or 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX) (RBI) were added to this solution as indicated. After each drug application, drug-free solutions were superfused for at least 15 min before new recordings were made. To electrically stimulate the slices, brief current pulses (0.5 ms, 3-100 µA) were applied through an array of eight extracellular thin (~20 µm diam) tungsten wire electrodes (NB Labs, Denison, TX) positioned parallel to the dorsal surface of the superior colliculus within the superficial gray layer (individual wires were placed ~350 µm from each other so that the array was ~2.5 mm wide). Of these eight electrodes, the one that induced the most vigorous responses was used; typically, this electrode was the one closest to the cell body (within 350 µm). The evoked responses were recorded by a Warner PC501A patch clamp amplifier, digitized with an Axon 1200 series Digidata A/D board, acquired at 4-20 KHz, and analyzed with pCLAMP 6 software (Axon Instruments).
Histology
Individual cells were labeled for subsequent morphological
identification by diffusing a 5% biocytin solution into their
cytoplasm from the patch pipette. Slices were then fixed in 4%
paraformaldehyde and processed histologically to reveal the biocytin as
described in Hall and Lee (1997) and Lee and Hall
(1995)
.
In several brains, sections 60 µm thick were cut and stained for
acetylcholinesterase activity to identify unequivocally the borders
between the layers. The sections were soaked overnight in 0.1 M
phosphate buffer at 4°C, rinsed briefly, and then immersed in an
acetylthiocholine solution for 1 h followed by treatment with
sodium sulfide solution for 1 min. The reaction was intensified with
silver nitrate (Billet et al. 1999).
The acetylcholinesterase-stained section shown in Fig.
1 illustrates the nomenclature that we
used for the layers of the superior colliculus in the rat. The stain
demonstrates the well-differentiated superficial and intermediate
layers in the rat and provides an unambiguous basis for relating these
layers in the rat to layers defined by the same criteria in the tree
shrew (Hall and Lee 1997), cat (Graybiel
1978
; Illing 1990
; Illing and Graybiel
1985
), and rhesus monkey (Ma et al. 1991
). In
the rhesus monkey, the intermediate layer defined by the dense band of
cholinergic axons contains a majority of presaccadic cells (Ma
et al. 1991
) whereas in the tree shrew, the similarly defined
layer contains mainly cells, that project to pontine gaze centers via
the predorsal bundle (Hall and Lee 1997
).
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RESULTS |
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The goal of our experiments was to investigate the circuitry
responsible for the prolonged and vigorous bursts of EPSCs that are
generated by intermediate layer neurons in response to a single, brief
electrical stimulus in the superficial layer. Because these bursts had
only been described in the tree shrew (Lee et al. 1997), we first asked whether they also were generated by circuitry found in
slices of the rat superior colliculus.
Responses of intermediate layer neurons
Bursts of EPSCs were recorded from four of the five intermediate
gray layer neurons that responded to electrical stimulation of the
superficial layer. The mean duration of the bursts evoked in these
cells by single-current pulses (10-100 µA) varied from 67 ± 41 to 287 ± 24 ms (mean ± SE). Figure
2 illustrates the functional properties
of the connection between the superficial and intermediate layers. The
dendrites of this cell extended vertically into the overlying optic and
superficial gray layers (Fig. 2A), as was described for some
predorsal bundle cells in the rodent (Rhoades et al.
1987). Thus even though the axon of this cell was not filled with biocytin, the location and morphology of its soma and dendrites were consistent with its identity as a projection neuron.
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This cell responded to the stimulus pulse in the superficial layer with a powerful burst of inward EPSCs that lasted up to 330 ms. The magnitude and duration of the currents varied according to the intensity of the stimulus, with larger stimuli producing more EPSCs (Fig. 2B, top). The synaptic responses evoked by the most intense stimulus (50 µA) were sufficient to generate unclamped action potentials (asterisks in Fig. 2B, top).
To examine the ability of the EPSC bursts to excite the intermediate layer neurons, evoked responses also were recorded under current-clamp conditions. The resultant excitatory postsynaptic potentials (EPSPs) depolarized the intermediate layer cell and, if the stimulus was sufficiently strong (30-50 µA), produced multiple action potentials (Fig. 2B, bottom). In this cell, a 50-µA stimulus evoked bursts of action potentials that lasted up to 200-300 ms (e.g., top of Fig. 2D).
To quantify how these responses varied with the intensity of the
superficial layer stimulus, the EPSC bursts were integrated over time
while the unclamped action potentials were digitally removed to prevent
them from contaminating the integral measurements. The relationship
between stimulus intensity and the amplitude of postsynaptic responses
was sigmoidal and saturated at approximately 30-50 µA (Fig.
2C). This relationship between stimulus intensity and
response magnitude is very similar to that observed in tree shrew
collicular slices (Lee et al. 1997). The fact that
synaptic transmission between the two layers was a graded function of
stimulus intensity indicates that multiple synapses connect the
superficial layer to individual intermediate layer neurons in both
species; presumably this is true in other species as well.
To examine the synaptic process responsible for the intermediate
layer cell responses, the slice was treated with CNQX, a blocker of
AMPA (-amino-3-hydroxy-5-methyl-isoxazole propionic acid)-type
glutamate receptors (Honore et al. 1988
). The EPSPs and
action potentials were completely blocked by bath application of CNQX
(10 µM; Fig. 2D). This result shows that at least one synapse in the circuit activated by superficial layer stimulation is
mediated by glutamate binding to AMPA-type receptors. The observation that CNQX completely blocked the responses of the intermediate layer
cells also demonstrated that none of the activity could be attributed
to direct stimulation of their dendrites.
In summary, brief electrical stimulation of the superficial layer evoked strong postsynaptic responses in intermediate layer cells of rat collicular slices. These synaptic responses consisted of bursts of EPSCs that were caused by activation of multiple glutamatergic synapses and were capable of eliciting prolonged bursts of action potentials. These results are similar to observations in the superior colliculus of tree shrews and permit the use of rat slices to elucidate the circuit mechanisms underlying the generation of the EPSC bursts in the intermediate layer.
Responses of superficial layer neurons
The preceding results show that some mechanism intrinsic to the superior colliculus converts a brief electrical stimulus in the superficial layer into prolonged synaptic excitation of the premotor neurons in the intermediate layer. We next wanted to determine whether neurons in the superficial layer directly provide the synaptic drive for the EPSC bursts. As mentioned in the INTRODUCTION, the EPSC bursts could arise from bursts of action potentials in superficial layer neurons or could be the product of excitatory feedback in the deeper layers of the superior colliculus. The first hypothesis predicts that superficial layer neurons generate prolonged bursts of action potentials whereas the second hypothesis predicts that superficial layer neurons will produce transient responses. To distinguish between these two possibilities, we examined the responses of superficial layer neurons to the same stimulus that produced the EPSC bursts in the intermediate layer neurons.
Responses were detected with whole-cell current clamp recordings from a total of 61 superficial layer neurons (Fig. 3A). Although every cell responded to the stimulus at 10-100 µA intensity, the responses of these cells to even the most intense stimuli varied. Approximately one-third of the superficial layer cells (21/61) did not generate any action potentials in response to superficial layer stimulation but instead produced subthreshold synaptic potentials. Another one-third of the cells (21/61) responded to even the most intense stimuli with a single action potential. The remaining cells (19/61) produced two or more action potentials in response to maximal superficial layer stimulation. By filling the cells with biocytin, we were able to obtain information about the morphology of 23 of the 61 superficial layer cells (Fig. 3B). Two of these cells were identified as horizontal cells, 12 were wide-field vertical cells, and nine were narrow-field vertical cells.
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Among the superficial cells that produced two or more action potentials
in response to the stimulus, the duration of the evoked activity and
the number of action potentials were quite variable as a function of
stimulus intensity. When measured from stimulus onset to the time of
the peak of the last action potential, the response duration ranged
from a few ms to several hundred ms (Fig. 3C). The median
duration of the responses of these cells to maximal stimuli was 18 ms
and the mean was 124 ms. As our morphological results will
demonstrate, some of this variability in response duration can
be accounted for by the presence of several different types of neurons
in this layer (Langer and Lund 1974; Lund and Lund 1972
; Sterling 1971
).
Superficial cells that produced transient responses
As predicted from the hypothesis that recurrent collaterals in the deeper layers are responsible for burst production, several types of superficial layer neurons produced only transient responses to the stimulus.
WIDE-FIELD VERTICAL CELLS.
Wide-field cells in the superficial layer of the superior colliculus
project to the deeper layers and therefore potentially provide
monosynaptic input to the intermediate layer premotor cells (Lee
and Hall 1995; Mooney et al. 1988
). An example
of this type of cell is shown in Fig. 4.
The soma of this cell was located in the lower part of the superficial
gray layer and its dendrites extended vertically and diagonally into
the upper superficial gray and zonal layers (Fig. 4A). The
broad dendritic field of this neuron is characteristic of wide-field
vertical neurons (Lee and Hall 1995
; Mooney et
al. 1988
). Although the axon of the cell in Fig. 4 was not
well-filled, previous studies demonstrated that this cell type projects
extensively to the deeper layers (Lee and Hall 1995
;
Mooney et al. 1988
).
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NARROW-FIELD VERTICAL CELLS.
Narrow-field vertical cells comprise a second type of superficial layer
cell that has extensive projections to the deeper layers (Hall
and Lee 1993; Langer and Lund 1974
; Lee
and Hall 1995
; Mooney et al. 1988
). We recorded
from nine identified narrow-field vertical cells. Similar to the
wide-field cells, most of the narrow-field cells (6/9) generated either
no spikes (n = 2) or only one spike (n = 4) in response to superficial layer stimulation.
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OTHER CELLS. Twenty additional cells that generated either no spikes (n = 17) or only one spike (n = 13) in response to superficial layer stimulation could not be unequivocally identified morphologically either because the area around the cell body was stained with biocytin or because the dendrites and axon were insufficiently filled. Regardless of their type, their brief responses indicate that these cells cannot be directly responsible for the prolonged bursts of EPSCs in the intermediate layer.
Superficial cells that produced multiple action potentials
Nineteen superficial layer neurons produced two or more spikes in response to the stimulus (Fig. 3A). Eleven of these 19 cells were defined morphologically. Such neurons are potential sources for the EPSC bursts in the intermediate layer should belong to this group, so their morphology and the temporal properties of their responses will be described in detail.
HORIZONTAL CELLS.
Two cells that produced prolonged trains of action potentials resembled
the GABAergic horizontal cells that were described in previous studies
(Langer and Lund 1974; Mize et al. 1982
;
Mooney et al. 1988
; Warton et al. 1990
).
A drawing of one of these cells is shown in Fig.
6A. The cell had a dendritic
field that extended in both directions from the cell body, tangential
to the dorsal surface of the superior colliculus, and a small (8-10
µm) cell body that was located within 100 µm of the surface.
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WIDE-FIELD CELLS. Six of 12 wide-field vertical cells produced two or more action potentials in response to the superficial layer stimulus. The duration of the trains of action potentials that we recorded from these six wide-field cells ranged from 35 to 250 ms in response to stimuli of up to 90 µA. A typical example of such cells is shown in Fig. 7A. This cell responded to a 60-µA stimulus with brief bursts of action potentials (Fig. 7B). These spikes began shortly after the stimulus and lasted for up to 50 ms. The response of this wide-field cell consisted of up to five action potentials and the maximum frequency of spikes during the bursts was 167 Hz. Voltage clamp recordings demonstrated that the evoked response included a brief EPSC that peaked within 10 ms and decayed within 50 ms. This EPSC was very large, more than 200 pA, and often was sufficiently powerful to produce unclamped action potentials (Fig. 7C, asterisk).
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NARROW-FIELD VERTICAL CELLS. Three of the nine identified narrow-field vertical cells generated two or more action potentials in response to superficial layer stimulation. Two of these cells showed responses with shorter duration than those of the EPSC bursts in the intermediate layer, whereas one cell in this group generated prolonged trains of action potentials that increased in frequency and duration with the intensity of stimulus. A drawing of this cell is shown in Fig. 8A. The cell was located in the upper part of the superficial layer and gave rise to an axon with multiple terminals in the optic and intermediate layers. Stimuli in the range of 50-80 µA evoked trains of action potentials that lasted an average of 163 ± 23 ms (Fig. 8B). In response to a 100-µA stimulus, this cell produced a burst of 11 action potentials that lasted 626 ms (not shown). Voltage clamp measurements showed that the burst was triggered by a short-latency EPSC with multiple peaks followed by a small outward current (Fig. 8C). The EPSC lasted approximately 20 ms, far shorter than the duration of the action potential burst (Fig. 8B), which suggests that the cell may have had some intrinsic capacity to produce bursts of action potentials in response to brief currents.
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Temporal profiles of the responses in the superficial and intermediate layers
To examine more quantitatively the temporal correlation between activity in superficial layer and intermediate layer neurons, we compared the timing of the EPSC bursts recorded in the intermediate layer with the timing of action potentials generated by the wide- and narrow-field cells of the superficial layer (Fig. 9). For this analysis, the temporal profile of the intermediate layer EPSC bursts was determined by dividing the responses into 10-ms-long bins. We then counted the number of discrete EPSCs that occurred in each time bin for EPSC bursts evoked in the four intermediate layer cells in response to a 50 µA stimulus. The number of EPSCs reached a peak 25 ± 1 ms after the stimulus and then declined over the next several hundred ms (Fig. 9A). For comparison, the temporal pattern of action potential discharge for the 16 wide- and narrow-field vertical cells that responded with at least one action potential to the stimulation of the superficial layer is shown in Fig. 9B. The one narrow-field cell that generated prolonged trains of action potentials (Fig. 9D) is excluded from this sample of wide- and narrow-field cells to distinguish more clearly between the temporal response patterns of the different subgroups of superficial gray layer cells. In Fig. 9B, the number of action potentials that occurred within 10-ms-long time bins was determined for each neuron. The latency for each spike is defined as the time between the onset of the stimulus and the peak of the individual action potential. Thus a few neurons with higher numbers of action potentials had responses with latencies as late as 700 ms.
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Given that both wide- and narrow-field cell types project to the intermediate layer, Fig. 9B provides our best estimate of the temporal distribution of the action potentials that are transmitted from the superficial layer to an intermediate layer cell in response to a brief stimulus in the superficial layer. The number of action potentials peaks 5.4 ± 0.3 ms after the stimulus, reflecting our observation that 8/17 wide- and narrow-field cells generated only one action potential and that this response occurred with a short latency following the stimulus. Afterwards, the frequency of action potentials decreased rapidly because only 9/17 cells generated multiple action potentials in response to the stimulus. For comparison, the temporal pattern of discharge for only those narrow- and wide-field cells that generated two or more action potentials (n = 9) in response to the brief stimulus is illustrated in Fig. 9C. These cells are the best candidates in the superficial layer for the source of the intermediate layer EPSC bursts because they generate multiple action potentials in response to a brief stimulus. The temporal profile of this group resembles the pattern of discharge for the one narrow-field cell that generated trains of action potentials that were several millisecond long (Fig. 9D). The cell illustrated in Fig. 9D had an activity peak at 5.4 ± 0.6 ms shortly before the onset of the intermediate layer EPSC bursts; its activity then continued for several hundred milliseconds. Thus the most salient difference between the temporal patterns in Figs. 9A and 9B is the more rapid decline in the overall activity of the superficial layer neurons plotted in Fig. 9B. The population of narrow- and wide-field cells that generated two or more action potentials (n = 9) has a temporal profile that resembles the temporal pattern of EPSC bursts in the intermediate layer, but the more gradual decline in the activity of these cells appears to be largely, but not entirely, due to the contribution of the single narrow-field cell illustrated in Fig. 9D. The narrow-field cell in Fig. 9D exhibited a temporal profile of action potentials that closely resembled the timing of the responses in the intermediate layer and thus, of all the cells in our sample, can most adequately account for the prolonged bursts of EPSCs.
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DISCUSSION |
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Bursts of action potentials that are generated by premotor cells
in the intermediate gray layer in vivo comprise the command signal for
orienting movements of the head and eyes (Goldberg and Wurtz
1972; Munoz and Guitton 1986
; Munoz et
al. 1991
; Sparks 1978
; Sparks and Nelson
1987
; Wurtz and Goldberg 1972
; Wurtz and Mohler 1976
). In the tree shrew slice preparation (Lee
et al. 1997
), and now in rat collicular slices, we found that
the application of a single current pulse, 0.5 ms in duration, to the
superficial layer can produce a prolonged burst of EPSCs in
intermediate layer cells. In the present experiments we also found
that, even in a slice preparation, these EPSCs are capable of producing
prolonged bursts of action potentials in intermediate layer neurons.
These prolonged responses indicate that circuitry within the colliculus is capable of amplifying and prolonging responses triggered by transient inputs. Thus the results suggest that one function of the
intrinsic circuitry of the superior colliculus may be to generate the
prolonged bursts that command orienting movements in vivo. The results
also suggest that this circuitry is preserved in collicular slices,
making possible the detailed patch clamp analysis of its mechanisms.
Our experiments demonstrated that the same current pulses that, when
delivered to the superficial layer, generate the prolonged bursts in
the intermediate layer neurons also evoke a variety of responses in the
superficial layer cells. The majority of superficial cells responded
with subthreshold postsynaptic currents or only one action potential,
regardless of the intensity of the stimulus. However, a smaller subset
of superficial neurons (19/61) produced two or more action potentials.
Since nine of these neurons are types known to project to the
intermediate layer, they are potential sources of direct, monosynaptic
inputs that could contribute to the EPSC bursts in the intermediate
layer cells. However, all but one of these cells exhibited responses
that were shorter than the duration of the intermediate layer bursts.
Thus the results suggest that while the superficial layer may be
included in the circuitry that enhances and prolongs transient inputs
to generate EPSC bursts, other sources, such as the recurrent circuitry
within the deeper layers (Pettit et al. 1999), may also
play an important role.
The use of rat superior colliculus for in vitro studies
The decision to use rats for these experiments was initially based
on previous studies that demonstrated that the laminar organization of
the superior colliculus is similar in most mammals. In support of these
studies, we illustrated the superficial and intermediate layers in the
rat with an acetylcholinesterase-stained section (Fig. 1). The section
shows the distinct differentiation of these layers in the rat and also
provides a basis for relating them to the layers defined by the same
criteria in the cat (Graybiel 1978; Illing and
Graybiel 1985
), tree shrew (Hall and Lee 1997
), and rhesus monkey (Ma et al. 1991
). Further evidence for
a similar laminar organization across species was provided by studies
that demonstrated projections from the superficial to the intermediate layer in species as diverse as the tree shrew (Hall and Lee
1997
; Lee and Hall 1995
), hamster (Mooney
et al. 1988
), and squirrel monkey (Moschovakis et al.
1988
). Finally, our experiments provided evidence for a strong
functional connection between these layers by demonstrating that, as in
the tree shrew (Lee et al. 1997
), stimulation of the
superficial gray layer in the rat evokes powerful synaptic responses in
intermediate layer cells (Fig. 2).
Rats between the ages of P11 and P19 were used because it is more
practical to obtain patch clamp recordings in slices from young animals
(Aitken et al. 1995; Lipton et al. 1995
;
Plant et al. 1995
). However, the use of young animals
raises the question of whether our observations also apply to adults.
Several lines of evidence support the argument that circuits with
properties similar to those we described in young animals are present
in adults. First, both the morphologies and the interlaminar
projections of the cells that we filled with biocytin are very similar
to those in adults (Hall and Lee 1993
; Langer and
Lund 1974
; Lee and Hall 1995
; Lund and
Lund 1972
; Mooney et al. 1988
). Second, glutamatergic receptor activity changes from immature to adult levels
by the time that eyes are opened (~P11-P14) (Shi et al. 1997
). Third, while there are suggestions that the development of collicular GABAergic pathways may be incomplete at this age (Grantyn et al. 1984
; Lund and Lund 1972
;
Mize 1992
; Mize et al. 1982
; Shi
et al. 1997
; Warton and McCart 1989
;
Warton et al. 1990
), our whole-cell recordings provide
unequivocal evidence of strong bicuculline-sensitive inhibition at the
ages used in our experiments. Specifically, in recordings from seven
cells in animals with age ranges from P11 to P17, large outward
currents that could be blocked with bicuculline were revealed in the
presence of CNQX, and the application of bicuculline strongly enhanced
the excitatory responses of these cells in the absence of CNQX.
Moreover, for those cells that fired two or more action potentials,
neither the number of action potentials nor their frequency showed any
dependence upon the age of the animal. Finally, the phasic responses
that predominate in the superficial layer of young rat slices are also
characteristic of superficial cells in vivo in the adult
(Goldberg and Wurtz 1972
; Sefton 1969
).
In the slices, these phasic responses appeared to be mediated, at least
in part, by intracollicular inhibition because treatment of the slices
with bicuculline both amplified the inward currents of the superficial
cells and converted their responses from one or two action potentials
to prolonged bursts (Fig. 4E). Thus it is likely that our
observations describe mechanisms that operate in the superior
colliculus of adult rats and other species.
The relationship between activity in the superficial and deep layers
The goal of our work was to understand the circuitry responsible
for the EPSC bursts that occur in intermediate layer neurons following
stimulation of the superficial layer (Lee et al. 1997). The two hypotheses that we considered predicted that superficial layer
neurons would respond to brief stimulation with either transient or
prolonged responses. In fact, we observed both types of responses. While most superficial layer cells responded phasically to the stimulus, 19 of 61 cells produced multiple action potentials, which
could account for the generation of the EPSC bursts in the intermediate
layer. Two of the superficial cells that exhibited prolonged and
high-frequency trains of action potentials were horizontal cells and
eight of them were morphologically unidentified cells. Since evidence
from previous studies indicates that horizontal cells are GABAergic
neurons that do not project to the intermediate layer (Langer
and Lund 1974
; Sterling 1971
; Warton et
al. 1990
), they are unlikely to contribute directly to the EPSC
bursts. Instead, they may contribute to the trains of outward currents
that we recorded from superficial cells in the presence of CNQX (Figs. 4 and 5). The unidentified cells may contribute to the EPSC bursts either directly or indirectly depending on their type.
In contrast, both wide- and narrow-field cells project to the
underlying layers (Figs. 7A and 8A) (Lee
and Hall 1995; Mooney et al. 1988
) and are in a
position to make monosynaptic contacts with intermediate cells that
generate the bursts. Comparison of the temporal profiles of the EPSC
bursts with the temporal distribution of the evoked responses of the
wide- and narrow-field cells (Fig. 9) provides some support for both
hypotheses about the synaptic relationships between the superficial and
intermediate layers.
Our observation of a superficial layer neuron that produced prolonged responses that tracked the time course of EPSC bursts (Fig. 9D) indicates that the superficial layer is capable of generating prolonged activity, which is consistent with the hypothesis that such activity produces the EPSC bursts. However, because the majority of the cells produced either subthreshold responses, only one action potential, or bursts of two or more action potentials of shorter duration than the duration of EPSC bursts in the intermediate layer, if this hypothesis is correct then superficial cells with prolonged responses must make a disproportionately large contribution to synaptic excitation of the premotor neurons. The relative contribution of each cell type will depend not only on the proportion of each type in the superficial layer but also on the number of action potentials produced by each cell and the strength of the synaptic connections between these cells and the premotor neurons.
Alternatively, the observation that the responses of most superficial
layer neurons decline more rapidly than do the EPSC bursts in the
intermediate layer implies that their output must be further amplified
by circuitry in the deeper layers, in the optic layer, or, more likely,
by recurrent excitation in the intermediate layer (Arai et al.
1994; Pettit et al. 1999
). The same circuitry also may amplify signals that reach the intermediate layer from other
sources such as the frontal eye fields (Schlag-Rey et al. 1992
) and the auditory and somatosensory systems (Sparks
and Nelson 1987
).
A model of superficial layer connectivity
Although our experiments were not designed to determine intrinsic
synaptic connections, the responses generated by the various collicular
cell types suggest a minimal model for the intrinsic circuitry of the
superficial layer (Fig. 10). The
horizontal cells from which we recorded are representative of a
population of inhibitory interneurons that may contact wide- and
narrow-field cells, and also each other, through dendrodendritic
synapses (Langer and Lund 1974; Sterling
1971
; Warton et al. 1990
). The proposed contacts of horizontal cells with narrow- and wide-field cells could account for
the complex outward currents observed in the latter cell types in the
presence of CNQX and could contribute to the transient nature of their
responses in normal conditions. The output signals of the superficial
layer are transmitted to the intermediate layer by axons of the wide-
and narrow-field cells (Isa et al. 1998
; Lee et
al. 1997
). According to the model, a small subset of these projecting cells may have relatively little input from local inhibitory neurons and may be able, perhaps through local recurrent circuitry, to
generate high-frequency and prolonged trains of action potentials. These trains of spikes may combine with the excitatory local circuitry within the intermediate layer (Pettit et al. 1999
) to
generate the bursts of action potentials that command saccades. Future experiments could use in vitro methods to test these ideas by directly
measuring the influence of individual superficial cells on intermediate
cells.
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ACKNOWLEDGMENTS |
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We thank M. Helms and P. Lee for helpful comments during the course of the work and Dr. M. Schmidt, J. Laughlin, and M. Riddle for comments on the manuscript. We especially thank Dr. N. Cant for assistance with the acetylcholinesterase histochemistry and photomicroscopy.
This work was supported by National Institutes of Health Grants EY-08233 and NS-34045 and a Fogarty International Research Fellowship to G. Özen.
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FOOTNOTES |
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Address for reprint requests: G. Özen, Dept. of Neurobiology, Duke University Medical Center, Box 3209, Durham, NC 27710 (E-mail: ozeng{at}neuro.duke.edu).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
Received 5 January 2000; accepted in final form 2 April 2000.
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REFERENCES |
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