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The Journal of Neuroscience, April 15, 2001, 21(8):2699-2710
Diverse Types of Interneurons Generate Thalamus-Evoked
Feedforward Inhibition in the Mouse Barrel Cortex
James T.
Porter1,
Cary
K.
Johnson1, and
Ariel
Agmon1, 2
Department of 1 Neurobiology and Anatomy and
2 the Sensory Neuroscience Research Center, West Virginia
University, Morgantown, West Virginia 26506-9128
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ABSTRACT |
Sensory information, relayed through the thalamus, arrives in the
neocortex as excitatory input, but rapidly induces strong disynaptic
inhibition that constrains the cortical flow of excitation both
spatially and temporally. This feedforward inhibition is generated by
intracortical interneurons whose precise identity and properties were
not known. To characterize interneurons generating feedforward
inhibition, neurons in layers IV and V of mouse somatosensory ("barrel") cortex in vitro were tested in the
cell-attached configuration for thalamocortically induced firing and in
the whole-cell mode for synaptic responses. Identification as
inhibitory or excitatory neurons was based on intrinsic firing patterns
and on morphology revealed by intracellular staining. Thalamocortical
stimulation evoked action potentials in ~60% of inhibitory
interneurons but in <5% of excitatory neurons. The inhibitory
interneurons that fired received fivefold larger thalamocortical inputs
compared with nonfiring inhibitory or excitatory neurons.
Thalamocortically evoked spikes in inhibitory interneurons followed at
short latency the onset of excitatory monosynaptic responses in the
same cells and slightly preceded the onset of inhibitory responses in
nearby neurons, indicating their involvement in disynaptic inhibition. Both nonadapting (fast-spiking) and adapting (regular-spiking) inhibitory interneurons fired on thalamocortical stimulation, as did
interneurons expressing parvalbumin, calbindin, or neither calcium-binding protein. Morphological analysis revealed that some
interneurons might generate feedforward inhibition within their own
layer IV barrel, whereas others may convey inhibition to upper layers,
within their own or in adjacent columns. We conclude that feedforward
inhibition is generated by diverse classes of interneurons, possibly
serving different roles in the processing of incoming sensory information.
Key words:
feedforward inhibition; thalamocortical; somatosensory
cortex; barrel cortex; mice; parvalbumin; calbindin; FS cells; RSNP
cells; spiny stellate cells; GABAergic interneurons
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INTRODUCTION |
The mammalian neocortex is a densely
interconnected neuronal network in which sensory information relayed
via the thalamus is processed and transformed into conscious sensory
perception, to be acted on or stored in memory, as needed. Although the
thalamocortical input to the neocortex is purely excitatory
(glutamatergic), as determined by electrophysiological, electron
microscopic, and immunocytochemical evidence (White, 1978 ; Ferster and
Lindstrom, 1983; Agmon and Connors, 1992; Kharazia and Weinberg, 1993),
inhibitory (GABAergic) mechanisms are recruited from the very first
stage of intracortical processing. Indeed, electrical stimulation of thalamocortical afferents in vivo (Ferster and Lindstrom,
1983; Swadlow, 1989, 1990) or in vitro (Agmon and Connors,
1992; Gil and Amitai, 1996), as well as controlled sensory stimulation
(Simons and Carvell, 1989; Simons, 1995; Brumberg et al., 1996; Swadlow et al., 1998; Zhu and Connors, 1999), result in a brief excitation of
neocortical neurons, immediately followed by a pronounced inhibitory response mediated by intracortical inhibitory interneurons. The short
latency of the inhibitory response indicates that the inhibitory interneurons eliciting it must be excited directly by the
thalamocortical afferents, consistent with anatomical data (White,
1978; Fairén and Valverde, 1979; Freund et al., 1985; Keller and
White, 1987), and in turn inhibit other cortical neurons
disynaptically. This feedforward inhibition is a highly robust feature
that can be engaged by even a single thalamocortical action potential
(Swadlow and Gusev, 2000), can influence the spread of
thalamocortically evoked excitation, and can shape the cortical
representation of the sensory environment (Sillito, 1975; Tsumoto et
al., 1979; Sillito et al., 1980; Hicks and Dykes, 1983; Dykes et al.,
1984; Kyriazi et al., 1996; Kyriazi et al., 1998).
Intracortical inhibitory neurons are a diverse population (Cauli et
al., 1997; Kawaguchi and Kubota, 1997; Gupta et al., 2000). Although
they all use GABA as a neurotransmitter and have a nonpyramidal morphology with nonspiny or sparsely spiny dendrites, they vary considerably in other properties that may determine their effect on
their postsynaptic targets. Different subpopulations of GABAergic interneurons contact postsynaptic neurons on different parts of their
membrane (Somogyi, 1977; Jones and Hendry, 1984; Kawaguchi and Kubota,
1997; Tamas et al., 1997a), express different palettes of ionic
channels resulting in different firing patterns (Cauli et al., 1997;
Kawaguchi and Kubota, 1997; Porter et al., 1999), form synapses with
very different temporal dynamics (Thomson et al., 1996; Reyes et al.,
1998; Gupta et al., 2000), and exhibit different "spheres of
influence", as reflected in the laminar and horizontal spread of
their axonal arbors (Xiang et al., 1998). Our goal was to identify
which of these diverse subpopulations were involved in mediating
feedforward thalamocortical inhibition. To do so, we tested inhibitory
interneurons of the mouse barrel cortex for firing in response to
thalamocortical stimulation in vitro, recorded their
synaptic inputs and intrinsic firing patterns, characterized their
cytochemical markers, and traced their dendritic and axonal
morphologies. Our results indicate that thalamocortical feedforward
inhibition is not the product of one specific subpopulation of
interneurons, but rather the concerted effect of several distinct electrophysiological, cytochemical, and morphological classes.
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MATERIALS AND METHODS |
Preparation of thalamocortical brain slices. The
procedure for preparing thalamocortical slices was modified from Agmon
and Connors (1991). ICR white mice (postnatal days 9-18;
Hilltop Lab Animals, Scottdale, PA) were anesthetized with
methoxyflurane (Metofane; Mallinckrodt Veterinary, Mandelein, IL),
decapitated, and their brains were removed into ice-cold artificial
CSF (ACSF). The brain was dissected along the midline, and each
hemisphere was placed with the midsagittal plane down on a circular
glass coverslip, with the anterior pole pointing forward ("north"). The coverslip was then placed on a homemade sectioning platform, rotated horizontally 10° to the right if the right hemisphere or to
the left if the left hemisphere, and a cut was made at approximately one-third the distance from the anterior to the posterior pole, using a
razor blade with its edge parallel to the east-west line and slanted
35° northward. The razor blade was supported on a semicircular metal
frame that could be rotated around the east-west axis, and both the
10° and the 35° angles were set using graduated circles printed on
acetate film, cut out, and pasted to the sectioning platform in the
horizontal and vertical (north-south) planes, respectively. This
modification of the original method allowed preparation of
thalamocortical slices from both hemispheres. The resultant block of
tissue was glued with the anterior cut surface down onto a Vibroslicer
stage (WPI, Sarasota, FL), and 300- to 500-µm-thick slices were cut
and examined by transillumination under a stereomicroscope. Slices
containing both the ventrobasal thalamic complex (VB) and the barrel
cortex were saved and incubated for 1 hr at room temperature in ACSF
containing (in mM): 126 NaCl, 3 KCl, 1.25 NaH2PO4, 2.5 CaCl2, 1.3 MgSO4, 26 NaHCO3, and 20 glucose, bubbled with carbogen
(95% O2 and 5% CO2).
Extracellular recording and stimulation. Individual slices
were transferred to a submersion recording chamber (Dagan Corporation, Minneapolis, MN) mounted on an Olympus BX50 upright microscope, and
perfused with room temperature, carbogenated ACSF at a rate of 2-3
ml/min. The slices were placed with their anterior surface up, because
intact thalamocortical axons are more likely to be near the anterior
surface (Agmon et al., 1993). Bright-field illumination revealed the
basic anatomical landmarks of the thalamocortical pathway, including
individual layer IV barrels (Fig.
1A,B). To stimulate
thalamocortical axons, a unipolar tungsten microelectrode (AM Systems,
Carlsborg, WA) was placed in the VB or at the border of the VB and the
reticular nucleus (RTN) (Fig. 1A), and 0.1 msec cathodal current pulses of increasing intensity were elicited every
10-30 sec using a Master-8 pulse generator and stimulus isolation unit
(AMPI, Jerusalem, Israel). Field potentials were recorded with glass
micropipettes (1 mm outer diameter, 0.58 mm inner diameter; AM Systems)
that were pulled on a Flaming-Brown pipette puller (Sutter
Instruments, Novato, CA), slightly broken under a microscope, filled
with 0.9% NaCl, and placed within a barrel "hollow" in layer IV
(Fig. 1B). Field potentials were amplified 1000×
(Intronix Technologies, Bolton, Ontario, Canada), low-pass-filtered at
1 kHz, and digitized at 2.5 kHz. The positions of the stimulating and
recording micropipettes were adjusted to maximize the amplitude of the
evoked field potential.
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Figure 1.
Experimental setup. A, A
low-magnification image of a fixed thalamocortical slice, illustrating
typical placement of the stimulation microelectrode near the VB
complex-RTN border in the thalamus. The rectangular frame
delineates the region of barrel cortex most likely to receive
thalamocortical inputs in the slice (the dark blotches
within this rectangle are three biocytin-filled inhibitory
interneurons that fired in response to thalamocortical
stimulation). B, The barrel cortex in a live
thalamocortical slice, as visualized during the experiment by
bright-field illumination. A field potential micropipette is inserted
in a layer IV barrel (note the three barrels visible to the
right of the micropipette tip). C, A
high-power microscopic field from a layer IV barrel, as visualized
during the experiment under DIC optics, showing a patch pipette
(emphasized by the overlay) during a cell-attached and whole-cell
recording from an inhibitory interneuron.
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Cell-attached and whole-cell recording. Single neurons were
visualized by infrared video-enhanced microscopy with differential interference contrast (DIC) optics (Stuart et al., 1993), using a
Dage-MTI (San Diego, CA) CCD camera. To maximize the likelihood of
recording from inhibitory interneurons, we targeted neurons with large,
nonpyramidal appearing cell bodies (Simons and Woolsey, 1984; Lin et
al., 1985) (Fig. 1C). Cell-attached and whole-cell recordings in current-clamp and voltage-clamp modes were performed with
a patch-clamp amplifier (Axopatch 200A; Axon Instruments, Foster City,
CA). Patch pipettes (3-5 M ), pulled from high-lead content glass
capillaries (Corning #0010 glass; WPI), were filled with an internal
solution containing (in mM): 136 K methylsulfate, 2 MgCl2, 0.6 EGTA, and 10 HEPES, pH 7.2, 285-295
mOsm, for current-clamp experiments, or with: 122 Cs gluconate, 2 MgSO4, 0.6 EGTA, 10 HEPES, 0.1 Spermine, and 10 QX-314, pH 7.2, 285-295 mOsm, for voltage-clamp experiments in which
the synaptic responses were recorded at depolarized potentials. Current
or voltage pulse protocols were generated with the Master-8 pulse
generator. After achieving a cell-attached configuration, the
thalamocortical fibers were stimulated with increasing intensity, until
spikes were evoked or up to a maximum of 200 µA. (The 200 µA cap on
the intensity of the stimulation was chosen because pilot experiments
indicated that further increase in stimulus intensity was unlikely to
increase the probability of firing; the majority (62%,
n = 60) of discharging cells fired at an intensity
 120 µA.) The seal was then ruptured, and a whole-cell configuration
was established. Resting membrane potential was measured just after
achieving the whole-cell configuration, and only cells with a resting
membrane potential more negative than  50 mV were analyzed. The
intrinsic firing pattern of the neurons was tested by applying
depolarizing current steps in the current-clamp mode. In some neurons,
recorded with the Cs-gluconate-based pipette solution, thalamocortical
synaptic currents were recorded while varying the holding potential in
the voltage-clamp mode. Voltage or current records were low-pass
filtered at 2-5 kHz, digitized at 10-20 kHz, saved to disk, and
analyzed off-line. Data acquisition and processing was done with
software written by A. Agmon in LabView (National Instruments,
Austin, TX). All membrane potential values were corrected for a
junction potential of 11 mV (Agmon et al., 1996).
Data analysis. The action potentials elicited by current
steps were analyzed with MiniAnalysis (Synaptosoft, Leonia, NJ) to determine the threshold for action potential initiation and the amplitude of the afterhyperpolarizing potential (AHP). The action potential threshold was determined as the point at which the second derivative of the voltage trace was zero. The AHP amplitude was defined
as the minimum point relative to threshold after the decay phase of the
action potential. The spike frequency adaptation ratio was defined as
the ratio of the first interspike interval divided by the average of
the last three interspike intervals during a 500- to 800-msec-long
spike train. Input resistance was calculated from the voltage response
induced by a 500-800 msec hyperpolarizing current pulse.
Morphological identification. For morphological
characterization of individual neurons, 1-2 mg/ml biocytin (Sigma, St.
Louis, MO) was included in the intracellular solutions. After fixing overnight with 4% paraformaldehyde, rinsing with PBS, and
permeabilizing with 0.25% Triton X-100, the slices were incubated for
3 hr with ABC solution (Vector Laboratories, Burlingame, CA). After
five rinses in PBS, the slices were preincubated with 0.7 mg/ml of 3'3'-diaminobenzidine (DAB; Sigma) for 15 min, and then the reaction was initiated by adding 0.3%
H2O2. The reaction was
stopped by rinsing with ice-cold PBS, and the slices were mounted in
PBS-glycerol, coverslipped, and sealed with nail polish. Stained
neurons were visualized on an Olympus AX microscope with a 60×, NA
1.2, long working-distance water-immersion objective or a 100×, NA
1.4, oil immersion objective, traced and digitally reconstructed with Neurolucida (MicroBrightField, Colchester, VT). Digital images were
taken using a Magnafire CCD camera (Optronics, Goleta, CA).
Identification of interneurons expressing parvalbumin and
calbindin-28K. After fixing overnight with 4% paraformaldehyde, the slices were washed three times with Tris buffer and incubated for 1 hr in 0.25% Triton X-100 in Tris buffer and 5% normal horse serum
(NHS). Slices were then incubated for 3 d at 4°C with a 1:500
dilution of mouse anti-parvalbumin (PV) monoclonal antibody (P-3171; Sigma) and/or a 1:500 dilution of rabbit anti-calbindin-28K (CB) polyclonal antibody (AB1778; Chemicon, Temecula, CA) in
0.25% Triton X-100 in Tris buffer with 1% NHS. Next, slices were
washed three times with Tris buffer and incubated 3 d in a 1:500
dilution of allophycocyanin-conjugated goat anti-mouse IgG antibody
(Molecular Probes, Eugene, OR) to label the PV-expressing cells, and in
a 1:1000 dilution of Alexa 546-conjugated goat anti-rabbit IgG
(Molecular Probes) to label the CB-expressing cells, in 0.25% Triton
X-100 in Tris buffer with 1% NHS. Slices were then washed with Tris buffer, mounted in PBS-glycerol, coverslipped, and sealed with nail
polish. Images of the fluorescently labeled cells were obtained using a
Zeiss LSM510 confocal microscope. The PV- and CB-expressing cells were
visualized with the 633 nm red HeNe laser excitation line (650 nm
emission filter) and with the 543 nm green HeNe laser excitation line
(560-615 nm emission filter), respectively. To identify the recorded
neurons on the confocal microscope, Lucifer yellow (potassium salt, 1 mg/ml; Sigma) was included in the patch pipette in addition to
biocytin, and the Lucifer yellow fluorescence was visualized using the
488 nm line of the Argon laser. Alternatively, slices were incubated
with a 1 µg/ml solution of fluorescein
isothiocyanate-conjugated streptavidin (Molecular Probes) for 30 min after completing the incubation with the secondary antibody and
then visualized with the 488 nm laser line (530-585 nm emission
filter). After immunocytochemical characterization, a DAB reaction was
performed as described above (under "Morphological
identification"), starting with the five rinses with PBS.
Statistical tests. To determine statistical
significance of difference between means, the observed difference was
compared to differences calculated from 10,000 random permutations of
the labels (Good, 1999). Permutation tests were programmed in Mathcad (Mathsoft, Cambridge, MA).
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RESULTS |
Distinguishing inhibitory from excitatory neurons
To characterize the neocortical interneurons that mediate
feedforward inhibition, neurons in layers IV and V of the mouse somatosensory (barrel) cortex were tested in the cell-attached configuration, which does not disrupt the ionic and electrical integrity of the neurons, for action potential firing in response to
thalamocortical stimulation. Their intrinsic firing patterns and
thalamocortical synaptic responses were subsequently recorded in the
whole-cell configuration. Recordings were made from a total of 135 neurons sampled from 67 slices prepared from 48 juvenile mice, 9- to
18-d-old. The basic experimental setup is shown in Figure 1. Inclusion
of biocytin in the pipette allowed the recorded neurons to be
morphologically identified post hoc as either inhibitory or
excitatory neurons: excitatory cortical neurons have either pyramidal
or spiny stellate morphologies, whereas inhibitory interneurons exhibit
nonpyramidal, aspiny, or sparsely spiny morphologies (Simons and
Woolsey, 1984; Peters and Kara, 1985a,b). Because not all of our
neurons were recovered morphologically, the intrinsic firing patterns
of the recorded cells were also used to distinguish inhibitory from
excitatory neurons. As previously described (McCormick et al., 1985),
pyramidal neurons encountered in this study showed strongly adapting
responses to depolarizing current pulses. Typically, the first two or
three spikes in a train occurred at much shorter interspike intervals
than the rest of the spike train (data not shown). The firing patterns
of the neurons that we identified morphologically as spiny stellate
cells were also examined. As shown in Figure
2A, left,
spiny stellate cells were multipolar, with several fine dendrites
radiating out from the soma. When observed at high magnification, their
dendrites exhibited numerous spines (short arrows).
Injection of depolarizing current pulses (Fig. 2A,
right) induced the firing of action potentials that, as in
pyramidal neurons, showed strong frequency adaptation. In addition, the
AHP at the end of each action potential (arrowhead) was
small and repolarized slowly. In contrast, neurons identified morphologically as inhibitory interneurons, i.e., neurons that were
neither pyramidal nor spiny stellates in morphology (Fig. 2B, left), exhibited much less spike frequency
adaptation during induced trains of action potentials (Fig.
2B, right) and AHPs that were generally larger and
repolarized faster (arrowhead). These differences are
quantified and plotted in Figure 2C, in which only neurons
with a positive morphological identification are included. Because
there was virtually no overlap between spike train parameters of
morphologically identified excitatory and inhibitory neurons, the
intrinsic firing patterns were used to distinguish inhibitory from
excitatory neurons in those cases in which morphological identification
was not possible. In total, our sample of whole-cell recordings
included 19 pyramidal neurons, 11 spiny stellate cells, and 105 inhibitory interneurons.
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Figure 2.
Morphologically identified excitatory and
inhibitory neurons exhibit distinct firing patterns. A,
B, Images of representative neurons labeled with
biocytin and their corresponding voltage responses to hyperpolarizing
and depolarizing current steps (arrows).
A, A spiny stellate cell. Note the extremely thin and
spine-bearing dendrites and the profoundly adapting spikes with shallow
rounded AHPs (arrowhead). B, An
inhibitory interneuron. Note the relatively thick, aspiny dendrites and
that the action potentials exhibit less adaptation and deeper, shorter
AHPs (arrowhead). Scale bar: A, 30 µm;
B, 50 µm. Pial surface is up.
C, Separation of morphologically identified inhibitory
interneurons (n = 56), pyramidal cells
(n = 5), and spiny stellate cells
(n = 7) according to their AHP peak amplitudes and
spike frequency adaptation ratios (see Materials and Methods). Note
that with one exception in each case, all neurons with an AHP amplitude
>10 mV were morphologically identified as inhibitory interneurons,
whereas all neurons with AHP amplitude <10 mV were morphologically
identified as excitatory (pyramidal or spiny stellate). There was also
very little overlap in adaptation ratios.
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Spikes in inhibitory interneurons are appropriately timed to
mediate disynaptic inhibition
To mediate feedforward, disynaptic inhibition, interneurons should
fire at a monosynaptic latency after a thalamocortical volley, and
their action potentials should evoke inhibitory responses in
surrounding neurons. As shown in Figure
3, inhibitory interneurons indeed
discharged in a manner consistent with this expectation. The left
vertical guideline in this figure indicates the onset of the
thalamocortically evoked field potential (Fig. 3A), which is
a good indicator for the onset of the monosynaptic excitatory postsynaptic response in the layer IV population (Agmon and Connors, 1991, 1992). A spiny stellate neuron in the barrel did not discharge spikes in the cell-attached (CA) mode of recording (Fig. 3B, top trace), but when recorded in the whole-cell voltage-clamp (WC) mode (Fig. 3B, middle and bottom traces), it was
found to receive an EPSC coincident with the monosynaptic field
potential (left guideline). This monosynaptic EPSC was
immediately followed by an IPSC, the onset of which is indicated by the
right vertical guideline. The inhibitory nature of this second response
is evident from the record at a depolarized potential, which shows that
at 35 mV the current was already outward, indicating an inhibitory reversal potential. The IPSC began 3.0 msec after the onset of the
EPSC, a latency that leaves time for one intercalated inhibitory neuron
to fire.
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Figure 3.
Interneuronal spikes are appropriately timed to
mediate disynaptic inhibition. All traces were recorded from the same
barrel column and are aligned on the stimulus onset. A,
Averaged thalamocortically evoked field potential (FP)
recorded in layer IV. The arrowhead indicates the
stimulus onset; the left vertical guideline indicates
the onset of the field EPSP. B, A spiny stellate cell.
Top panel, Four superimposed cell-attached responses
(CA) with no detectable spikes; bottom
panels, averaged whole-cell responses (WC) with
holding potentials indicated above each trace. This cell received a
monosynaptic EPSC (onset coincident with field EPSP, left
guideline; note that the postsynaptic current is inward at both
holding potentials) followed by a disynaptic IPSC (onset indicated by
the right guideline; note that the postsynaptic current
reverses between 82 and 35 mV). C, An inhibitory
interneuron. Top panel, Four superimposed cell-attached
responses; note that the cell fired consistently. Bottom
panels, Four or five superimposed whole-cell responses. This
cell received a monosynaptic EPSC slightly before the EPSC in the spiny
stellate cell (left guideline), followed by a dual IPSC,
the early IPSC indicated by the arrow, and the late IPSC
coincident with the IPSC in the spiny stellate cell (right
guideline). Vertical calibrations apply, from
top to bottom, to A,
B, and C, respectively. D,
Biocytin staining of the two neurons illustrating their relative
locations in the same barrel column. E, Cumulative
probabilities of the latencies of EPSCs and spikes in 59 barrel
interneurons and of IPSCs in 17 excitatory neurons, in response to
thalamocortical stimulation. Latencies were measured from the beginning
of the field EPSP. F, The fraction of pyramidal
(P; n = 19), spiny stellate
(SS; n = 11), and inhibitory
(II; n = 105) neurons that fired
(filled bars) or did not fire (open
bars) in response to thalamic stimulation.
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The inhibitory interneuron recorded in the same barrel (Fig. 3D,
bottom cell) could have been such an intercalated neuron. Examination of this neuron in the whole-cell voltage-clamp mode (Fig.
3C, middle and bottom traces) indicated that it
received a thalamocortical input nearly coincident with the
monosynaptic field potential. This coincidence, and the negligible
sweep-to-sweep variability in the onset of the whole-cell responses
(note superimposed traces), indicate that these were monosynaptic EPSCs
(Agmon and Connors, 1992; Agmon et al., 1996). This neuron discharged a
single spike (Fig. 3C, top trace) with an average latency of
1.8 msec after the onset of the monosynaptic EPSC (left
guideline) and 1.2 msec before the onset of the disynaptic IPSC in
the spiny stellate cell (right guideline). Analysis of the
latencies from the onset of the postsynaptic component of the field
potential to all the monosynaptic EPSCs and spikes in 59 inhibitory
interneurons, and to the IPSCs in 17 excitatory neurons (Fig.
3E), indicated that, as a population, the spikes followed
the monosynaptic EPSCs in the inhibitory interneurons by 1.9 msec and
preceded the IPSCs in the excitatory neurons by 1.3 msec
(median-to-median intervals), as expected if these spikes were
mediating disynaptic inhibition.
Inhibitory interneurons receive feedforward inhibition
Similar to the inhibitory interneuron shown in Figure 3, all but
three of the 59 inhibitory interneurons that discharged spikes in
response to thalamocortical stimulation fired single action potentials.
This was somewhat surprising, because inhibitory cortical neurons are
capable of firing trains of action potentials at high frequency when
activated by synaptic inputs in vitro (McCormick et al.,
1985; Agmon and Connors, 1992) or in vivo (Swadlow, 1989; Azouz et al., 1997; Zhu and Connors, 1999). We hypothesized that the
inhibitory interneurons in our sample were prevented from firing
multiple spikes by short-latency disynaptic inhibition mediated by
other inhibitory interneurons in their barrel column. Examination of
synaptic responses of the inhibitory interneuron shown in Figure 3 at a
holding potential of 31 mV indicated that this cell, like the spiny
stellate in the same column, received disynaptic inhibition (Fig.
3C; this cell appeared to receive a dual IPSC: the onset of
the first IPSC is indicated by an arrow, whereas the onset
of the second IPSC coincided with the IPSC in the spiny stellate cell
and is indicated by the right vertical guideline). Of the 15 inhibitory
interneurons that fired single spikes in response to thalamic
stimulation and were tested for inhibitory inputs, 11 received
disynaptic IPSCs at a latency consistent with the hypothesis that
disynaptic inhibition prevented them from firing multiple action potentials.
Although most interneurons fired only once, three interneurons fired
trains of long-latency action potentials after thalamocortical activation. Whole-cell recordings showed that these trains coincided with long-latency barrages of synaptic inputs (data not shown), similar
to those reported in mouse somatosensory cortex during the first
postnatal week (Agmon et al., 1996). Interneurons firing long-latency
barrages were excluded from further analysis.
Excitatory neurons were less responsive to thalamic inputs
Of 105 inhibitory interneurons recorded from in the cell-attached
mode, 57% fired action potentials at an apparent monosynaptic latency
(Fig. 3F, right bar). In marked contrast to the
responsiveness of interneurons, the majority of excitatory neurons
examined in this study did not discharge in response to thalamic
stimulation. A population of 30 excitatory cells in layers IV-V, 19 pyramidal cells and 11 spiny stellate cells, were examined for spike
discharges in response to the same range of intensities of thalamic
stimulation used to evoke spikes in the inhibitory interneurons. Only a
single pyramidal neuron fired (Fig. 3F), although
75% of all excitatory cells tested in the whole-cell mode
(n = 20) were found to receive thalamocortical EPSCs
(Fig. 3B). These results indicate that inhibitory interneurons are considerably more excited by thalamic input than excitatory neurons.
Selective activation of some inhibitory interneurons
As summarized in Figure 3F, close to half of the
inhibitory interneurons in our sample did not fire in response to
thalamocortical stimulation. Because our study was conducted in a slice
preparation, many thalamocortical axons were likely to have been
truncated during the slicing procedure. In addition, the density of
intact thalamocortical innervation in the thalamocortical slice varies between barrels (Agmon et al., 1993). Therefore, it was possible that inhibitory interneurons that did not fire were located in barrels
that did not receive thalamocortical inputs. That this was not the case
was evident from the records of 24 nondischarging inhibitory
interneurons tested for thalamocortical synaptic inputs in the
whole-cell mode. Of these, 79% were found to receive
monosynaptic thalamocortical inputs. Moreover, often other inhibitory
interneurons in the very same barrel column did fire in the
cell-attached mode, making it unlikely that the absence of firing was
attributable to a loss of intact thalamocortical axons. An example is
shown in Figure 4, which illustrates two
inhibitory interneurons in close proximity within a single barrel (Fig.
4A). Only interneuron 2 fired in the
cell-attached mode in response to thalamocortical activation (Fig.
4B, CA), but both cells exhibited a monosynaptic EPSC
in the whole-cell mode (Fig. 4B, WC). Of the 45 inhibitory interneurons that did not fire in response to
thalamocortical stimulation, 58% were located in barrels or columns in
which at least one other interneuron did fire. Thus, in the in
vitro thalamocortical slice some inhibitory interneurons discharge
in response to a thalamocortical input volley, but others do not.
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Figure 4.
Thalamocortical stimulation activates some
interneurons but not others. A, Two biocytin-filled
inhibitory interneurons in the same barrel. B, Four
superimposed traces (5 sec intervals) from interneuron 1 (top
traces) and interneuron 2 (bottom traces) in the
cell-attached (CA) and whole-cell (WC)
modes. Note that despite the close proximity between the two cells,
thalamic stimulation elicited spikes only in interneuron 2. Cell 1 was
stimulated at 100 µA, and cell 2 was stimulated at 40 µA.
Calibration is 10 pA for CA and 100 pA for WC.
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Amplitude of synaptic input determines responsiveness to
thalamic stimulation
Whether a neuron fires in response to a synaptic input or not is
determined by two general factors, the strength of the input and the
intrinsic integrative properties of the neuron. For example, all
intrinsic parameters being equal, a stronger synaptic input would be
more effective in firing the cell than a weaker one, whereas for a
given strength, a synaptic input would be more effective if the neuron
had a higher input resistance or a lower firing threshold relative to
the resting membrane potential. To determine whether the discharging
interneurons exhibited intrinsic properties that made them more
responsive to thalamic inputs, the input resistance, resting membrane
potential, and the threshold for action potentials were compared
between discharging and nondischarging inhibitory interneurons and
between discharging inhibitory interneurons and nondischarging
excitatory neurons. There were no statistically significant differences
in resting membrane potential between discharging inhibitory
interneurons and either inhibitory or excitatory nondischarging neurons
(Table 1; Vm,
two-tailed probabilities were p = 0.19 and
p = 0.59, respectively). The amount of depolarization required to reach threshold (Table 1;
Threshold-Vm) was, on average, somewhat higher in
the discharging inhibitory interneurons compared to nondischarging
inhibitory or excitatory neurons (p = 0.06, p = 0.03, respectively), and the discharging
interneurons had a significantly lower input resistance than either
inhibitory or excitatory nondischarging cells (Table 1; Rm,
p < 0.01 and p < 0.0001, respectively). Both of these differences, however, would actually make
the discharging interneurons less sensitive to synaptic input and
therefore cannot account for the observed differences in response to
thalamocortical stimulation. This suggested that interneurons that
discharged received larger thalamocortical synaptic inputs, as in the
case shown in Figure 4B. Consistent with this
hypothesis, thalamocortical stimulation induced, on average, fivefold
larger synaptic currents in the interneurons that discharged spikes
compared to inhibitory neurons that did not fire and to excitatory
neurons (Table 1; Isynaptic,
p < 0.0001).
Both fast spiking and regular-spiking nonpyramidal interneurons
mediate feedforward inhibition
Inhibitory cortical interneurons exhibit different patterns of
repetitive firing in response to intracellular current injections (Kawaguchi and Kubota, 1997). This diversity suggests that different types of interneurons express different palettes of voltage- and calcium-gated channels and are likely to respond differently during natural, thalamocortically relayed sensory stimulation. It was therefore of interest to determine the firing patterns in our sample of
thalamocortically discharging inhibitory interneurons. Figure
5A shows repetitive firing
elicited in the two interneurons illustrated in Figure 4 (cell 1 and
cell 2, left and middle traces, respectively) and
in a third cell that discharged in response to thalamic stimulation
(right trace). It is evident that the three interneurons
exhibited markedly different spike frequency adaptation patterns, with
the left trace showing the most adaptation, and the right trace the
least adaptation. To characterize such differences quantitatively, we
recorded spike trains from 57 discharging and nondischarging inhibitory
interneurons and calculated a spike frequency adaptation ratio from
each record (see Materials and Methods; adaptation ratios are indicated
in Fig. 5A above each trace). The histogram of the spike
frequency adaptation ratios exhibited two large peaks (Fig.
5B). A value of 0.8, which lies between the two major peaks,
was used to divide the population into two groups, one with adaptation
ratios  0.8, and one with adaptation ratios <0.8, which were called,
following the nomenclature of Kawaguchi (1995), fast spiking (FS) and
regular-spiking nonpyramidal (RSNP) cells, respectively. For example,
the two neurons whose spike trains are illustrated in the left and
middle traces of Figure 5A were classified as RSNP, whereas
the neuron represented by the rightmost spike train was classified as
FS. Unlike adapting inhibitory interneurons in layer V of rat frontal
cortex (Kawaguchi, 1993; Xiang et al., 1998), RSNP neurons in our
sample did not exhibit a low-threshold spike (LTS) after recovery from
hyperpolarization.
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Figure 5.
Both adapting (RSNP) and
nonadapting (FS) interneurons mediate thalamocortical
feedforward inhibition. A, Intrinsic firing patterns of
three inhibitory interneurons that fired in response to thalamic
stimulation, illustrating the large differences in spike frequency
adaptation during the 500 msec current pulse. The left
and middle traces are, respectively, from cells 1 and 2 in Figure 4. B, The distribution of spike frequency
adaptation ratios in a sample of 56 inhibitory interneurons. The value
of 0.8 was selected as a separation point between the FS and RSNP cell
classes. C, Probability of thalamocortically evoked
firing of 24 FS and 33 RSNP neurons. Differences were statistically
insignificant.
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Of all 57 inhibitory interneurons in our sample tested for firing
patterns, 58% were classified as RSNP and 42% as FS. Of 39 thalamocortically discharging inhibitory interneurons, 56% were
classified as RSNP and 44% as FS. As shown in Figure 5C, probabilities of firing in response to thalamocortical stimulation were
66% for RSNP interneurons and 71% for FS cells, and the difference was statistically insignificant (p = 0.48;
Fisher's exact test, single-tailed). We conclude that inhibitory
interneurons from both classes contribute to feedforward inhibition,
approximately at the ratio of their occurrence in the general population.
Interneurons expressing PV or CB are excited by thalamic input
Cortical inhibitory interneurons can be characterized by their
pattern of expression of calcium-binding proteins such as PV and CB
(Celio, 1986; Hendry et al., 1989; Kawaguchi and Kubota, 1993; Cauli et
al., 1997). The calcium-binding protein content of an inhibitory
interneuron correlates with its level of metabolic activity (Maier and
McCasland, 1997) and is also an indicator of the neuropeptides that it
co-releases with GABA (Cauli et al., 1997). It was therefore of
interest to determine the calcium-binding protein content in the
population of thalamocortically discharging inhibitory interneurons.
Figure 6A illustrates a
neuron that discharged spikes in response to thalamic stimulation and
was found to express PV. Of 30 discharging interneurons tested, 50%
were found to express PV. Thirteen neurons of the same group were
tested also for CB immunoreactivity; 15% were CB positive, and one
neuron expressed both markers. We conclude that both PV-expressing and
CB-expressing interneurons contribute to feedforward inhibition in the
barrel cortex, as do interneurons expressing neither marker.
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Figure 6.
PV- or CB-immunopositive and immunonegative
interneurons mediate feedforward thalamocortical inhibition.
A, Confocal images of layer IV in a thalamocortical
slice stained for PV. Pia is toward the left.
Left, PV immunofluorescence (red).
Center, the same microscopic field showing Lucifer yellow
fluorescence (green) in a recorded interneuron
that discharged in response to thalamic stimulation.
Right, Overlay of the two panels at left,
showing colocalization (yellow) of Lucifer yellow
and PV. B, Thalamocortically evoked firing probability
in a population of PV-immunopositive (PV+; n = 18),
PV-immunonegative (PV; n = 24), CB-immunopositive
(CB+; n = 3), and CB-immunonegative (CB;
n = 17) inhibitory interneurons. Differences were
not statistically significant.
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To test whether thalamocortical inputs excite preferentially PV- and/or
CB-expressing inhibitory interneurons, we also tested nondischarging
neurons for PV and CB immunoreactivity. A total of 42 discharging and
nondischarging inhibitory interneurons were tested for PV
immunoreactivity (including the cells described above), and 43% were
immunopositive. Of these, 83% responded to thalamic input with spikes,
whereas of the interneurons that were immunonegative for PV, only 63%
fired (Fig. 6B). Thus, PV-expressing neurons tended
to have a higher probability of firing compared with PV-immunonegative
cells; however this difference did not attain statistical significance
(p = 0.13; Fisher's exact test, single-tailed).
Of 20 inhibitory interneurons tested for CB immunoreactivity, three
were found to express calbindin, and all three fired, whereas of the 17 CB-immunonegative interneurons, 59% fired (Fig. 6C). The
difference in firing probability between CB-immunopositive and
-immunonegative cells was not statistically significant
(p = 0.25). There was also no correlation in our
sample between calcium-binding protein expression and firing patterns
(p = 0.26). We conclude that the type of
calcium-binding protein expressed by an inhibitory interneuron is only
weakly correlated with its probability of activation by thalamocortical afferents.
Several distinct morphological types of interneurons mediate
disynaptic thalamocortical inhibition
Neocortical inhibitory interneurons are a highly diverse group,
not only in their firing patterns and calcium-binding protein contents,
but also in their morphologies (Houser et al., 1983; Cobas et al.,
1987; Kisvarday et al., 1990; Lorente de Nó, 1992; Prieto et al.,
1994; Kawaguchi and Kubota, 1997). Of all morphological features,
probably the one most likely to affect the functional role of a neuron
in the cortical circuit is the spatial distribution of its synaptic
terminals, which can be inferred from the distribution of its axonal
arborizations. It was therefore of interest to determine the axonal
trajectories of thalamocortically discharging inhibitory interneurons
in our sample. A total of 19 biocytin-stained discharging interneurons,
selected for good filling of their axonal arbors, were reconstructed
morphologically; of these, 11 are illustrated in Figure
7. With two exceptions, all the
reconstructed interneurons had cell bodies within layer IV or
straddling the IV/V border and had most of their dendritic processes
(Fig. 7, blue) within layer IV. Based on their axonal arbor
(Fig. 7, red), the reconstructed neurons fell into five
morphological types (A-E). Types A and B had an
axonal arbor that formed a dense plexus coextensive with their
dendritic tree, either restricted to layer IV (type A;
n = 5) or extending into lower layer III (type B;
n = 4), with only sparse branches in layer V, if at
all. Type C was represented in our sample by two neurons with a cell
body in lower layer V and with dendrites straddling the layers V/VI
border and not extending into layer IV. Both had an elaborate axonal
plexus in layer IV, and one (Fig. 7C) had a bilaminar axonal
plexus, with a lower plexus in lower layer V surrounding its dendritic
tree. Types D and E had axonal trees that formed a plexus extending
beyond the dendritic branches into layers II/III vertically (type D; n = 2) or both vertically and horizontally (type E;
n = 6). The horizontal extent in layers II/III of the
axonal arbor of type E varied between 350 and 776 µm. Because our
plane of section was approximately parallel to the rows of barrels (A. Agmon, unpublished observations) and therefore parallel to the minor
axis of the barrels, which in mouse is <200-µm-long (Woolsey and Van
der Loos, 1970), excitation of type E interneurons would provide
inhibition to at least one additional barrel column in the same row, on
either or both sides of their own column. Several neurons of all five types, specifically those with cell bodies close to the layers IV/V
border, closely resembled the so-called "Lorente de Nó cells" (Cobas et al., 1987; Fairén, 1993) (compare the middle neuron of
Fig. 7B to Fig. 13C of Lorente de Nó,
1992). The morphological type of a neuron appeared to be independent of
its immunocytochemical or electrophysiological identities; for example,
both immunopositive and immunonegative PV and CB interneurons and both
FS and RSNP cells were among those classified as type A. We conclude
that several distinct morphological types of interneurons mediate
feedforward thalamocortical inhibition, some of them generating
feedforward inhibition within their own barrels, whereas others are
likely to relay disynaptic inhibition to the upper cortical layers
within their own columns and to columns outside their barrel of
origin.
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Figure 7.
Several morphological types of interneurons
mediate feedforward thalamocortical inhibition. Computer-assisted
reconstructions of 14 biocytin-filled neurons, with cell bodies and
dendritic trees in blue and axonal arborizations in
red. Dendrites and axons are represented with lines of
constant width. Laminar boundaries are indicated by thin green
lines and labeled with roman numerals on the
right. For ease of comparison, tracing sizes were adjusted
to the same apparent vertical extent of layer IV, so the scale bar
varies slightly between panels but is ~200 µm. See Results for
descriptions of the five morphological types.
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DISCUSSION |
Disynaptic, feedforward inhibition plays an all-important role in
the initial processing of incoming sensory information by the
neocortex, but the precise identity of the interneurons that generate
it has been largely unknown. To our knowledge this is the first
detailed intracellular examination, in any cortical area, of inhibitory
interneurons that fire in response to a thalamocortical input volley.
Our results suggest that no single, uniform class of interneurons can
be considered the sole source of disynaptic inhibition.
Thalamic inputs preferentially excite inhibitory interneurons
In the present study, excitatory neurons were unresponsive to the
same intensities of thalamic stimulation that excited inhibitory interneurons. This finding is in agreement with previous data in
vivo showing that, compared with excitatory neurons, putative inhibitory neurons respond more vigorously, at lower thresholds, and
with shorter latencies (Simons, 1978; Yamamoto et al., 1988; Simons and
Carvell, 1989; Swadlow, 1989; Welker et al., 1993) and are
metabolically more active (Nie and Wong-Riley, 1995; McCasland and
Hibbard, 1997). It was previously suggested (Simons, 1995) that the
thalamocortical synapses may be more effective on inhibitory neurons
because they impinge on their somata and proximal dendritic shafts,
while impinging on dendritic spines of excitatory neurons (Peters et
al., 1976; White et al., 1984; Keller and White, 1987; Staiger et
al., 1996). However, computational and analytical models suggest that
the efficacy of excitatory inputs on spines and on dendritic shafts is
likely to be similar (Johnston and Wu, 1995; Koch, 1999). Our data
(Table 1) suggest that it is the considerably stronger thalamocortical
synaptic currents in (some) inhibitory interneurons, compared with
excitatory neurons, which accounted for the differences in firing
probability. The effect of a larger synaptic current would be to
generate a faster rising EPSP (because at the onset of the EPSP,
dVm/dt = Isynaptic/Cm),
causing the inhibitory interneurons to fire first and thereby to
generate IPSPs in the excitatory neurons, preventing them from reaching threshold. A stronger thalamocortical synaptic current may be attributable to the higher single-channel conductance of AMPA-subtype glutamate receptors in inhibitory interneurons, most of which lack the
GluR2 receptor subunit (Angulo et al., 1997; Swanson et al., 1997).
Only a subset of all inhibitory interneurons are
activated by thalamocortical inputs
Our results indicate that only a subset of interneurons within
each barrel column fired in response to thalamocortical stimulation. Comparison of responsive and nonresponsive inhibitory interneurons suggested that, as in the comparison with excitatory neurons above, it
was not the intrinsic properties of the interneuron that
determined its responsiveness, but most likely the magnitude of the
thalamocortical synaptic input it received. The differences in the
magnitude of thalamic input onto different inhibitory interneurons are
probably the functional correlates of the variability in the numbers
and locations of thalamocortical synapses made on them (White and Rock,
1981; White et al., 1984; Keller and White, 1987).
Mutual suppression of firing by
inhibitory interneurons
The great majority of the inhibitory neurons examined in our study
fired a single spike after thalamocortical stimulation. This could be
explained by our finding that layer IV interneurons receive disynaptic
thalamocortical inhibition, presumably via other inhibitory neurons in
their vicinity. Dual recordings in the rat (Gibson et al., 1999) and
cat (Tamas et al., 1998) have confirmed directly that neocortical layer
IV interneurons inhibit other layer IV interneurons in their proximity.
GABAergic cortical neurons can also inhibit themselves through autapses
(Thomson et al., 1996; Tamas et al., 1997b). Thus, inhibitory
interneurons effectively suppress each other's firing after their
first spike, a mechanism that may allow for a faster recovery of the
cortex from the inhibitory volley.
Both FS and RSNP interneurons mediate feedforward inhibition
Inhibitory interneurons in our sample could be broadly divided by
their intrinsic firing patterns into two groups, FS and RSNP, which
differed in the degree of spike frequency adaptation. Similar
differences in spike frequency adaptation were previously found among
inhibitory interneurons in various cortical areas and layers
(Kawaguchi, 1993; Hirsch, 1995; Kawaguchi, 1995; Cauli et al., 1997;
Gibson et al., 1999; Dantzker and Callaway, 2000; Gupta et al., 2000).
FS interneurons discharge at short latency in response to whisker
stimulation in vivo (Simons, 1978; Swadlow, 1989; Zhu and
Connors, 1999) and receive monosynaptic thalamocortical input in the
thalamocortical slice (Agmon and Connors, 1992; Gibson et al., 1999).
Our data confirm that FS interneurons are discharged by thalamocortical
afferents, but show that RSNP interneurons, which are characterized by
a pronounced spike frequency adaptation, also mediate feedforward
inhibition. RSNP cells have not been identified in single-unit
recordings, and therefore our data do not conflict with the
extracellular studies cited above. Our findings are apparently at odds
with those of Gibson et al. (1999), who report that thalamocortical
responses are smaller and less frequently observed in the adapting
(their LTS) compared with the nonadapting (FS) interneurons. Gibson et
al. (1999) used a stimulation protocol that was intended to activate
only a single axon; it is therefore possible that adapting interneurons
receive convergent input from many thalamocortical axons, thereby
compensating for the small size of each unitary EPSP. Alternatively, it
is possible that there is no precise correspondence between the RSNP
and LTS classes, or that differences in species or recording conditions
(e.g., temperature) accounted for the discrepancy. Both nonadapting and adapting layer IV neurons are coupled to other neurons of their own
kind by gap junctions (Galarreta and Hestrin, 1999; Gibson et al.,
1999; Beierlein et al., 2000). Thus, thalamocortical activation of even
a subset of these cells may result in a synchronous inhibitory spike
volley caused by the spread of excitation through a large population of
electrically coupled cells.
Thalamic excitation of parvalbumin- and
calbindin-expressing interneurons
PV-expressing interneurons in the somatosensory cortex receive
multiple thalamocortical contacts (Staiger et al., 1996) and are
metabolically more active than CB-expressing interneurons (Maier and
McCasland, 1997), suggesting that the former may be more likely to fire
in response to thalamocortical input. In our sample we found a higher
firing probability of PV-expressing compared to nonexpressing neurons,
but this difference did not attain statistical significance. The
fraction of PV-immunopositive cells in our sample (43%) was smaller
than found previously in layer IV (73%; Ren et al., 1992), possibly
because PV expression in layer IV has not peaked yet at the ages we
studied (Sanchez et al., 1992; del Rio et al., 1994; Alcantara et al.,
1996) or because of experimental limitations (e.g., dialysis of the
antigen by the recording solution). This could have caused us to
underestimate the difference in firing probabilities between
PV-immunopositive and PV-immunonegative interneurons.
Nevertheless, our data clearly show that neurons expressing PV, neurons
expressing CB, and neurons expressing neither marker participate in
feedforward inhibition.
Morphological types of inhibitory interneurons and their
functional roles
Inhibitory interneurons of cortical layers IV and V activated
thalamocortically were heterogeneous also in their dendritic and axonal
morphologies. Within this heterogeneity, however, there was a clear
grouping of cells into several distinct morphological types (Fig. 7),
which differed in the vertical and horizontal distributions of their
axons, and thereby in their potential role in the thalamocortical
circuit. Thus, neurons of type A, with an axonal arbor restricted to
their own barrel, are likely to generate strong disynaptic inhibition
in other barrel neurons, both excitatory and inhibitory. Because
putative inhibitory barrel neurons often have multiwhisker receptive
fields (Simons and Carvell, 1989; Swadlow, 1989; Welker et al., 1993),
type A neurons may also mediate the adjacent-whisker inhibition
observed in vivo (Simons, 1995; Goldreich et al., 1999).
Types B, D, and E neurons, with a sphere of influence extending to
layers II/III, probably mediate the strong disynaptic inhibition
observed in supragranular neurons in vivo (Ferster and
Lindstrom, 1983; Kyriazi et al., 1998; Brumberg et al., 1999; Zhu and
Connors, 1999) or in vitro (Agmon and Connors, 1992).
Finally, inhibitory neurons of morphological type E, with axonal trees
that extend tangentially at least one barrel width on either or both
sides of the column of origin, will generate the short-latency
cross-column inhibition that is a prominent feature in supragranular
layers of mouse barrel cortex in vivo (Welker et al.,
1993).
Excitatory and inhibitory flow after a thalamocortical volley
The overwhelming preponderance of upwardly directed axonal arbors
of layer IV interneurons indicates that the flow of inhibition in the
barrel cortex, after a thalamocortical volley, will be toward the upper
layers. Interestingly, this is also the main direction of flow of
excitation mediated by spiny stellate and star pyramidal cells' axons
(Lund et al., 1979; Ferster and Lindstrom, 1983; Armstrong-James et
al., 1992; Anderson et al., 1994; Lubke et al., 2000). Thus, inhibition
in the cortex is inextricably linked to excitation, apparently
following it along its intracortical course. This close association
between excitatory and inhibitory influences ensures that the most
pertinent sensory information will be incorporated into a conscious
sensory experience, while other, weaker and potentially distracting,
inputs will be suppressed (Welker et al., 1993; Moore and Nelson,
1998), in effect producing a contrast-enhancement operation on the
cortical representation of the sensory environment.
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FOOTNOTES |
Received Nov. 20, 2000; revised Jan. 22, 2001; accepted Jan. 31, 2001.
This work was supported by National Institutes of Health Grant HD33463.
J.T.P. was supported by National Institutes of Health Grant NS10902. We
thank Drs. Diane O'Dowd and George Spirou for a critical reading of an
earlier version of this manuscript.
Correspondence should be addressed to Ariel Agmon, Department of
Anatomy, P.O. Box 9128, West Virginia University, Morgantown, WV
26506-9128. E-mail: aagmon{at}wvu.edu.
Dr. Porter's present address: Department of Pharmacology and
Toxicology, Ponce School of Medicine, P.O. Box 7004, Ponce, Puerto Rico 00732.
| |
REFERENCES |
-
Agmon A,
Connors BW
(1991)
Thalamocortical responses of mouse somatosensory (barrel) cortex in vitro.
Neuroscience
41:365-379[Web of Science][Medline].
-
Agmon A,
Connors BW
(1992)
Correlation between intrinsic firing patterns and thalamocortical synaptic responses of neurons in mouse barrel cortex.
J Neurosci
12:319-329[Abstract].
-
Agmon A,
Yang LT,
O'Dowd DK,
Jones EG
(1993)
Organized growth of thalamocortical axons from the deep tier of terminations into layer IV of developing mouse barrel cortex.
J Neurosci
13:5365-5382[Abstract].
-
Agmon A,
Hollrigel G,
O'Dowd DK
(1996)
Functional GABAergic synaptic connection in neonatal mouse barrel cortex.
J Neurosci
16:4684-4695[Abstract/Free Full Text].
-
Alcantara S,
de Lecea L,
Del Rio JA,
Ferrer I,
Soriano E
(1996)
Transient colocalization of parvalbumin and calbindin D28k in the postnatal cerebral cortex: evidence for a phenotypic shift in developing nonpyramidal neurons.
Eur J Neurosci
8:1329-1339[Web of Science][Medline].
-
Anderson JC,
Douglas RJ,
Martin KA,
Nelson JC
(1994)
Synaptic output of physiologically identified spiny stellate neurons in cat visual cortex.
J Comp Neurol
341:16-24[Web of Science][Medline].
-
Angulo MC,
Lambolez B,
Audinat E,
Hestrin S,
Rossier J
(1997)
Subunit composition, kinetic, and permeation properties of AMPA receptors in single neocortical nonpyramidal cells.
J Neurosci
17:6685-6696[Abstract/Free Full Text].
-
Armstrong-James M,
Fox K,
Das-Gupta A
(1992)
Flow of excitation within rat barrel cortex on striking a single vibrissa.
J Neurophysiol
68:1345-1358[Abstract/Free Full Text].
-
Azouz R,
Gray CM,
Nowak LG,
McCormick DA
(1997)
Physiological properties of inhibitory interneurons in cat striate cortex.
Cereb Cortex
7:534-545[Abstract/Free Full Text].
-
Beierlein M,
Gibson JR,
Connors BW
(2000)
A network of electrically coupled interneurons drives synchronized inhibition in neocortex.
Nat Neurosci
3:904-910[Web of Science][Medline].
-
Brumberg JC,
Pinto DJ,
Simons DJ
(1996)
Spatial gradients and inhibitory summation in the rat whisker barrel system.
J Neurophysiol
76:130-140[Abstract/Free Full Text].
-
Brumberg JC,
Pinto DJ,
Simons DJ
(1999)
Cortical columnar processing in the rat whisker-to-barrel system.
J Neurophysiol
82:1808-1817[Abstract/Free Full Text].
-
Cauli B,
Audinat E,
Lambolez B,
Angulo MC,
Ropert N,
Tsuzuki K,
Hestrin S,
Rossier J
(1997)
Molecular and physiological diversity of cortical nonpyramidal cells.
J Neurosci
17:3894-3906[Abstract/Free Full Text].
-
Celio MR
(1986)
Parvalbumin in most gamma-aminobutyric acid-containing neurons of the rat cerebral cortex.
Science
231:995-997[Abstract/Free Full Text].
-
Cobas A,
Welker E,
Fairen A,
Kraftsik R,
Van der Loos H
(1987)
GABAergic neurons in the barrel cortex of the mouse: an analysis using neuronal archetypes.
J Neurocytol
16:843-870[Web of Science][Medline].
-
Dantzker JL,
Callaway EM
(2000)
Laminar sources of synaptic input to cortical inhibitory interneurons and pyramidal neurons.
Nat Neurosci
3:701-707[Web of Science][Medline].
-
del Rio JA,
de Lecea L,
Ferrer I,
Soriano E
(1994)
The development of parvalbumin-immunoreactivity in the neocortex of the mouse.
Brain Res Dev Brain Res
81:247-259[Medline].
-
Dykes RW,
Landry P,
Metherate R,
Hicks TP
(1984)
Functional role of GABA in cat primary somatosensory cortex: shaping receptive fields of cortical neurons.
J Neurophysiol
52:1066-1093[Abstract/Free Full Text].
-
Fairén A
(1993)
Axonal patterns of interneurons in the cerebral cortex: in memory of Rafael Lorente de No.
In: The mammalian cochlear nuclei: organization and function (Merchan MA,
Juiz JM,
Godfried DA,
Mugnaini E,
eds), pp 467-478. New York: Plenum.
-
Fairén A,
Valverde F
(1979)
Specific thalamo-cortical afferents and their presumptive targets in the visual cortex. A Golgi study.
Prog Brain Res
51:419-438[Medline].
-
Ferster D,
Lindstrom S
(1983)
An intracellular analysis of geniculo-cortical connectivity in area 17 of the cat.
J Physiol (Lond)
342:181-215[Abstract/Free Full Text].
-
Freund TF,
Martin KA,
Somogyi P,
Whitteridge D
(1985)
Innervation of cat visual areas 17 and 18 by physiologically identified X- and Y- type thalamic afferents. II. Identification of postsynaptic targets by GABA immunocytochemistry and Golgi impregnation.
J Comp Neurol
242:275-291[Web of Science][Medline].
-
Galarreta M,
Hestrin S
(1999)
A network of fast-spiking cells in the neocortex connected by electrical synapses.
Nature
402:72-75[Medline].
-
Gibson JR,
Beierlein M,
Connors BW
(1999)
Two networks of electrically coupled inhibitory neurons in neocortex.
Nature
402:75-79[Medline].
-
Gil Z,
Amitai Y
(1996)
Properties of convergent thalamocortical and intracortical synaptic potentials in single neurons of neocortex.
J Neurosci
16:6567-6578[Abstract/Free Full Text].
-
Goldreich D,
Kyriazi HT,
Simons DJ
(1999)
Functional independence of layer IV barrels in rodent somatosensory cortex.
J Neurophysiol
82:1311-1316[Abstract/Free Full Text].
-
Good PI
(1999)
In: Resampling methods. Boston: Birkhauser.
-
Gupta A,
Wang Y,
Markram H
(2000)
Organizing principles for a diversity of GABAergic interneurons and synapses in the neocortex.
Science
287:273-278[Abstract/Free Full Text].
-
Hendry SH,
Jones EG,
Emson PC,
Lawson DE,
Heizmann CW,
Streit P
(1989)
Two classes of cortical GABA neurons defined by differential calcium binding protein immunoreactivities.
Exp Brain Res
76:467-472[Web of Science][Medline].
-
Hicks TP,
Dykes RW
(1983)
Receptive field size for certain neurons in primary somatosensory cortex is determined by GABA-mediated intracortical inhibition.
Brain Res
274:160-164[Web of Science][Medline].
-
Hirsch JA
(1995)
Synaptic integration in layer IV of the ferret striate cortex.
J Physiol (Lond)
483:183-199[Abstract/Free Full Text].
-
Houser CR,
Hendry SH,
Jones EG,
Vaughn JE
(1983)
Morphological diversity of immunocytochemically identified GABA neurons in the monkey sensory-motor cortex.
J Neurocytol
12:617-638[Web of Science][Medline].
-
Johnston D,
Wu SM
(1995)
Dendritic spines and their effects on synaptic inputs.
In: Foundations of cellular neurophysiology, pp 400-411 Cambridge, MA: MIT.
-
Jones EG,
Hendry SH
(1984)
Basket cells.
In: Cellular components of the cerebral cortex (Peters A,
Jones EG,
eds), pp 309-336. New York: Plenum.
-
Kawaguchi Y
(1993)
Groupings of nonpyramidal and pyramidal cells with specific physiological and morphological characteristics in rat frontal cortex.
J Neurophysiol
69:416-431[Abstract/Free Full Text].
-
Kawaguchi Y
(1995)
Physiological subgroups of nonpyramidal cells with specific morphological characteristics in layer II/III of rat frontal cortex.
J Neurosci
15:2638-2655[Abstract].
-
Kawaguchi Y,
Kubota Y
(1993)
Correlation of physiological subgroupings of nonpyramidal cells with parvalbumin- and calbindin D28k-immunoreactive neurons in layer V of rat frontal cortex.
J Neurophysiol
70:387-396[Abstract/Free Full Text].
-
Kawaguchi Y,
Kubota Y
(1997)
GABAergic cell subtypes and their synaptic connections in rat frontal cortex.
Cereb Cortex
7:476-486[Abstract/Free Full Text].
-
Keller A,
White EL
(1987)
Synaptic organization of GABAergic neurons in the mouse SmI cortex.
J Comp Neurol
262:1-12[Web of Science][Medline].
-
Kharazia VN,
Weinberg RJ
(1993)
Glutamate in terminals of thalamocortical fibers in rat somatic sensory cortex.
Neurosci Lett
157:162-166[Web of Science][Medline].
-
Kisvarday ZF,
Gulyas A,
Beroukas D,
North JB,
Chubb IW,
Somogyi P
(1990)
Synapses, axonal and dendritic patterns of GABA-immunoreactive neurons in human cerebral cortex.
Brain
113:793-812[Abstract/Free Full Text].
-
Koch C
(1999)
Dendritic spines.
In: Biophysics of computation, pp 280-307 New York: Oxford UP.
-
Kyriazi H,
Carvell GE,
Brumberg JC,
Simons DJ
(1998)
Laminar differences in bicuculline methiodide's effects on cortical neurons in the rat whisker/barrel system.
Somatosens Mot Res
15:146-156[Web of Science][Medline].
-
Kyriazi HT,
Carvell GE,
Brumberg JC,
Simons DJ
(1996)
Effects of baclofen and phaclofen on receptive field properties of rat whisker barrel neurons.
Brain Res
712:325-328[Web of Science][Medline].
-
Lin CS,
Lu SM,
Schmechel DE
(1985)
Glutamic acid decarboxylase immunoreactivity in layer IV of barrel cortex of rat and mouse.
J Neurosci
5:1934-1939[Abstract].
-
Lorente de Nó R
(1992)
The cerebral cortex of the mouse (a first contribution-the "acoustic" cortex).
Somatosens Mot Res
9:3-36[Web of Science][Medline]. (English translation of the original 1922 paper, translated by Fairén A, Regidor J, and Kruger L).
-
Lubke J,
Egger V,
Sakmann B,
Feldmeyer D
(2000)
Columnar organization of dendrites and axons of single and synaptically coupled excitatory spiny neurons in layer 4 of the rat barrel cortex.
J Neurosci
20:5300-5311[Abstract/Free Full Text].
-
Lund JS,
Henry GH,
MacQueen CL,
Harvey AR
(1979)
Anatomical organization of the primary visual cortex (area 17) of the cat. A comparison with area 17 of the macaque monkey.
J Comp Neurol
184:599-618[Web of Science][Medline].
-
Maier DL,
McCasland JS
(1997)
Calcium-binding protein phenotype defines metabolically distinct groups of neurons in barrel cortex of behaving hamsters.
Exp Neurol
145:71-80[Web of Science][Medline].
-
McCasland JS,
Hibbard LS
(1997)
GABAergic neurons in barrel cortex show strong, whisker-dependent metabolic activation during normal behavior.
J Neurosci
17:5509-5527[Abstract/Free Full Text].
-
McCormick DA,
Connors BW,
Lighthall JW,
Prince DA
(1985)
Comparative electrophysiology of pyramidal and sparsely spiny stellate neurons of the neocortex.
J Neurophysiol
54:782-806[Abstract/Free Full Text].
-
Moore CI,
Nelson SB
(1998)
Spatio-temporal subthreshold receptive fields in the vibrissa representation of rat primary somatosensory cortex.
J Neurophysiol
80:2882-2892[Abstract/Free Full Text].
-
Nie F,
Wong-Riley MT
(1995)
Double labeling of GABA and cytochrome oxidase in the macaque visual cortex: quantitative EM analysis.
J Comp Neurol
356:115-131[Web of Science][Medline].
-
Peters A,
Kara DA
(1985a)
The neuronal composition of area 17 of rat visual cortex. I. The pyramidal cells.
J Comp Neurol
234:218-241[Web of Science][Medline].
-
Peters A,
Kara DA
(1985b)
The neuronal composition of area 17 of rat visual cortex. II. The nonpyramidal cells.
J Comp Neurol
234:242-263[Web of Science][Medline].
-
Peters A,
Feldman M,
Saldanha J
(1976)
The projection of the lateral geniculate nucleus to area 17 of the rat cerebral cortex. II. Terminations upon neuronal perikarya and dendritic shafts.
J Neurocytol
5:85-107[Web of Science][Medline].
-
Porter JT,
Cauli B,
Tsuzuki K,
Lambolez B,
Rossier J,
Audinat E
(1999)
Selective excitation of subtypes of neocortical interneurons by nicotinic receptors.
J Neurosci
19:5228-5235[Abstract/Free Full Text].
-
Prieto JJ,
Peterson BA,
Winer JA
(1994)
Morphology and spatial distribution of GABAergic neurons in cat primary auditory cortex (AI).
J Comp Neurol
344:349-382[Web of Science][Medline].
-
Ren JQ,
Aika Y,
Heizmann CW,
Kosaka T
(1992)
Quantitative analysis of neurons and glial cells in the rat somatosensory cortex, with special reference to GABAergic neurons and parvalbumin-containing neurons.
Exp Brain Res
92:1-14[Web of Science][Medline].
-
Reyes A,
Lujan R,
Rozov A,
Burnashev N,
Somogyi P,
Sakmann B
(1998)
Target-cell-specific facilitation and depression in neocortical circuits.
Nat Neurosci
1:279-285[Web of Science][Medline].
-
Sanchez MP,
Frassoni C,
Alvarez-Bolado G,
Spreafico R,
Fairen A
(1992)
Distribution of calbindin and parvalbumin in the developing somatosensory cortex and its primordium in the rat: an immunocytochemical study.
J Neurocytol
21:717-736[Web of Science][Medline].
-
Sillito AM
(1975)
The contribution of inhibitory mechanisms to the receptive field properties of neurones in the striate cortex of the cat.
J Physiol (Lond)
250:305-329[Abstract/Free Full Text].
-
Sillito AM,
Kemp JA,
Milson JA,
Berardi N
(1980)
A re-evaluation of the mechanisms underlying simple cell orientation selectivity.
Brain Res
194:517-520[Web of Science][Medline].
-
Simons DJ
(1978)
Response properties of vibrissa units in rat SI somatosensory neocortex.
J Neurophysiol
41:798-820[Abstract/Free Full Text].
-
Simons DJ
(1995)
Neuronal integration in the somatosensory whisker/barrel cortex.
In: Cerebral cortex (Jones EG,
Diamond IT,
eds), pp 263-297. New York: Plenum.
-
Simons DJ,
Carvell GE
(1989)
Thalamocortical response transformation in the rat vibrissa/barrel system.
J Neurophysiol
61:311-330[Abstract/Free Full Text].
-
Simons DJ,
Woolsey TA
(1984)
Morphology of Golgi-Cox-impregnated barrel neurons in rat SmI cortex.
J Comp Neurol
230:119-132[Web of Science][Medline].
-
Somogyi P
(1977)
A specific "axo-axonal" interneuron in the visual cortex of the rat.
Brain Res
136:345-350[Web of Science][Medline].
-
Staiger JF,
Zilles K,
Freund TF
(1996)
Distribution of GABAergic elements postsynaptic to ventroposteromedial thalamic projections in layer IV of rat barrel cortex.
Eur J Neurosci
8:2273-2285[Web of Science][Medline].
-
Stuart GJ,
Dodt HU,
Sakmann B
(1993)
Patch-clamp recordings from the soma and dendrites of neurons in brain slices using infrared video microscopy.
Pflügers Arch
423:511-518[Web of Science][Medline].
-
Swadlow HA
(1989)
Efferent neurons and suspected interneurons in S-1 vibrissa cortex of the awake rabbit: receptive fields and axonal properties.
J Neurophysiol
62:288-308[Abstract/Free Full Text].
-
Swadlow HA
(1990)
Efferent neurons and suspected interneurons in S-1 forelimb representation of the awake rabbit: receptive fields and axonal properties.
J Neurophysiol
63:1477-1498[Abstract/Free Full Text].
-
Swadlow HA,
Gusev AG
(2000)
The influence of single VB thalamocortical impulses on barrel columns of rabbit somatosensory cortex.
J Neurophysiol
83:2802-2813[Abstract/Free Full Text].
-
Swadlow HA,
Beloozerova IN,
Sirota MG
(1998)
Sharp, local synchrony among putative feed-forward inhibitory interneurons of rabbit somatosensory cortex.
J Neurophysiol
79:567-582[Abstract/Free Full Text].
-
Swanson GT,
Kamboj SK,
Cull-Candy SG
(1997)
Single-channel properties of recombinant AMPA receptors depend on RNA editing, splice variation, and subunit composition.
J Neurosci
17:58-69[Abstract/Free Full Text].
-
Tamas G,
Buhl EH,
Somogyi P
(1997a)
Fast IPSPs elicited via multiple synaptic release sites by different types of GABAergic neurone in the cat visual cortex.
J Physiol (Lond)
500:715-738[Abstract/Free Full Text].
-
Tamas G,
Buhl EH,
Somogyi P
(1997b)
Massive autaptic self-innervation of GABAergic neurons in cat visual cortex.
J Neurosci
17:6352-6364[Abstract/Free Full Text].
-
Tamas G,
Somogyi P,
Buhl EH
(1998)
Differentially interconnected networks of GABAergic interneurons in the visual cortex of the cat.
J Neurosci
18:4255-4270[Abstract/Free Full Text].
-
Thomson AM,
West DC,
Hahn J,
Deuchars J
(1996)
Single axon IPSPs elicited in pyramidal cells by three classes of interneurones in slices of rat neocortex.
J Physiol (Lond)
496:81-102[Abstract/Free Full Text].
-
Tsumoto T,
Eckart W,
Creutzfeldt OD
(1979)
Modification of orientation sensitivity of cat visual cortex neurons by removal of GABA-mediated inhibition.
Exp Brain Res
34:351-363[Web of Science][Medline].
-
Welker E,
Armstrong-James M,
Van der Loos H,
Kraftsik R
(1993)
The mode of activation of a barrel column: response properties of single units in the somatosensory cortex of the mouse upon whisker deflection.
Eur J Neurosci
5:691-712[Web of Science][Medline]. [Erratum (1993) 5:1421]
-
White EL
(1978)
Identified neurons in mouse Sml cortex which are postsynaptic to thalamocortical axon terminals: a combined Golgi-electron microscopic and degeneration study.
J Comp Neurol
181:627-661[Web of Science][Medline].
-
White EL,
Rock MP
(1981)
A comparison of thalamocortical and other synaptic inputs to dendrites of two non-spiny neurons in a single barrel of mouse SmI cortex.
J Comp Neurol
195:265-277[Web of Science][Medline].
-
White EL,
Benshalom G,
Hersch SM
(1984)
Thalamocortical and other synapses involving nonspiny multipolar cells of mouse SmI cortex.
J Comp Neurol
229:311-320[Web of Science][Medline].
-
Woolsey TA,
Van der Loos H
(1970)
The description of a cortical field composed of discrete cytoarchitectonic units.
Brain Res
17:205-242[Web of Science][Medline].
-
Xiang Z,
Huguenard JR,
Prince DA
(1998)
Cholinergic switching within neocortical inhibitory networks.
Science
281:985-988[Abstract/Free Full Text].
-
Yamamoto T,
Samejima A,
Oka H
(1988)
Short latency activation of local circuit neurons in the cat somatosensory cortex.
Brain Res
461:199-203[Web of Science][Medline].
-
Zhu JJ,
Connors BW
(1999)
Intrinsic firing patterns and whisker-evoked synaptic responses of neurons in the rat barrel cortex.
J Neurophysiol
81:1171-1183[Abstract/Free Full Text].
Copyright © 2001 Society for Neuroscience 0270-6474/01/2182699-12$05.00/0
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|
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|
|
|
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5069 - 5082.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
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16(4):
541 - 552.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
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26(11):
3056 - 3065.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
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Cereb Cortex,
February 1, 2006;
16(2):
223 - 236.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
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J. Neurosci.,
January 25, 2006;
26(4):
1219 - 1230.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
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Balanced Excitation and Inhibition Determine Spike Timing during Frequency Adaptation
J. Neurosci.,
January 11, 2006;
26(2):
448 - 457.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
E. Foeller, T. Celikel, and D. E. Feldman
Inhibitory Sharpening of Receptive Fields Contributes to Whisker Map Plasticity in Rat Somatosensory Cortex
J Neurophysiol,
December 1, 2005;
94(6):
4387 - 4400.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
L. S. Krimer, A. V. Zaitsev, G. Czanner, S. Kroner, G. Gonzalez-Burgos, N. V. Povysheva, S. Iyengar, G. Barrionuevo, and D. A. Lewis
Cluster Analysis-Based Physiological Classification and Morphological Properties of Inhibitory Neurons in Layers 2-3 of Monkey Dorsolateral Prefrontal Cortex
J Neurophysiol,
November 1, 2005;
94(5):
3009 - 3022.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
D. F. McLaughlin and S. L. Juliano
Disruption of Layer 4 Development Alters Laminar Processing in Ferret Somatosensory Cortex
Cereb Cortex,
November 1, 2005;
15(11):
1791 - 1803.
[Abstract]
[Full Text]
[PDF]
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C. P. Pluto, N. L. Chiaia, R. W. Rhoades, and R. D. Lane
Reducing Contralateral SI Activity Reveals Hindlimb Receptive Fields in the SI Forelimb-Stump Representation of Neonatally Amputated Rats
J Neurophysiol,
September 1, 2005;
94(3):
1727 - 1732.
[Abstract]
[Full Text]
[PDF]
|
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|
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H. J. Rose and R. Metherate
Auditory Thalamocortical Transmission Is Reliable and Temporally Precise
J Neurophysiol,
September 1, 2005;
94(3):
2019 - 2030.
[Abstract]
[Full Text]
[PDF]
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V. C. Kotak, S. Fujisawa, F. A. Lee, O. Karthikeyan, C. Aoki, and D. H. Sanes
Hearing Loss Raises Excitability in the Auditory Cortex
J. Neurosci.,
April 13, 2005;
25(15):
3908 - 3918.
[Abstract]
[Full Text]
[PDF]
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R. D. Traub, D. Contreras, M. O. Cunningham, H. Murray, F. E. N. LeBeau, A. Roopun, A. Bibbig, W. B. Wilent, M. J. Higley, and M. A. Whittington
Single-Column Thalamocortical Network Model Exhibiting Gamma Oscillations, Sleep Spindles, and Epileptogenic Bursts
J Neurophysiol,
April 1, 2005;
93(4):
2194 - 2232.
[Abstract]
[Full Text]
[PDF]
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D. Feldmeyer, A. Roth, and B. Sakmann
Monosynaptic Connections between Pairs of Spiny Stellate Cells in Layer 4 and Pyramidal Cells in Layer 5A Indicate That Lemniscal and Paralemniscal Afferent Pathways Converge in the Infragranular Somatosensory Cortex
J. Neurosci.,
March 30, 2005;
25(13):
3423 - 3431.
[Abstract]
[Full Text]
[PDF]
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J. Watts and A. M. Thomson
Excitatory and inhibitory connections show selectivity in the neocortex
J. Physiol.,
January 1, 2005;
562(1):
89 - 97.
[Abstract]
[Full Text]
[PDF]
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R. N. S. Sachdev, F. F. Ebner, and C. J. Wilson
Effect of Subthreshold Up and Down States on the Whisker-Evoked Response in Somatosensory Cortex
J Neurophysiol,
December 1, 2004;
92(6):
3511 - 3521.
[Abstract]
[Full Text]
[PDF]
|
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J. T. Porter and D. Nieves
Presynaptic GABAB Receptors Modulate Thalamic Excitation of Inhibitory and Excitatory Neurons in the Mouse Barrel Cortex
J Neurophysiol,
November 1, 2004;
92(5):
2762 - 2770.
[Abstract]
[Full Text]
[PDF]
|
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|
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E. E. Kwegyir-Afful and A. Keller
Response Properties of Whisker-Related Neurons in Rat Second Somatosensory Cortex
J Neurophysiol,
October 1, 2004;
92(4):
2083 - 2092.
[Abstract]
[Full Text]
[PDF]
|
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|
|
|
|
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M. Zhang and K. D. Alloway
Stimulus-Induced Intercolumnar Synchronization of Neuronal Activity in Rat Barrel Cortex: A Laminar Analysis
J Neurophysiol,
September 1, 2004;
92(3):
1464 - 1478.
[Abstract]
[Full Text]
[PDF]
|
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|
|
|
|
|
Y. Zhu, R. L. Stornetta, and J. J. Zhu
Chandelier Cells Control Excessive Cortical Excitation: Characteristics of Whisker-Evoked Synaptic Responses of Layer 2/3 Nonpyramidal and Pyramidal Neurons
J. Neurosci.,
June 2, 2004;
24(22):
5101 - 5108.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
C. Wirth and H.-R. Luscher
Spatiotemporal Evolution of Excitation and Inhibition in the Rat Barrel Cortex Investigated With Multielectrode Arrays
J Neurophysiol,
April 1, 2004;
91(4):
1635 - 1647.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M. F. Casanova, D. Buxhoeveden, and J. Gomez
Disruption in the Inhibitory Architecture of the Cell Minicolumn: Implications for Autisim
Neuroscientist,
December 1, 2003;
9(6):
496 - 507.
[Abstract]
[PDF]
|
|
|
|
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|
|
M. Beierlein, J. R. Gibson, and B. W. Connors
Two Dynamically Distinct Inhibitory Networks in Layer 4 of the Neocortex
J Neurophysiol,
November 1, 2003;
90(5):
2987 - 3000.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
S. Butovas and C. Schwarz
Spatiotemporal Effects of Microstimulation in Rat Neocortex: A Parametric Study Using Multielectrode Recordings
J Neurophysiol,
November 1, 2003;
90(5):
3024 - 3039.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
R. M. Bruno, V. Khatri, P. W. Land, and D. J. Simons
Thalamocortical Angular Tuning Domains within Individual Barrels of Rat Somatosensory Cortex
J. Neurosci.,
October 22, 2003;
23(29):
9565 - 9574.
[Abstract]
[Full Text]
[PDF]
|
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|
|
|
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D. Schubert, R. Kotter, K. Zilles, H. J. Luhmann, and J. F. Staiger
Cell Type-Specific Circuits of Cortical Layer IV Spiny Neurons
J. Neurosci.,
April 1, 2003;
23(7):
2961 - 2970.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
H. A. Swadlow
Fast-spike Interneurons and Feedforward Inhibition in Awake Sensory Neocortex
Cereb Cortex,
January 1, 2003;
13(1):
25 - 32.
[Abstract]
[Full Text]
[PDF]
|
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K. D. Miller
Understanding Layer 4 of the Cortical Circuit: A Model Based on Cat V1
Cereb Cortex,
January 1, 2003;
13(1):
73 - 82.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
|
|
|
M.-C. Perreault, Y. Qin, P. Heggelund, and J J. Zhu
Postnatal development of GABAergic signalling in the rat lateral geniculate nucleus: presynaptic dendritic mechanisms
J. Physiol.,
January 1, 2003;
546(1):
137 - 148.
[Abstract]
[Full Text]
[PDF]
|
|
|
|
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R. M. Bruno and D. J. Simons
Feedforward Mechanisms of Excitatory and Inhibitory Cortical Receptive Fields
J. Neurosci.,
December 15, 2002;
22(24):
10966 - 10975.
[Abstract]
[Full Text]
[PDF]
|
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|
|
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|
M. Beierlein, C. P. Fall, J. Rinzel, and R. Yuste
Thalamocortical Bursts Trigger Recurrent Activity in Neocortical Networks: Layer 4 as a Frequency-Dependent Gate
J. Neurosci.,
November 15, 2002;
22(22):
9885 - 9894.
[Abstract]
[Full Text]
[PDF]
|
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M. Beierlein and B. W. Connors
Short-Term Dynamics of Thalamocortical and Intracortical Synapses Onto Layer 6 Neurons in Neocortex
J Neurophysiol,
October 1, 2002;
88(4):
1924 - 1932.
[Abstract]
[Full Text]
[PDF]
|
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|
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M. F. Casanova, D. P. Buxhoeveden, and C. Brown
Clinical and Macroscopic Correlates of Minicolumnar Pathology in Autism
J Child Neurol,
September 1, 2002;
17(9):
692 - 695.
[Abstract]
[PDF]
|
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|
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M. E. Larkum and J. J. Zhu
Signaling of Layer 1 and Whisker-Evoked Ca2+ and Na+ Action Potentials in Distal and Terminal Dendrites of Rat Neocortical Pyramidal Neurons In Vitro and In Vivo
J. Neurosci.,
August 15, 2002;
22(16):
6991 - 7005.
[Abstract]
[Full Text]
[PDF]
|
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C. C. H. Petersen
Short-Term Dynamics of Synaptic Transmission Within the Excitatory Neuronal Network of Rat Layer 4 Barrel Cortex
J Neurophysiol,
June 1, 2002;
87(6):
2904 - 2914.
[Abstract]
[Full Text]
[PDF]
|
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|
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D. P. Buxhoeveden and M. F. Casanova
The minicolumn hypothesis in neuroscience
Brain,
May 1, 2002;
125(5):
935 - 951.
[Abstract]
[Full Text]
[PDF]
|
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|
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|
W. Bair, J. R. Cavanaugh, M. A. Smith, and J. A. Movshon
The Timing of Response Onset and Offset in Macaque Visual Neurons
J. Neurosci.,
April 15, 2002;
22(8):
3189 - 3205.
[Abstract]
[Full Text]
[PDF]
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S. J. Cruikshank, H. J. Rose, and R. Metherate
Auditory Thalamocortical Synaptic Transmission In Vitro
J Neurophysiol,
January 1, 2002;
87(1):
361 - 384.
[Abstract]
[Full Text]
[PDF]
|
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C. Rozas, H. Frank, A. J. Heynen, B. Morales, M. F. Bear, and A. Kirkwood
Developmental Inhibitory Gate Controls the Relay of Activity to the Superficial Layers of the Visual Cortex
J. Neurosci.,
September 1, 2001;
21(17):
6791 - 6801.
[Abstract]
[Full Text]
[PDF]
|
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X. Jin, P. H. Mathers, G. Szabo, Z. Katarova, and A. Agmon
Vertical Bias in Dendritic Trees of Non-pyramidal Neocortical Neurons Expressing GAD67-GFP In Vitro
Cereb Cortex,
July 1, 2001;
11(7):
666 - 678.
[Abstract]
[Full Text]
[PDF]
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TOP
ABSTRACT
INTRODUCTION
