Prefrontal Microcircuits: Membrane Properties and Excitatory Input of Local, Medium, and Wide Arbor Interneurons

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (55)

Citing Articles via Google Scholar

Google Scholar

Articles by Krimer, L. S.

Articles by Goldman-Rakic, P. S.

Search for Related Content

PubMed

PubMed Citation

Articles by Krimer, L. S.

Articles by Goldman-Rakic, P. S.

Previous Article  |  Next Article

The Journal of Neuroscience, June 1, 2001, 21(11):3788-3796

Prefrontal Microcircuits: Membrane Properties and Excitatory Input of Local, Medium, and Wide Arbor Interneurons
Leonid S. Krimer and Patricia S. Goldman-Rakic
Section of Neurobiology, Yale University School of Medicine, New Haven, Connecticut 06520-8001

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

To elucidate cortical mechanisms involved in higher cortical functions such as working memory, we have examined feedforwardexcitation transmitted by identified pyramidal cells to interneuronswith predominantly horizontal axonal arbors, using dual somaticrecordings in prefrontal cortical slices. Interneurons with local(narrow) axonal arbors, especially chandelier interneurons, exhibitedextremely narrow action potentials and high evoked firing rates,whereas neurons identified with wide arbor axons generated widerspikes and lower evoked firing rates with considerable spike adaptation,resembling that of pyramidal cells. Full reconstruction of differentiallylabeled neuronal pairs revealed that local arbor cells generallyreceived a single but functionally reliable putative synapticinput from the identified pyramidal neuron member of the pair.In contrast, more synapses (two to five) were necessary to depolarizemedium and wide arbor neurons reliably. The number of putativesynapses and the amplitude of the postsynaptic response were remarkablyhighly correlated within each class of local, medium, and widearbor interneurons (r = 0.88, 0.95, and 0.99, respectively). Similarlystrong correlations within these subgroups were also present betweenthe number of putative synapses and variance in the EPSP amplitudes,supporting the validity of our morphological analysis. We concludethat interneurons varying in the span of their axonal arbors andhence in the potential regulation of different numbers of corticalmodules differ also in their excitatory synaptic input and physiologicalproperties. These findings provide insight into the circuit basisof lateral inhibition and functional interactions within and betweencortical columns in the cerebralcortex.

Key words: interneurons; membrane properties; unitary EPSPs; synaptic efficacy; paired recordings; synaptic number; prefrontal cortex

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Local circuit neurons of the cerebral cortex participate in structuring receptive fields of pyramidal cells via inhibitoryGABAergic neurotransmission. In visual cortex they contributeto orientation and direction tuning of excitatory neurons (Sillito,1975; Eysel et al., 1998). Lateral inhibition, including oblique-and cross-orientation inhibition (Kisvarday et al., 1994), hasbeen hypothesized to account for these effects (Sillito, 1984;Eysel, 1992). Recent evidence from this laboratory indicates thatsimilar inhibitory mechanisms operate in the prefrontal cortexto shape the memory fields of neurons that are engaged in workingmemory tasks (Wilson et al., 1994; Rao et al., 1999, 2000).

Another point of interest is the recent evidence that pyramidal neurons project preferentially onto nearby, but not onto distant(>250 µm), interneurons (Elhanany and White, 1990; McGuire etal., 1991; Melchitzky et al., 1998; Muly et al., 1998). As such,it appears that a major mode, perhaps the major mode of intercolumnarinhibition of both pyramidal and nonpyramidal neurons, is vialocal pyramidal-interneuronal circuits. Supporting this organization,GABAergic fast-spiking interneurons recently have been found todischarge only in synchrony with neighboring neurons, indicatingthat local excitatory input to interneurons may be the only inputdriving the inhibitory network in the regulation of rhythmic excitationas well as constraining epileptiform activity (Sanchez-Vives andMcCormick, 2000).

Given the signal importance of inhibition in cortical function, the present study was designed to examine further the intrinsiccircuits in prefrontal cortex, with a focus on the interactionsbetween principal neurons and local circuit neurons in this cortex,which single-unit recording, lesion, and imaging studies haveshown to subserve mnemonicfunctions.

Such interactions have been characterized recently in other cortical areas, using a paired recording technique (Thomson etal., 1995; Buhl et al., 1997; Galarreta and Hestrin, 1998; Tarczy-Hornochet al., 1998; Angulo et al., 1999), and distinct physiologicalproperties of excitatory synapses have been associated with differenttypes of postsynaptic neuron (Reyes et al., 1998). We here examine,in prefrontal cortex, the local excitatory input to three groupsof interneurons with predominantly horizontal axonal arbors: localarbor cells (LACs), medium arbor cells (MACs), and wide arborcells (WACs), similar to those described in primate prefrontalcortex by Lund and Lewis (1993) and in rat by Kawaguchi (1995).Such neurons represent a large population of interneurons in theprefrontal cortex and are likely to play distinct functional rolesbecause of the differential range of influence conveyed by thelength of their axonal arbors. Although LACs (including chandelierinterneurons) with narrow, ~300 µm, axonal arbors may provideinhibitory effects within narrow cortical modules, medium (500µm axonal extent) and especially wide arbor (>1000 µm axonal extent)neurons could influence neighboring modules (Bugbee and Goldman-Rakic,1983; Goldman-Rakic, 1984; Lund and Lewis, 1993; Melchitzky etal., 2001).

Our findings indicate that interneurons differentiated by the span of their horizontal axonal arbors could be distinguishedfurther on the basis of their physiological membrane propertiesas well as on the properties of their local excitatory input.This study also examined the structure-function relationshipsbetween physiological response and excitatory input by full anatomicalreconstruction of virtually every physiologically characterizedpair ofneurons.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation. Twenty connected neuronal pairs were identified in slices of medial prefrontal cortex taken from 1.5- to 4-month-oldferrets. Two of the pairs were excluded from further analysisbecause we were unable to recover in full the axons of their presynapticpyramids in our anatomical reconstructions. However, two additionalsmall arbor neurons and two chandelier cells (ChCs) that wererecorded individually were included in the analysis of morphologicaland membraneproperties.

The animals were anesthetized deeply with sodium pentobarbital and decapitated. The brain was removed quickly and chilledfor a few minutes in ice-cold Ringer's solution. The frontal lobewas separated, and 400 µm sagittal sections were cut through themedial prefrontal region on a DTK-1500E microslicer (Dosaka, Kyoto,Japan). Sections were incubated at 35°C and after at least 1.5hr were submerged in the perfusion chamber at 31-32°C. Extracellularsolution contained (in mM): 126 NaCl, 2.5 KCl, 1.25 NaH₂PO₄, 2CaCl₂, 1 MgSO₄, 26 NaHCO₃, and 10 dextrose, pH 7.4, perfused witha 95%O₂/5%CO₂ gas mixture. Structures were visualized by usinginfrared differential interference contrast video microscopy asdescribed previously (Stuart et al., 1993). Interneurons of laminaeII/III were selected visually on the basis of their lack of anapical dendrite and small soma size (relative to pyramidalcells).

Physiological analysis. Dual whole-cell voltage recordings were used for analysis of pyramidal-to-nonpyramidal monosynapticconnections. Patch electrodes with electrical resistances of 10-12M $Omega$ were filled with a solution containing (in mM): 114 K-gluconate,6 KCl, 0.5 CaCl, 1 EGTA, 4 ATP-Mg, and 10 HEPES, pH-adjusted to7.25 with KOH. Lucifer yellow (0.2%, dipotassium salt; Sigma,St. Louis, MO) was added for morphological identification of interneurons,and 0.5% biocytin (Molecular Probes, Eugene, OR) was used to labelpyramidal cells. Membrane was broken by suction at $>=$ 5 G $Omega$ sealresistance. Both access resistance and capacitance were compensatedon-line. Access resistance was determined from the settings ofthe bridge balance from the current-clamp amplifiers (Markramet al., 1997) and typically was 15-25 M $Omega$ . It was stable duringrecordings, as indicated by low noise (0.11 ± 0.02 mV) and itssmall variance (CV = 18%). The root mean square (rms) noise wasmeasured for 15 neuronal pairs from the baseline within 30 msecbefore EPSP onset. Sweeps contaminated with spontaneous EPSPswere eliminated for all measurements. Pyramidal cells within ~100µm were tested for monosynaptic connections to a given interneuron.They were stimulated with narrow 10-msec-duration rectangularsuprathreshold current pulses (Markram et al., 1997) at 1 Hz;20 trials were averaged on-line to confirm connectivity. Then20-50 single trials were recorded at 0.17-0.25 Hz for furtheroff-line analysis. EPSPs were measured as follows: latencies,from peak of presynaptic spike to the onset of EPSPs; amplitudes,from baseline to peak of EPSPs; rise time, from onset of EPSPsto its peak; and 50% decay, from the peak of EPSPs to its halfvalue. Time constant was calculated from a curve fitting to therepolarization slope of EPSPs and best described as first-orderexponential decay. There was no EPSP run-down over the testedtime range of 8-20 min (n = 4). The method of whole-cell recordingthat was used allowed for low noise data acquisition with reliabledetection of evoked postsynaptic events. There was almost no overlapbetween noise and EPSP amplitudes for all of our recordings (Fig.1), and that enabled accurate detection of the failure incidenceamong the identified synaptic transmissions. Accordingly, therewas no correlation between the percentage of failures and themagnitude of rms noise (coefficient of correlation, 0.08).

View larger version (28K):
[in this window]
[in a new window]
Figure 1. Distribution of amplitudes for noise (on the left) and for EPSPs recorded in postsynaptic interneurons. There is almost no overlap in amplitude distributions between noise and EPSPs for all of the recorded pairs.

To characterize electrical membrane properties of neurons, we applied hyper-and depolarizing rectangular current pulses of500 msec duration in 50 pA increments (Kawaguchi, 1995). Singleaction potentials also were evoked by single 30-msec-durationdepolarizing current pulses. In general, postsynaptic nonpyramidalneurons satisfied the physiological criteria of interneurons (McCormicket al., 1985, Chen et al., 1996). They typically had narrow spikes(0.43 ± 0.07 msec) with amplitudes, on average, of 25 mV smaller(80 ± 7 mV as measured from the baseline) than those of pyramidalcells. Interneurons discharged at 2-36 Hz in response to just-above-thresholdstimulation, with the first spike consistently occurring at thebeginning of the current pulse. Stronger stimulation currentsfurther demonstrated the high firing rates of these cells andthe lack of significant spike adaptation for most of these cells.Interneurons had membrane potentials of $-$ 67 ± 4 mV (measurementswere not compensated for liquid junction potential), input resistancesof 109 ± 29 m $Omega$ , and time constants of 10.5 ± 2.8 msec (the lasttwo parameters were measured on sweeps produced by 50 pA hyperpolarizingpulses). For pyramidal cells the average values were membranepotential, $-$ 69 ± 5 mV; input resistance, 101 ± 45 m $Omega$ ; time constant,26.2 ± 12.2 msec; action potential amplitude, 105 ± 9 mV; andaction potential width, 1.11 ± 0.18 msec. All pyramidal cellsgenerated considerably lower firing frequencies (than interneurons),with prominent spike adaptation in response to 500-msec-depolarizinginjectedcurrents.

Voltages were amplified and filtered at 2 kHz, using two Intracellular Electrometers IE-210 (Warner Instrument, Hamden, CT)operating in bridge balance mode, and acquired on the computerat sampling rates of 10-30 kHz, using DigiData 1200 interfaceand pClamp 6 software program (Axon Instruments, Foster City,CA). In addition to pClamp 6, Axoscope (Axon Instruments), MicrosoftExcel, and Origin 5.0 software programs were used for data analysis.The data are presented in average ± SD values throughout the text.For statistical analysis two-sample Student's t test was usedunless otherwisespecified.

Morphological analysis. After recordings, the pairs were left patched for a total of 1-2 hr for good dye labeling of theirdendritic and axonal arbors. Free-floating slices were fixed incold 4% paraformaldehyde for 72 hr, transferred into anti-freezingsolution (mixture of ethylene glycol and glycerol in 0.1 M phosphatebuffer), and stored at $-$ 79°C. Later they were sectioned into 5× 60 µm sections on the microslicer. Sections were reacted with1% H₂O₂ and placed in blocking serum with 0.5% Triton X-100 at4°C for 12 hr. Then they were incubated in avidin-biotin complex(ABC) for 4 hr at room temperature and, after being rinsed, weretransferred to a solution of anti-Lucifer yellow biotinylatedrabbit IgG (Molecular Probes) for 48 hr. Biocytin-labeled pyramidswere developed by using the black Ni-DAB chromogen. Lucifer yellow-labeledinterneurons were stained golden brown, using a plain diaminobenzidine(DAB) reaction after additional ABC incubation. To avoid extensiveshrinkage in thickness, we dehydrated sections while they werefree-floating.

Neuronal three-dimensional reconstruction and morphometric measurements of dendritic and axonal arbors were made with Neurolucidasoftware (MicroBrightField, Colchester, VT) and an optical set-upas described previously (Krimer et al., 1997). To avoid significantdeterioration of optical resolution deep in the sections, we mountedthem between two coverslips and analyzed them on both sides. Thedouble immunolabeling procedure that was used allowed for clearcolor distinction between pyramidal and nonpyramidal neurons,reliable cell reconstruction, and analysis of putative synapticcontacts (Fig. 2a,b). In fact, the color differentiation was soclear (especially when focusing up and down along the axons andobserving the color of their boutons) that we easily could distinguishputative synapses (black) from multiple autapses on the interneurons(stained brown). In addition, as a conservative measure, we alsotraced axons with putative contacts on interneurons back to theirpyramidal cell origins to further reassure the accuracy of theanalysis. Morphometric analysis for recorded neurons includedmeasurements of soma perimeter, total dendritic and axonal length,and distance from soma to the pia and to the soma of the otherconnected neuron. To classify interneurons accurately, we furthercharacterized their axonal arbors for width, height, area, anddensity of distribution. Pyramidal neurons had distinctive morphologicalfeatures, namely the presence of apical and basal dendrites withnumerous spines. However, the morphology of their dendritic andlocal axonal arbors exhibited substantial variation (see Figs.2, 3). The quantitative measurements were not corrected for tissueshrinkage, which is known to be ~30% for free-floating dehydrationof cortical slices (Krimer et al., 1997).

View larger version (78K):
[in this window]
[in a new window]
Figure 2. Morphological analysis of recorded neuronal pairs. a, Low-power photomicrograph. The presynaptic pyramidal neuron (black) was loaded with biocytin and reacted with NI-DAB; the postsynaptic medium arbor basket neuron (black) was filled with Lucifer yellow and developed with DAB. b, High-power microphotographs depicting en passe and terminal putative synapses established by axons (black) of the presynaptic pyramids on the dendrites (brown) of the postsynaptic interneurons. c, d, Examples of three-dimensional reconstructed neuronal pairs of presynaptic pyramids and postsynaptic interneurons from the group of small interneurons. c, Small arbor basket cell. d, Small chandelier cell. Note that presynaptic pyramids (dendrites are orange, and axons are green) establish only one putative synapse (white circle) on these small postsynaptic interneurons (dendrites are light blue, and axons are darker blue).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Anatomy of interneurons

The three-dimensional reconstructions and morphometric measurements revealed three classes of interneurons that are basedon the size of their soma and width of axonal arbor cells withnarrow or local axonal arbors (LACs), medium arbor cells (MACs),and wide arbor cells (WACs), a classification very similar tothat reported in a previous Golgi analysis of layer III pyramidalneurons in the primate prefrontal cortex (Lund and Lewis, 1993).The soma of LACs were small, and their horizontal axonal arborswere, on average, ~300 µm in width (Fig. 2c, Table 1). Theirlabeled axons consistently had numerous and well developed boutons,many of which contacted unidentified cell bodies and/or proximaldendrites of pyramidal cells as visualized under differentialinterference contrast. Among LAC, the ChC had the narrowest horizontalaxonal span with >100 reconstructed axonal cartridges arrangedin the classical vertical manner known to target the axon initialsegments of an equal number of pyramidal cells (Fig. 2d, Table1) (Williams et al., 1992). The dendrites of LACs were usuallysmooth, relatively linear, and slightly biased vertically withbranching points close to the soma, and that of the chandeliercell had a notably narrow vertical course. However, their highaxonal density in tissue volume was relatively high (0.23 and0.26 µm/µm³), compatible with extensive influence over multiple cells inthe local vicinity.


View this table:
[in this window]
[in a new window]
Table 1. Anatomical and physiological properties of pyramidal to nonpyramidal cell connections

MACs and WACs had significantly larger cell bodies, and their symmetrical axonal arbors covered a wider span of cortical modulesthan those of the LACs, with ~600 and 900 µm symmetrical horizontalaxonal spans, respectively (Table 1, Fig. 3a,c). Although thearea of their axonal distribution was considerably larger thanfor LACs, their axonal density per tissue volume was almost twofoldlower (0.16 vs 0.26 µm/µm³, respectively). This anatomical finding suggests that, althoughMACs and WACs are likely to control wider cortical expanses, theymay have weaker effects on their targets. WACs in particular arein position to influence several cortical modules. Interestingly,their axons made both local and remote arborizations (Fig. 3c).The local plexus was very similar to that of LACs in total axonallength, height, width, and density, whereas their long-range axonsgave off short and rather scarce branches along their trunks.

View larger version (46K):
[in this window]
[in a new window]
Figure 3. Three-dimensional reconstruction of monosynaptically connected neuronal pairs of presynaptic pyramids and postsynaptic interneurons from groups of medium and wide arbor interneurons. a, Medium arbor basket cell. b, Dendrite-targeting cell. c, Wide arbor basket cell. Note that presynaptic pyramids (dendrites are orange, and axons are yellow) establish two and three putative synapses (white circles) on medium and wide arbor basket cells, respectively (dendrites are light blue, and axons are darker blue).

Membrane properties of interneurons

LACs and ChCs, in particular, were the fastest spiking interneurons under study. In line with previous reports (Kawaguchi,1995), LACs generated narrow spikes with widths of 0.42 ± 0.07msec and high firing rates of 40.4 ± 7.47 (Fig. 4). Evoked trainsof action potentials did not show spike adaptation. The membraneproperties of three chandelier cells were also distinct not onlyfrom the rest of interneurons but even from the other LACs (Fig.4). Their firing rates were 42% higher (p < 0.01; Mann-WhitneyU test) and the action potentials were narrower [0.35 ± 0.01 msec;p < 0.04; Mann-Whitney U test) than those of other LACs. The membraneproperties of MACs were very similar to those of LACs. They displayedfast-spiking rates with action potentials and no noticeable adaptationbetween action potentials. However, they tended to generate slightlywider spikes (0.47 ± 0.035) with lower evoked firing rates (33± 6 Hz; Fig. 4) than LACs. WACs had the lowest firing rates (16± 10.6 Hz) and the widest spikes (0.52 ± 0.02 msec) of all nonpyramidalcell classes that were examined. They also displayed considerablespike adaptation (Fig. 4). In fact, their firing pattern was verysimilar to that of pyramidal cells. However, WACs still couldbe distinguished easily from the latter on the basis of theirtwofold narrower spikes. The latter were also ~25 mV smaller inamplitude than the action potentials of pyramidal cells.

View larger version (33K):
[in this window]
[in a new window]
Figure 4. Distinctive membrane properties of the subtypes of postsynaptic interneurons. The consecutive traces (from the bottom to the top) are evoked neuronal responses by current pulse injections of 50 pA increments and 500 msec duration. The chandelier neuron (ChC) displays the highest firing rates, with no spike adaptation. This is followed by the small arbor (SAC) and then by medium arbor (MAC) basket cells. Note that the MAC displays some spike adaptation. The wide arbor basket cell (WAC) has low evoked firing rates and prominent spike adaptation. In fact, these two parameters are almost identical to those of pyramidal cells (PC); hence the WAC does not really fall into the fast-spiking cell classification, as commonly defined. Nevertheless, it is distinguishable from pyramidal cells by its smaller and narrower action potentials, which are characteristic of interneurons.

Local excitatory unitary input to interneurons

Approximately every fourth pyramidal cell that was tested in laminae II/IIIa established monosynaptic connections with aninterneuron within 100 µm of its soma. All of the evoked EPSPshad short latencies of 1.2 ± 0.35 msec. In general, the evokedpostsynaptic response was quite strong, with the amplitude ofthe unitary EPSPs across all pairs averaging 1.3 ± 0.56 mV; 15pairsexhibited EPSPs at or above 1 mV (see Fig. 1, Table 1).Among the latter, eight pairs had EPSP amplitudes between 1.5and 2.5 mV, and some of the individual postsynaptic responsesreached 4 mV. Only five pairs had postsynaptic responses <0.8mV. The EPSPs had fast rise times (1.4 ± 0.40 msec) and shortduration (50% decay time of 7.5 ± 2.65 msec). In all pairs, theevoked EPSPs had a first-order exponential decay of $tau$ = 10.1 ±2.85 msec. Synaptic transmission from the pyramids to interneuronswas remarkably reliable and failed, on average, in 15 ± 19% ofthe trials. Only three recorded pairs demonstrated a high rateof failures, i.e., $>=$ 42% (Table 1).

Pyramidal-to-LAC neurotransmission generally was accomplished via a single synaptic contact and was remarkably reliable. Onlyone putative synapse was found in seven of nine pairs of LACs(see Fig. 2, Table 1). These connections had mean amplitudesof 0.9 mV (Fig. 5) and, with the exception of the ChC, only 11.4± 9.8% of neurotransmission failures. The average variance inEPSP amplitude was relatively low (SD = 0.3 mV). The remainingtwo LAC pairs had two and three putative synaptic connections,respectively. Remarkably, their mean EPSP amplitudes were twofoldlarger (1.95 mV; p < 0.0001) as were their average variances (SD= 0.74 mV; p < 0.00003). The ChC was different from all of theother LACs recorded here in having a high neurotransmission failurerate of 50%.

View larger version (13K):
[in this window]
[in a new window]
Figure 5. Unitary EPSPs recorded in local, medium, and wide arbor basket postsynaptic interneurons. Evoked action potential in presynaptic pyramidal cells (bottom trace) produced monosynaptic EPSPs in postsynaptic cells (top traces). One putative synapse in LAC (this pair is reconstructed in Fig. 2c) generated an average EPSP of 1 mV, as did three synapses in WAC (reconstructed in Fig. 3c). Two synapses in MAC (reconstructed in Fig. 3a) produced an average 1.5 mV EPSP.

Pyramidal-to-MAC unitary connections were multisynaptic (see Figs. 3, 5, Table 1). The number of putative synapses on MACsvaried between two and five, significantly more than on LACs (p< 0.05). These connections, with one exception, were functionallyvery reliable, with 1.9 ± 0.6 mV mean EPSP amplitude and 7.2 ±7.8% neurotransmission failures. Pyramidal-to-WAC unitary connectionswere similar to MACs but had somewhat smaller amplitudes (seeFigs. 3, 5, Table 1). Exceptions to these findings were observedin two cases in which only a single putative synapse could beidentified in the reconstruction of axonal contacts. In both instances(one MAC and one WAC) we identified notably weak (mean amplitudesof 0.5 ± 0.29 and 0.3 ± 0.11 mV, respectively) and unreliable(50 and 42%, respectively) connections. We attribute the unusuallylow amplitude EPSPs and high failure rates in these cases to theloss of synapses duringsectioning.

Number of appositions correlate with synaptic efficacy

The amplitude of the postsynaptic response was correlated strongly with the number of putative synapses within each groupof LACs, MACs, and WACs (r = 0.88, 0.95, and 0.99, respectively).Strong correlations also were observed between the number of putativesynapses and variance in EPSP amplitude within each of these groups(r = 0.89, 0.71, and 0.99, respectively). However, the same numberof synapses produced a stronger response in the group of LACsthan in MACs and especially in WACs. To calculate the postsynapticdepolarization produced by a single contact (unit EPSP), we dividedthe mean unitary EPSP by the number of putative synapses. We founda strong negative correlation (r = $-$ 0.83; p < 0.0001; see alsoFig. 6B) between the soma size of interneurons and the amplitudeof unit EPSPs, indicating that a single synapse has a greaterimpact on LACs than on MACs and especially greater than on WACs.Indeed, one synapse usually produced the same (~1 mV) postsynapticdepolarization in LACs that three to five synapses did in theWACs (see Fig. 5A). This influence of postsynaptic interneuronobviously weakened across the correlation of the groups (r = 0.67;Fig. 6A) as compared with within-groups correlation between thenumber of contacts and strength of response (r = 0.88, 0.95, and0.99 for LACs, MACs, and WACs, respectively).

View larger version (11K):
[in this window]
[in a new window]
Figure 6. Structure-function correlates of intrinsic excitatory neurotransmission in the pyramidal-interneuron circuit. A, A strong positive correlation (r = 0.78) between the number of putative synapses and the strength of the postsynaptic response. B, A strong negative correlation (r = $-$ 0.83) between the unit mean amplitude of EPSPs (calculated as the mean EPSP divided by the number of synapses) and the soma size of the postsynaptic interneurons, which correspond to distinct interneuronal subtypes. Circles, LACs; triangles, MACs; diamonds, WACs.

Interestingly, single connections across the groups had twofold smaller EPSP amplitudes (0.8 vs 1.6 mV, respectively; p <0.0001, one way ANOVA) and twofold lower variability (SD ± 0.3vs SD ± 0.6; p < 0.0001) as compared with multiple connections(Fig. 7).

View larger version (35K):
[in this window]
[in a new window]
Figure 7. Distribution of the EPSP amplitudes in the identified pyramidal-to-interneuron connections. Both the amplitudes and variance for the group with single-contact connections (filled columns) are twofold smaller than for the group of multi-contact connections (patterned columns).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Anatomical and physiological properties of interneurons

There is, as yet, no universally established classification scheme of neocortical interneurons. In the present study we haveanalyzed synaptic transmission between identified pyramidal neuronsand three groups of interneurons in layers II/III of prefrontalcortex that are differentiated by the spread of their axonal arborsand, consequently, by the size of cortical territories and numberof neurons each interneuron has the potential to innervate andinhibit. The width of axonal distribution of an interneuron alsois correlated with the size of its soma. These groups of interneuronsoriginally were described anatomically in the monkey prefrontalcortex, with LACs and WACS expressing parvalbumin immunoreactivityand MACs containing cholecystokinin (Lund and Lewis, 1993). Incontrast, parvalbumin-containing interneurons in the rat havebeen categorized physiologically as a single group of fast-spikingcells. On the basis of these previous findings, we initially expectedthat local, medium, and wide arbor interneurons also would belongto one category of fast-spiking cells. However, the present findingsdemonstrate that each of these morphological groups has distinctphysiological correlates that are based on their firing ratesand spike widths. LACs (including ChCs), MACs, and WACs, respectively,have progressively lower evoked firing rates and wider actionpotentials. Chandelier interneurons occupied one extreme of thisorder, demonstrating the highest evoked firing rates and the narrowestspikes, whereas WACs with the lowest firing rates and the widestaction potentials were at the other extreme. Indeed, the low firingrates of WACs, often with considerable spike adaptation, resembledthe firing pattern of pyramidal neurons, although they still couldbe differentiated from the latter by narrower spikes of loweramplitude. Thus, it appears that fast-spiking interneurons canbe differentiated further both physiologically and morphologicallyand, on this basis, can be predicted to have different roles incortical function yet to be determined.

View larger version (30K):
[in this window]
[in a new window]
Figure 8. Summary diagram of the three types of interneurons and their associated EPSPs that were examined in the present study, illustrating the putative synaptic connections that were observed between pyramidal and interneuron pairs and the presumed targets of the local arbor (LAC), medium arbor (MAC), and wide arbor (WAC) neurons (see Fig. 3 for documentation of the axonal arbors that are illustrated here).

Pyramidal cell innervation of LACs, MACs, and WACs

Feedforward excitation from pyramidal neurons onto interneurons is a well established fact of cortical architecture (Shepherd,1974), although there are more physiological investigations offeedforward inhibition onto principal neurons than the reverse(Eysel, 1992; Gulyas et al., 1993; Buhl et al., 1997; Eysel etal., 1998). However, the nature of inhibitory input on neuronsin the same cortical column (presumably LACs) or in neighboringcortical columns (for MACs and WACs) is highly relevant to thefunction of lateral inhibitory mechanisms controlling neuronalexcitability generally and receptive field conformation specifically.The present study is the first to examine pyramidal-interneuronalinteractions in prefrontal cortex of any species and to correlatephysiological properties within identified anatomical circuits.Here we demonstrate that interneurons with different widths ofhorizontal axonal spread and therefore with presumptive controlover different cortical modules receive a distinctive excitatoryunitary input from local pyramidal cells, among other possiblesources of innervation. LACs were driven reliably by a singlecontact, similar to findings in hippocampal basket interneurons(Gulyas et al., 1993) but contrasting with very unreliable pyramidal-to-burstfiring spiny interneuronal connections in rat somatomotor cortex(Deuchars and Thomson, 1995). The latter may be another exampleof an influence of postsynaptic interneurons on the propertiesof their synaptic input. More contacts (two to five) appear tobe necessary for reliable neurotransmission in MACs and WACs becausetheir efficacy, calculated per single contact, exhibited a progressivedecline. One possible explanation for this decline may be a lowerprobability of neurotransmitter release in multisynaptic versusmonosynaptic connections, as indicated by a twofold higher variancein EPSP amplitudes (SD ± 0.66) with multiple as compared withsingle putative synapses (average SD ± 0.33). Other possibilitiesinclude changes in membrane conductance and/or number and sensitivityof postsynaptic receptors. Clearly, further studies are necessaryto address whether presynaptic or postsynaptic mechanisms areinvolved.

Correlation of morphologically identified contacts, EPSP amplitudes, and type of postsynaptic interneuron

The present study demonstrated that the number of synapses established by presynaptic pyramidal neurons on their postsynaptictargets correlated with the type of postsynaptic interneuron.Single synapse unitary connections generally appeared to be therule for the group of LACs, because only one synapse was foundin seven of nine pairs in the group. In contrast, two to fivesynapses per unitary connection usually were found in the twogroups of MACs and WACs. The study also provides evidence of astrong structure-function correlation, that between the numbersof putative excitatory contacts on identified interneurons andsynaptic efficacy. An important caveat in this study is that appositionsbetween identified terminals and postsynaptic interneurons inthis study were not confirmed at the electron microscopic (EM)level for several reasons. Although such analysis would be ideal,it is not feasible considering the fact that our light microscopicobservation included 39 putative synaptic contacts. Despite thatprecaution, the following arguments make us confident in the numbersof estimated putative synapses. First, almost one-half (9 of 20)of the physiologically connected neuronal pairs had a single putativesynapse, which strongly argues against light microscopic overestimationof contacts. Second, we have used an identical labeling protocolin a previous study and provided EM confirmation of our lightmicroscopic analysis in the four of four contacts that were examined(Krimer et al., 1997). Also, other previous studies (Buhl et al.,1997; Markram et al., 1997) in which light electron microscopiccorrelation was performed similarly have found high (90-100%)agreement between the light microscopic estimation and ultrastructuralanalysis of synaptic contacts. Third, our differential labelingof presynaptic and postsynaptic neurons by two chromogens notonly enabled us to reconstruct neuronal pairs accurately but alsoallowed us to distinguish synapses reliably from autapses. Further,our anatomical estimation is supported strongly by the physiologicaldata, which show a systematic, replicable, and highly significantassociation between putative synaptic number and synaptic efficacyin each subgroup of identified interneuron. Finally, the meanEPSP amplitude and mean variance for the multiple putative synapseconnections were approximately twice as high as those for singleputative synapse connections. This difference was highlysignificant.

Surprisingly, support in the literature for strong correlations between synaptic number and postsynaptic response generallyhas been sparse and weak. In a study similar to ours, Buhl etal. (1997) analyzed five pyramidal-to-interneuronal pairs in catvisual cortex. Three basket cells, one dendrite-targeting cell,and one double bouquet cell represented the postsynaptic interneurons.In these pairs the mean EPSPs of 0.3, 0.4, 1.2, 0.9, and 0.7 mVcorresponded to 1, 2, 2, 4, and 7 synapses, respectively. Thelimited number of observations precluded correlation analysisin that study. This issue also has been addressed in other modelsystems such as the goldfish Mauthner cell (Korn et al., 1986),layer IV stellate (Feldmeyer et al., 1999), and layer V tuftedpyramids of rat somatosensory cortex (Markram et al., 1997), butstrong correlations were not observed. In the goldfish Mauthnercell the number of identified synapses was quite extensive (3-52),yet only a trend correlation was observed and only among the neuronswith small numbers of presynaptic terminals (Korn et al., 1986).It seems distinctly possible that multiple synaptic connectionsmay be associated with a different probability of transmitterrelease, which could obscure any correlation between synapticnumber and postsynaptic response. In support of this supposition,linear summation of mimicked EPSPs has been demonstrated in CA1hippocampal pyramidal neurons when the presynaptic component wasbypassed with local iontophoresis of glutamate (Cash and Yuste,1999). The range of synapses examined in our study was only oneto five, and this could favor the observed strong correlationbetween the number of appositions and EPSP amplitude. In addition,the different membrane properties of layer V pyramidal neurons(Markram et al., 1997), and stellate neurons of layer IV (Feldmeyeret al., 1999) as compared with the nonpyramidal neurons studiedhere also may account for the differences in the strength of correlationsbetween these and our studies. For example, the amplitudes ofboth EPSPs (Stuart and Spruston, 1998) and backpropagated actionpotentials (Stuart and Sakmann, 1994; Spruston et al., 1995) arestrongly attenuated in distal dendrites of pyramidal neurons.In contrast, at least in certain subtypes of interneurons theseparameters are not affected significantly by dendritic location(Chitwood et al., 1999; Martina et al., 2000). In support of this,we did not observe any difference in response between putativesynapses located distally or more proximally on the dendritesofinterneurons.

Implications for working memory circuitry

The present study examined pyramidal-to-nonpyramidal interactions in prefrontal cortex for which the cortical modules in theprimate are composed of neurons with "memory fields." In the primatevisual memory system these neurons actively maintain mnemonictraces of the location of preferred spatial targets and oftenare inhibited in the direction opposite to the preferred target(Funahashi et al., 1989; Wilson et al., 1994; Rao et al., 1999).It has been proposed that an interneuron is a necessary intermediarybetween pyramidal neurons of opposite polarity, a propositionthat entails input to an interneuron from a nearby pyramidal neuronand/or common input to both and an output of the interneuron toa distant pyramidal cell (Goldman-Rakic, 1995). The interneuronswith differential horizontal axonal spans in the present studyare candidates for these intermediary functions. LACs, MACs, orWACs all may share the memory field of an adjacent pyramidal cellby virtue of proximity, common input, and/or axon collaterals.However, the same subgroups are candidates for inhibiting pyramidalcells in progressively more remote columns for which the neuronshave memory fields of adjacent, intermediate, and opponent polarities,respectively. Recent dual-cell extracellular recordings in monkeysperforming a spatial working memory task in this laboratory supportthis hypothesis: adjacent (within 50 µm) pyramidal-nonpyramidalpairs were found to share common specificities (within 60°) forthe location of visual stimuli in the memory fields of the neurons(Constantinidis et al., 1999), whereas such pairs at distances>200 µm from each other had progressively greater disparitiesup to 120° (Rao et al., 1999; Constantinidis et al., 2001). Thepresent in vitro results add a synaptic dimension to this circuitryby revealing that the MACs and WACs are amplified both in numberof pyramidal cell synapses and in their EPSP amplitude, possiblyto compensate for the distance and size of their terminal fields,which presumably mediate cross-directionalinhibition.

  FOOTNOTES

Received Jan. 19, 2001; revised March 13, 2001; accepted March 14, 2001.

This work was supported by National Institutes of Health Grants MH 38546, MH 44866, and MH 63561-01. We express appreciationto Dr. Graham Williams and Dr. Ethan D. Cohen for valuable technicaladvice on the physiological set-up in early stages of this research,to Dr. David McCormick for a generous donation of ferret tissuethat was used in this study, and to Dr. James Howe for valuablecomments on thismanuscript.
Correspondence should be addressed to Patricia S. Goldman-Rakic, Section of Neurobiology, Yale University School of Medicine,P.O. Box 208001, New Haven, CT 065120-8001. E-mail: patricia.goldman-rakic{at}yale.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Angulo MC, Staiger JF, Rossier J, Audinat E (1999) Developmental synaptic changes increase the range of integrative capabilities of an identified excitatory neocortical connection. J Neurosci 19:1566-1576[Abstract/Free Full Text].
Bugbee NM, Goldman-Rakic PS (1983) Columnar organization of corticocortical projections in squirrel and rhesus monkeys: similarity of column width in species differing in cortical volume. J Comp Neurol 220:355-364[ISI][Medline].
Buhl EH, Tamas G, Szilagyi T, Stricker C, Paulsen O, Somogyi P (1997) Effect, number, and location of synapses made by single pyramidal cells onto aspiny interneurons of cat visual cortex. J Physiol (Lond) 500:689-713[ISI][Medline].
Cash S, Yuste R (1999) Linear summation of excitatory inputs by CA1 pyramidal neurons. Neuron 22:383-394[ISI][Medline].
Chen W, Zhang JJ, Hu GY, Wu CP (1996) Electrophysiological and morphological properties of pyramidal and nonpyramidal neurons in the cat motor cortex in vitro. Neuroscience 73:39-55[ISI][Medline].
Chitwood RA, Hubbard A, Jaffe DB (1999) Passive electrotonic properties of rat hippocampal CA3 interneurons. J Physiol (Lond) 515:743-756[Abstract/Free Full Text].
Constantinidis C, Franowicz MN, Goldman-Rakic PS (1999) Multiple electrode analysis of local circuitry in the primate prefrontal cortex during spatial working memory. Soc Neurosci Abstr 25:44.1.
Constantinidis C, Franowicz MN, Goldman-Rakic PS (2001) Coding specificity in cortical microcircuits: a multiple electrode analysis of primate prefrontal cortex. J Neurosci 21:3646-3655[Abstract/Free Full Text].
Deuchars J, Thomson AM (1995) Innervation of burst firing spiny interneurons by pyramidal cells in deep layers of rat somatomotor cortex: paired intracellular recordings with biocytin filling. Neuroscience 69:739-755[ISI][Medline].
Elhanany E, White EL (1990) Intrinsic circuitry: synapses involving the local axon collaterals of corticocortical projection neurons in the mouse primary somatosensory cortex. J Comp Neurol 291:43-54[ISI][Medline].
Eysel UT (1992) Lateral inhibitory interactions in areas 17 and 18 of the cat visual cortex. Prog Brain Res 90:407-422[ISI][Medline].
Eysel UT, Shevelev IA, Lazareva NA, Sharaev GA (1998) Orientation tuning and receptive field structure in cat striate neurons during local blockade of intracortical inhibition. Neuroscience 84:25-36[ISI][Medline].
Feldmeyer D, Egger V, Lubke J, Sakmann B (1999) Reliable synaptic connections between pairs of excitatory layer 4 neurones within a single "barrel" of developing rat somatosensory cortex. J Physiol (Lond) 521:169-190[Abstract/Free Full Text].
Funahashi S, Bruce CJ, Goldman-Rakic PS (1989) Mnemonic coding of visual space in the monkey's dorsolateral prefrontal cortex. J Neurophysiol 61:331-349[Abstract/Free Full Text].
Galarreta M, Hestrin S (1998) Frequency-dependent synaptic depression and the balance of excitation and inhibition in the neocortex. Nat Neurosci 1:587-594[ISI][Medline].
Goldman-Rakic PS (1984) Modular organization of prefrontal cortex. Trends Neurosci 7:419-424[ISI].
Goldman-Rakic PS (1995) Cellular basis of working memory. Neuron 14:477-485[ISI][Medline].
Gulyas AI, Miles R, Sik A, Toth K, Tamamaki N, Freund TF (1993) Hippocampal pyramidal cells excite inhibitory neurons through a single release site. Nature 366:683-687[Medline].
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].
Kisvarday ZF, Kim DS, Eysel UT, Bonhoeffer T (1994) Relationship between lateral inhibitory connections and the topography of the orientation map in cat visual cortex. Eur J Neurosci 6:1619-1632[ISI][Medline].
Korn H, Faber DS, Triller A (1986) Probabilistic determination of synaptic strength. J Neurophysiol 55:402-421[Abstract/Free Full Text].
Krimer LS, Jakab RL, Goldman-Rakic PS (1997) Quantitative three-dimensional analysis of the catecholaminergic innervation of identified neurons in the macaque prefrontal cortex. J Neurosci 17:7450-7461[Abstract/Free Full Text].
Lund JS, Lewis DA (1993) Local circuit neurons of developing and mature macaque prefrontal cortex: Golgi and immunocytochemical characteristics. J Comp Neurol 328:282-312[ISI][Medline].
Markram H, Lubke J, Frotscher M, Roth A, Sakmann B (1997) Physiology and anatomy of synaptic connections between thick tufted pyramidal neurons in the developing rat neocortex. J Physiol (Lond) 500:409-440[ISI][Medline].
Martina M, Vida I, Jonas P (2000) Distal initiation and active propagation of action potentials in interneuron dendrites. Science 287:295-300[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].
McGuire BA, Gilbert CD, Rivlin PK, Wiesel TN (1991) Targets of horizontal connections in macaque primary visual cortex. J Comp Neurol 305:370-392[ISI][Medline].
Melchitzky DS, Sesack SR, Pucak ML, Lewis DA (1998) Synaptic targets of pyramidal neurons providing intrinsic horizontal connections in monkey prefrontal cortex. J Comp Neurol 390:211-224[ISI][Medline].
Melchitzky DS, Gonzalez-Burgos G, Barrionuevo G, Lewis DA (2001) Synaptic targets of the intrinsic axon collaterals of supragranular pyramidal neurons in monkey prefrontal cortex. J Comp Neurol 430:209-221[ISI][Medline].
Muly 3rd EC, Szigeti K, Goldman-Rakic PS (1998) D1 receptor in interneurons of macaque prefrontal cortex: distribution and subcellular localization. J Neurosci 18:10553-10565[Abstract/Free Full Text].
Rao SG, Williams GV, Goldman-Rakic PS (1999) Isodirectional tuning of adjacent interneurons and pyramidal cells during working memory: evidence for microcolumnar organization in PFC. J Neurophysiol 81:1903-1916[Abstract/Free Full Text].
Rao SG, Williams GV, Goldman-Rakic PS (2000) Destruction and creation of spatial tuning by disinhibition: GABA_A blockade of prefrontal cortical neurons engaged by working memory. J Neurosci 20:485-494[Abstract/Free Full Text].
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[ISI][Medline].
Sanchez-Vives MV, McCormick DA (2000) Cellular and network mechanisms of rhythmic recurrent activity in neocortex. Nat Neurosci 10:1027-1034.
Shepherd G (1974) In: The synaptic organization of the brain: an introduction. New York: Oxford UP.
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 (1984) Functional considerations of the operation of GABAergic inhibitory processes in the visual cortex. In: Cerebral cortex (Jones EG, Peters A, eds), pp 91-117. New York: Plenum.
Spruston N, Schiller Y, Stuart G, Sakmann B (1995) Activity-dependent action potential invasion and calcium influx into hippocampal CA1 dendrites. Science 268:297-300[Abstract/Free Full Text].
Stuart GJ, Sakmann B (1994) Active propagation of somatic action potentials into neocortical pyramidal cell dendrites. Nature 367:69-72[Medline].
Stuart GJ, Spruston N (1998) Determinants of voltage attenuation in neocortical pyramidal neuron dendrites. J Neurosci 18:3501-3510[Abstract/Free Full Text].
Stuart GJ, Dodt HU, Sakmann B (1993) Patch-clamp recordings from the soma and dendrites of neurons in brain slices using infrared video microscopy. Pfl $int$ gers Arch 423:511-518[ISI][Medline].
Tarczy-Hornoch K, Martin KA, Jack JJ, Stratford KJ (1998) Synaptic interactions between smooth and spiny neurons in layer 4 of cat visual cortex in vitro. J Physiol (Lond) 508:351-363[Abstract/Free Full Text].
Thomson AM, West DC, Deuchars J (1995) Properties of single axon excitatory postsynaptic potentials elicited in spiny interneurons by action potentials in pyramidal neurons in slices of rat neocortex. Neuroscience 69:727-738[ISI][Medline].
Williams SM, Goldman-Rakic PS, Leranth C (1992) The synaptology of parvalbumin-immunoreactive neurons in the primate prefrontal cortex. J Comp Neurol 320:353-369[ISI][Medline].
Wilson FA, O'Scalaidhe SP, Goldman-Rakic PS (1994) Functional synergism between putative $gamma$ -aminobutyrate-containing neurons and pyramidal neurons in prefrontal cortex. Proc Natl Acad Sci USA 91:4009-4013[Abstract/Free Full Text].

Copyright © 2001 Society for Neuroscience 0270-6474/01/21113788-09$05.00/0

This article has been cited by other articles:

O. Hoshino
Enhanced sound perception by widespread-onset neuronal responses in auditory cortex.
Neural Comput., December 1, 2007; 19(12): 3310 - 3334.
[Abstract] [Full Text] [PDF]

M. Inda, J DeFelipe, and A Munoz
The Distribution of Chandelier Cell Axon Terminals that Express the GABA Plasma Membrane Transporter GAT-1 in the Human Neocortex
Cereb Cortex, September 1, 2007; 17(9): 2060 - 2071.
[Abstract] [Full Text] [PDF]

M Medalla, P Lera, M Feinberg, and H Barbas
Specificity in Inhibitory Systems Associated with Prefrontal Pathways to Temporal Cortex in Primates
Cereb Cortex, September 1, 2007; 17(suppl_1): i136 - i150.
[Abstract] [Full Text] [PDF]

J. E. Crandall, D. M. McCarthy, K. Y. Araki, J. R. Sims, J.-Q. Ren, and P. G. Bhide
Dopamine Receptor Activation Modulates GABA Neuron Migration from the Basal Forebrain to the Cerebral Cortex
J. Neurosci., April 4, 2007; 27(14): 3813 - 3822.
[Abstract] [Full Text] [PDF]

W. van Drongelen, H. Koch, F. P. Elsen, H. C. Lee, A. Mrejeru, E. Doren, C. J. Marcuccilli, M. Hereld, R. L. Stevens, and J.-M. Ramirez
Role of Persistent Sodium Current in Bursting Activity of Mouse Neocortical Networks In Vitro
J Neurophysiol, November 1, 2006; 96(5): 2564 - 2577.
[Abstract] [Full Text] [PDF]

N.V. Povysheva, G. Gonzalez-Burgos, A.V. Zaitsev, S. Kroner, G. Barrionuevo, D.A. Lewis, and L.S. Krimer
Properties of Excitatory Synaptic Responses in Fast-spiking Interneurons and Pyramidal Cells from Monkey and Rat Prefrontal Cortex
Cereb Cortex, April 1, 2006; 16(4): 541 - 552.
[Abstract] [Full Text] [PDF]

Q. Xu, C. P. Wonders, and S. A. Anderson
Sonic hedgehog maintains the identity of cortical interneuron progenitors in the ventral telencephalon
Development, November 15, 2005; 132(22): 4987 - 4998.
[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]