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NEUROSCIENCE |
1 Abteilung Zellphysiologie, Max-Planck-Institut für medizinische Forschung, Jahnstr. 29, D-69120 Heidelberg, Germany
2 Institut für Neurowissenschaften und Biophysik-Medizin, Forschungszentrum Jülich, D-52425 Jülich, Germany
3 Institut für Anatomie und Zellbiologie der Albert-Ludwigs-Universität Freiburg, Albertstraße 17, D-79104 Freiburg i.Br, Germany
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Abstract |
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(Received 10 January 2006;
accepted after revision 21 June 2006;
first published online 22 June 2006)
Corresponding author D. Feldmeyer: Institut für Neurowissenschaften und Biophysik, AG Zelluläre Neurobiologie-Medizin, Forschungszentrum Jülich GmbH, Leo-Brandt-Straße, D-52425 Jülich, Germany. Email: d.feldmeyer{at}fz-juelich.de
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Introduction |
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Previously we have characterized in vivo the properties of L4 and L2/3 neurones (Brecht & Sakmann, 2002; Brecht et al. 2003) and in vitro the synaptic connections between L4 and L2/3 neurones (Feldmeyer et al. 2002). To characterize possible anatomical and functional determinants of the dynamic borders of the cortical (whisker deflection) maps in layer 2/3 we have examined both efficacy and morphology of individual synaptic connections between ‘barrel-related’ (i.e. intracolumnar) L2/3 pyramidal cells. Specifically, we measured latency, time course, amplitude and amplitude variability of unitary EPSPs in paired recordings from L2/3 pyramidal cells. Furthermore, we determined the number of synaptic contacts and their dendritic location within the ‘innervation domain’ of L2/3 pyramidal cells.
The present functional and morphometric analysis of L2/3-to-L2/3 unitary connections is part of an effort to delineate the factors generating the wave of excitation streaming through the different layers of a cortical column when a single whisker is briefly deflected. In conjunction with the previously reported characterization of sub- and suprathreshold responses of L4 neurones in vivo and the sub- and suprathreshold responses of L2/3 neurones we can now provide estimates of the determinants of sparse AP coding of a sensory stimulus in the L2/3 network of a PW column.
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Methods |
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All experimental procedures were carried out according to the animal welfare guidelines of the Max-Planck Gesellschaft. Wistar rats (17–23 days old) were anaesthetized with halothane and decapitated, and slices of somatosensory cortex were cut in cold extracellular solution using a vibrating microslicer (DTK-1000, Dosaka Co. Ltd, Kyoto, Japan). In order to obtain slices in which connections along barrel rows were largely maintained, we used a modified version of the method described by Agmon & Connors (1991). The brain was removed from the skull and placed on a ramp with a 10 deg slope with the anterior face downhill. The midline was adjusted so that it was parallel to the walls of the ramp. Subsequently, a vertical cut at an angle of 45 deg to the midline was made. The tissue rostral to the cut was discarded and the brain was glued with the cut face downward onto the chilled stage of the slicer. Three to four 
0.8–1.0 mm thick slices were cut and discarded. The remaining tissue was cut at slow speed and high vibration frequency into 300–400 µm thick ‘semicoronal’ slices each containing about one barrel row. Before recording, slices were incubated at room temperature (22–24°C) in an extracellular solution containing 1 mM CaCl2 and 4 mM MgCl2 to reduce overall synaptic activity and block NMDA receptors.
Solutions
Slices were continuously superfused with an extracellular solution containing (mM): 125 NaCl, 2.5 KCl, 25 glucose, 25 NaHCO3, 1.25 NaH2PO4, 2 CaCl2 and 1 MgCl2 bubbled with 95% O2 and 5% CO2. The pipette (intracellular) solution was based on K-gluconate and had a composition as follows: (mM) 105 K-gluconate, 30 KCl, 10 Hepes, 10 phosphocreatine, 4 ATP-Mg, 0.3 GTP (adjusted to pH 7.3 with KOH). The osmolarity of these solutions was 300 mosmol l–1. Biocytin (Sigma, Munich, Germany) at a concentration of 3 mg ml–1 was routinely added to the internal solution and cells were filled during 1–2 h of recording. For cell-attached stimulation (see below) we used a modified version of this solution containing (mM): 105 Na-gluconate, 30 NaCl, 10 Hepes, 10 phosphocreatine, 4 ATP-Mg, 0.3 GTP (adjusted to pH 7.3 with NaOH).
Identification of synaptically connected neurones in the barrel cortex
Slices were placed in the recording chamber under an upright microscope (Nikon, Düsseldorf, Germany; fitted with x4 plan/0.10 NA and x60-W/1.20 objectives) with the pial surface pointing forward and the hippocampus to the left so that the L2/3 axons pointed into the slice. The barrel field was visualized at low magnification under bright-field illumination and can be identified in layer 4 as narrow dark stripes with evenly spaced, light ‘hollows’ (Agmon & Connors, 1991; Feldmeyer et al. 1999). Barrel structures were present in four to five slices but continuous rows of barrels (B, C, D rows) were visible only in two to three slices just above the fimbria-fornix and the lateral ventricle. Individual L2/3 pyramidal cells down to 170 µm depth in the slice were identified at x60 magnification under infrared differential interference contrast (IR-DIC) optics using a narrow bandwidth infrared filter to allow patching of neurones deep in the slice. This was necessary in order to obtain intact axonal arbours and simultaneously retain the barrel structure. After the electrophysiological recordings (see below) the slice was photographed at low power with the electrodes in place to obtain an image of the pre- and postsynaptic neurones and their location relative to the barrel structure in layer 4 (see online Supplemental material, Supplemental Fig. 1A–C).
Electrophysiological recordings
Whole-cell voltage recordings from postsynaptic neurones were made using patch pipettes of 3.5–6 M
resistance pulled of thick borosilicate glass capillaries (outer diameter: 2.0 mm; inner diameter: 0.5 mm; F. Hilgenberg, Malsfeld, Germany). Searching for synaptic connections was performed in the loose seal configuration using a ‘searching’ patch pipette of 5–8 M resistance (Feldmeyer et al. 1999). After establishing a loose seal (i.e. RSeal < 1 G) on a potential presynaptic L2/3 pyramidal cell, the command potential was set to about –60 mV in current clamp mode. An AP was elicited by applying a 5 ms current pulse (0.2–2 nA). When an AP was elicited, this was in most cases visible as a small deflection on the voltage trace. In contrast to L4 spiny neurones, significantly higher stimulation intensities were necessary to evoke APs. When this loose-seal stimulation resulted in EPSPs in the postsynaptic L2/3 pyramidal cell at short latency (i.e. within 5 ms), the ‘searching’ pipette was withdrawn. The presynaptic cell was then re-patched with a new recording pipette (3.5–6 M) filled with a biocytin-containing intracellular solution, and APs were elicited in the whole-cell (current clamp) mode. Occasionally cell-attached stimulation of the presynaptic neurone was also performed throughout the entire recording (rather than using the whole-cell configuration). In three cells where this was tested no difference in the recorded EPSP amplitude was found when the presynaptic neurone was stimulated initially in cell-attached and subsequently in whole-cell mode.
Somatic whole-cell recordings were performed at 34–36°C. Signals were amplified using an Axopatch 200B in combination with an Axoclamp 2B (Axon Instruments, Union City, CA, USA), for current clamp recordings filtered at 1–3 kHz and sampled at 2–10 kHz and for voltage clamp recordings filtered at 5 kHz and sampled at 10 kHz using the program ‘Pulse’ (v. 8.54, HEKA Elektronik, Lambrecht, Germany). Membrane potential fluctuations during current clamp recordings were 5 mV (peak to peak). Cell pairs in which a clear drift in the membrane potential was observed were omitted from the analysis. Acquired data were stored on the hard disk of a Macintosh computer for off-line analysis (Igor, Wavemetrics, Lake Oswego, OR, USA).
Data analysis
EPSP amplitude, latency and kinetics were determined as previously described (Feldmeyer et al. 1999). In order to account for the extra-variance that resulted from membrane potential fluctuations, EPSP amplitudes were normalized to the mean membrane potential during the recording, assuming a linear current–voltage relationship and a near-zero reversal potential. This resulted in a slight reduction of the standard deviation of the EPSP amplitude and thus in a reduced coefficient of variation.
All recordings were inspected visually; failures were defined as events with amplitudes less than 1.5x the S.D. of the noise. In order to verify that small responses were not misclassified as failures due to a bad signal-to-noise ratio, failures were averaged in experiments with a high failure rate (> 10%, n = 3 out of 35). In all of these experiments the failure average was a flat line indicating that misclassification of records was negligible.
Histological procedures
Following recording, slices were fixed at 4°C for at least 24 h in 100 mM phosphate-buffered saline (PBS, pH 7.4), containing either 4% paraformaldehyde or 1% paraformaldehyde and 2.5% glutaraldehyde. Slices containing biocytin-filled neurones were processed using a modified protocol previously described (Lübke et al. 2000). For light microscopy they were incubated overnight in PBS–avidin-biotinylated horseradish peroxidase (ABC-Elite, Camon, Wiesbaden, Germany) containing 0.1% Triton X-100. Slices were then reacted using 3,3-diaminobenzidine (DAB) as a chromogen under light microscopic control until dendritic and axonal arborizations were clearly visible. Slices were then briefly postfixed in 0.1% OsO4 (1–3 min). After several rinses in 100 mM PBS they were mounted on slides, embedded in Moviol (Hoechst AG, Frankfurt, Germany) and enclosed with a coverslip. For electron microscopy, slices were cryo-protected in PBS-buffered sucrose, freeze–thawed in liquid nitrogen and then incubated overnight in the ABC solution at 4°C. After the DAB reaction they were postfixed in 0.5% OsO4 (30–45 min), then dehydrated through an ascending series of ethanol and finally flat-embedded in epoxy resin (Durcopan, Fluka AG, Germany) using a standard electron microscopic embedding protocol. Electron microscopy (EM) was carried out on one pair to confirm putative light microscopically identified synaptic contacts (Feldmeyer et al. 2002). Serial ultrathin sections through the dendritic and axonal domain were cut with an ultramicrotome (Leitz UItracut, Hamburg, Germany) and analysed for synaptic contacts using a Zeiss EM 10 electron microscope (Zeiss, Oberkochen, Germany).
Morphological reconstructions of biocytin-filled synaptically coupled neurones
Biocytin-labelled pairs of neurones were examined under the light microscope at high magnification to identify putative synaptic contacts. Representative pairs were photographed at low magnification to document dendritic and axonal arborization; potential synaptic contacts were identified as close appositions of a synaptic bouton and the postsynaptic dendrite in the same focal plane at a final magnification of x1200 (x100 objective and x12 eyepiece; Fig. 4). Subsequently, biocytin-labelled pairs of neurones were reconstructed with the Neurolucida software (MicroBrightfield, Colchester, VT, USA) using an Olympus BX50 microscope (Olympus, Hamburg, Germany) at a final magnification of x780 to x1200. During the reconstruction bouton counts were made on both deep and superficial axonal collaterals in order to determine their bouton density; the total axonal length of a neurone as well as its length within a barrel column was measured using Neuroexplorer software (MicroBrightfield, Colchester VT, USA). Furthermore, these reconstructions provided the basis for the quantitative morphological analysis of the location of the somata within the slice and the number and the dendritic location of putative synaptic contacts. For all data, means ± S.D. are given. In addition, the length of the apical dendrite, the apical tuft (defined as the part of the apical tuft following the bifurcation of the first-order apical dendrite) and the number of nodes in the apical tuft were determined. Data were not corrected for shrinkage.
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Two-dimensional (2D) maps of axonal and dendritic ‘length density’ were constructed using the computerized 3D reconstructions (for details see Lübke et al. 2003). The length of all axonal and dendritic branches was projected in the 2D plane and measured in a 50 µm x 50 µm Cartesian grid, yielding a raw density map. For alignment of these maps with respect to the barrel centre, barrel borders were identified in the low power (x 4 objective) bright-field micrographs made from the acute brain slice (Lübke et al. 2000, 2003; Feldmeyer et al. 2002). Spatial low-pass filtering of these maps was performed by 2D convolution with a Gaussian kernel (
= 50 µm) and continuous 2D density functions were constructed using bicubic interpolation in Mathematica 4.1 (Wolfram Research, Champaign, IL, USA). The axonal and the dendritic ‘length density’ maps thus obtained were then multiplied in order to calculate the predicted ‘innervation domain’ between pairs of L2/3 pyramidal cells (Lübke et al. 2003).
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Results |
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Functional properties of synapses between L2/3 pyramidal cell pairs
To characterize the connections between L2/3 pyramidal cells functionally, unitary EPSPs in pyramidal cells were analysed by measuring their latency, rise time, peak amplitude and decay time course in detail. Unitary EPSPs were elicited at a frequency of 0.033–0.05 Hz (every 20–30 s). Higher stimulation frequencies resulted in a rapid decrease in the unitary EPSP amplitude. However, when returning to lower stimulation rates, the EPSP amplitude recovered.
As for synaptically coupled pairs between L4 spiny neurones and L2/3 pyramidal cells (and in contrast to pairs between spiny neurones in layer 4; Feldmeyer et al. 1999), pairs between layer 2/3 pyramidal cells showed a relatively low spontaneous synaptic activity (Feldmeyer et al. 2002) which facilitated the analysis of EPSPs and the detection of small EPSPs.
EPSP latency and time course. Figure 1A shows a presynaptic AP and an evoked unitary EPSP in a pre- and postsynaptic L2/3 pyramidal cell, respectively. The latency between the peak of the AP and the unitary EPSP at an individual L2/3–L2/3 synaptic connection showed little variation (at most twofold) and latency histograms were narrow and showed a single peak (Fig. 1B). They are thus similar to the connection between L4 spiny neurones and L2/3 pyramidal cells (Feldmeyer et al. 2002). The data shown in Fig. 1C indicate that the average latency of EPSPs at synapses between L2/3 pyramidal cells ranged from 0.6 to 1.9 ms for individual connections and was on average 1.1 ± 0.4 (n = 21; temperature 35–37°C), indicating that the postsynaptic neurone is rapidly recruited.
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Voltage clamp recordings from synaptically coupled L2/3 pyramidal cells were performed to study the properties of the synaptic currents that mediated the EPSPs at the L2/3-L2/3 pyramidal cell synapse. When using 70–80% series resistance compensation, mean EPSC amplitudes varying from 6 to 111 pA were recorded; the average between pairs was 58 ± 35 pA (n = 7). The mean EPSC rise time was 0.35 ± 0.16 ms and the mean decay time constant 3.7 ± 1.2 ms (see Supplemental Online Material, Supplemental Fig. 3).
As for other synaptic connections (e.g. Feldmeyer et al. 2002), the decay time constant of the EPSP was significantly longer than that of the EPSC measured at the soma in the same neurone (18.3 ms versus 3.7 ms; P < 0.001). The EPSP time course is likely to be shaped to a considerable degree by the membrane time constant of the postsynaptic L2/3 pyramidal cell (which is 10.9 ± 2.4 ms; n = 35). The EPSP decay time constant was significantly longer (P < 0.0001) than the membrane time constant. Therefore, dendritic filtering may contribute to its slow time course.
Reliability of synaptic transmission. Intralaminar synaptic transmission between pairs of L2/3 pyramidal cells is reliable (Fig. 2) as observed for other intracortical connections (Stratford et al. 1996; Feldmeyer et al. 1999, 2002). Seventy-five per cent of the connections (n = 21 out of 28 analysed) showed virtually no failures (i.e. less than 2%) and only in four pairs was the percentage of failures higher than 10%. On average, the failure rate of the L2/3–L2/3 connections was 3.2 ± 7.8%.
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As described for layer 5B pyramidal cell pairs (Markram et al. 1997), for L4 spiny neurone pairs and for L4-to-L2/3 pairs (Feldmeyer et al. 1999, 2002), the C.V. was inversely related to the amplitude of the unitary EPSP. In simple binomial models of synaptic transmission this is to be expected when the unitary EPSP amplitude is primarily determined by the release probability (pr). For the L2/3–L2/3 connection, binomial release with varying quantal content but similar release probabilities have recently been demonstrated by Koester & Johnston (2005).
Calculations of limiting curves assuming binomial release with C.V.
=
[(1 –
pr)/(nbpr)] and pr
=
V/(nbqs), and fixed values for the number of release sites (nb) and the quantal amplitude (qS) were not entirely satisfactory, since EPSP amplitudes larger than 2.0 mV were not included. To obtain limits for nb and qS, we assumed that nb was 3 (i.e. close to the mean number of putative synaptic contacts as determined by light microscopical examination). The two limiting curves in Fig. 2C were calculated for qS
= 0.05 and 0.70 mV. The range of quantal EPSP amplitudes is smaller for intralaminar connection between L2/3 pyramidal cells than for the L4-to-L4 and L5-to-L5 connections in layer 5B (Markram et al. 1997; Feldmeyer et al. 1999; Feldmeyer & Sakmann, 2000) but larger than that observed for the interlaminar L4-to-L2/3 connection (Feldmeyer et al. 2002).
Paired pulse behaviour and EPSP summation. To test the frequency dependence of synaptic transmission between pairs of synaptically connected L2/3 pyramidal cells, we recorded bursts of five unitary EPSPs at various frequencies (corresponding to interstimulus intervals of 10, 20, 50, 100, 200 ms; n = 5). Figure 3A shows that EPSP trains in a L2/3 pyramidal cell depressed at most burst frequencies tested. Interestingly, facilitation occurred occasionally at higher burst frequencies. The EPSP amplitude ratio (i.e. the ratio of the 2nd, 3rd, 4th and 5th EPSP relative to the 1st EPSP) is plotted in Fig. 3B. For the 2nd EPSP the depression was already 0.61 ± 0.41 and 0.73 ± 0.23 for the 10 ms and 50 ms interstimulus interval) and became progressively larger for successive EPSPs in the train, being particularly strong for the 5th EPSP in the train (0.23 ± 0.04 and 0.55 ± 0.20 for the 10 ms and 50 ms interstimulus interval).
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Of the synaptically coupled pairs of L2/3 pyramidal cells, 11 (i.e. 22 neurones) were selected for further quantitative morphological analysis. About one-third of these neurones (n = 8) were in the lower half of layer 2/3 while the rest (n = 14) were located in the upper half of layer 2/3. A clear correlation between apical dendritic length of L2/3 pyramidal cells, the length of dendritic collaterals in the apical tuft and the number of nodes in the tuft was revealed using a Spearman rank order test, with correlation coefficient (rs) of 0.708 and 0.765, respectively. Pyramidal cells in the lower half of layer 2/3 have long apical dendrites (up to 440 µm long; mean 278 ± 89 µm) before bifurcating close to layer 1 and forming only comparatively small apical tufts with a dendritic length of 1033 ± 552 µm and 7.0 ± 4.1 bifurcating nodes (Fig. 5A, Neurolucida reconstruction). In contrast, pyramidal cells in the upper half of layer 2/3 display a relatively short apical dendrite (10–140 µm; average 79.8 ± 39.1 µm) that bifurcates in a terminal tuft with a significantly longer dendritic length of 1863 ± 628 µm (P = 0.002, unpaired, two-tailed t test) and significantly more bifurcating nodes (17.2 ± 7.4; P = 0.0005, unpaired, two-tailed t test) (Fig. 4A, halftone image; Fig. 5B, Neurolucida reconstruction). In addition, the axonal collaterals of the former pyramidal cells appear to ascend to the upper portion of layer 2/3, in contrast to the more horizontal collaterals formed by the more superficial pyramidal cells (Fig. 5; cf. Lübke et al. 2003). The total axonal length and that within the supragranular layer were statistically different for deep and superficial pyramidal cells, with 22095 ± 4884 µm (n = 10 pyramidal cells) versus 12931 ± 2857 µm (n = 4; P = 0.026) and 12226 ± 3336 µm versus 6911 ± 2772 µm, respectively (P = 0.039); however, their axonal length within a barrel column did not differ significantly (total length: 11329 ± 2585 µm versus 7823 ± 1811 µm; 6414 ± 1715 µm versus 4164 ± 1183 µm; P > 0.05).
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The dendritic location and distance of synaptic contacts from the soma were measured from the Neurolucida reconstructions of dendritic and axonal profiles. The insets in Fig. 5A and B illustrate the location of the three light microscopically identified synaptic contacts, identified for both pairs of neurones at the light microscopic level. Only the dendritic configuration of the target cell (white) is illustrated together with the location of the putative synaptic contacts (light blue squares). In the two cell pairs shown here all synaptic contacts were found exclusively on second- to fourth-order basal dendrites.
For eight reconstructed L2/3 pyramidal cell pairs, the mean number of synaptic contacts was 2.8 ± 0.7 with a minimum of two and a maximum of four (Fig. 6A, inset). Synaptic contacts were located between 18 and 170 µm from the soma with an average distance of 91 ± 47 µm (Fig. 6A). The vast majority (95%) was located on basal dendrites; only a small fraction (5%) was located on apical oblique dendrites; no synaptic contacts were found in the terminal tuft dendrites (see Table 1).
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Axonal ‘projection’ fields, dendritic ‘reception’ fields and synapse locations
Overlap of ‘projection’ and ‘reception’ fields in the L2/3-to-L2/3 pyramidal cell pairs. When all reconstructions of L2/3 pyramidal cell pairs (without obvious truncations in the axonal arbour down to layer 5; n = 8) are superimposed and aligned with respect to the barrel centre (Fig 7A and B) it is clearly evident that within a barrel column the ‘projection’ field of a presynaptic L2/3 axon overlaps to a very large extent with the dendritic ‘reception’ field of the postsynaptic L2/3 pyramidal cell. To quantify this overlap the axonal length of the presynaptic pyramidal cell axon was measured using a 50 µm x 50 µm grid superimposed on 2D projections of 3D reconstructions of the cell pairs (see Lübke et al. 2003). We then constructed a 2D map of the axonal ‘length density’ of L2/3 axons using bicubic interpolation of the original grid points yielding an ‘average’ axonal projection of the presynaptic L2/3 pyramidal cells. The reference point for alignment of the reconstructions was either the centre of the barrel (Fig. 7C1), or the soma of the postsynaptic L2/3 pyramidal cell (Fig. 7D1). The map of the L2/3 axonal ‘length density’ clearly shows that the axon of the presynaptic L2/3 pyramidal cell projects widely into neighbouring barrel columns (Fig. 7C1 and D1) as was reported in previous in vitro and in vivo studies (Gottlieb & Keller, 1997; Brecht et al. 2003). Comparing the outline of the average barrel column to the contour line including 80% of the presynaptic L2/3 axonal ‘length density’ shows that its density map includes at least the two neighbouring barrel columns (i.e. at least one on each side) both within layer 2/3 as well as in layers 5 and 6. In layer 2/3 the width of the 2D map is somewhat larger than in layers 5 and 6 (cf. Fig. 7C1 and D1; Table 2). In contrast, there is virtually no lateral projection of the L2/3 pyramidal cell axonal domain in layer 4 (cf. Lübke et al. 2003). In supragranular layers the total axonal length of a single pyramidal cell is on average 8715 ± 3638 µm of which 4704 ± 1924 µm is within the barrel column (cf. Fig. 8A and B). However, the total axonal length in particular that outside the ‘home’ barrel column is likely to be underestimated.
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Innervation domain and location of synaptic contacts.
We then calculated the predicted innervation domain by multiplying the axonal ‘length density’ and the dendritic ‘length density’ assuming that synaptic connections between axons and dendrites in a given region are formed by a random encounter (Fig. 7C3 and D3). The outline of this predicted innervation domain is limited by the extent of the dendritic arborization of the postsynaptic neurone. The sharp delineation of this innervation domain of L2/3 pyramidal cells is particularly clear when presynaptic axonal and postsynaptic dendritic length maps are normalized with respect to the somata of the postsynaptic L2/3 pyramidal cells. The 2D projected dimensions of the innervation domain are about 233 µm (horizontal) and 264 µm (vertical; see Table 2). The axonal arbours of the presynaptic L2/3 pyramidal cells predominantly overlap with the basal dendritic field of the postsynaptic neurones (Fig. 7C3 and D3). Within this round to oval innervation domain, the L2/3 axonal length was 2881 µm (barrel-centred); with a bouton density of 0.30 ± 0.02 µm–1, this corresponds to roughly 900 synaptic boutons per pyramidal cell in the innervation domain. In the barrel-centred map, the L2/3 dendritic length was 3200 µm, i.e. the ratio of dendritic to axonal length was 1.11. With these values and a spine density on the basal dendrites of 0.97 ± 0.07 µm–1 (Lübke et al. 2003), the fraction of synaptic contacts established by the axonal collaterals of the intracolumnar presynaptic L2/3 pyramidal cells can be estimated (see below).
To estimate whether the extent of the innervation domain of the presynaptic L2/3 pyramidal cell axonal collaterals and postsynaptic L2/3 pyramidal cell dendrites corresponds to the actual density of innervation, the location of synaptic contacts was marked in the innervation domain (Fig. 9; light blue dots). Indeed, the majority of synaptic contacts were located within the borders of the innervation domain. This is the case irrespective of whether the reconstructions were centred with respect to barrels (Fig. 9A) or to L2/3 pyramidal cell somata (Fig. 9B). Only 2 or 0 of 22 contacts (9 or 0%, barrel- or soma-centred maps, respectively; n = 8 L2/3 pyramidal cell pairs) were located outside the predicted innervation domain.
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Discussion |
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The present results are relevant to the question of which factors govern the horizontal spread of excitation within the PW column and out of the PW into the SuW columns when a single whisker has been deflected. To resolve this one has to determine under which conditions the excitation arriving via the L4 afferents is transformed by the intralaminar network of layer 2/3 into AP firing thereby mediating the spread of excitation over the cortical surface.
Local properties of L2/3 pyramidal cells
Comparison with previous results. Synaptic connections between pairs of L2/3 pyramidal cells have been studied in several cortical areas, most notably in the visual, auditory, somatosensory and motor cortex of juvenile and mature rats (Mason et al. 1991; Thomson & Deuchars, 1997; Thomson, 1997; Hardingham & Larkman, 1998; Thomson & Bannister, 1998; Egger et al. 1999; Reyes & Sakmann, 1999; Atzori et al. 2001; Thomson & West, 1993; Thomson et al. 2002; Holmgren et al. 2003; Koester & Johnston, 2005). The mean unitary EPSP amplitude from all these studies was about 0.8 mV (range 0.3–1.7 mV with no obvious differences between cortical areas), a value very close to that observed in the present study (1.0 ± 0.7 mV). L2/3–L2/3 connections are generally reliable with C.V. values varying from 0.10 to 0.55, although not as reliable as those between L4 spiny neurones and L2/3 pyramidal cells. The failure rate for L2/3–L2/3 connections in the barrel cortex has been reported to be low (7%, Atzori et al. 2001; 22%, Koester & Johnston, 2005; compared to 3% observed in this study), suggesting a relatively high reliability. However, in auditory cortex L2/3 pyramidal cell connections have only either a low or an intermediate release probability, indicating area specific differences between L2/3–L2/3 connections (Atzori et al. 2001).
In an in vivo study (Crochet et al. 2005), synaptically connected L2/3 pyramidal cells have been shown to be in either a ‘silent’ or an ‘active’ state. In the ‘silent’ state, the mean EPSP amplitude is 0.7 mV with a C.V. of 0.45 while in the ‘active’ state it decreases to 0.5 mV and is much less reliable (C.V. = 1.57). The EPSP amplitudes in the silent state are roughly similar to those measured here (1.0 ± 0.7 mV), despite the authors' assumption that in vivo the free extracellular Ca2+ concentration (and therefore the release probability) is lower than that in slice ASCF; this indicates that the slice situation is probably similar to the ‘silent’ or ‘down’ state of neurones (Petersen et al. 2003).
So far, L2/3 pyramidal cells have not been classified into morphologically distinct subgroups. While Larkman & Mason (1990) reported superficial L2/3 pyramidal cells with short apical dendrites and deeper neurones with longer apical dendrites, they did not quantify the relationship between the length of the apical dendrite and the extent of the apical tuft. As superficial pyramidal cells have broader and more elaborate tuft regions, inputs from the paralemniscal thalamic afferents as well as from L5A pyramidal cells could be integrated over a larger cortical area (Feldmeyer et al. 2005; Shepherd & Svoboda, 2005; Shepherd et al. 2005). This might result in different RF properties for deep and superficial pyramidal cells in layer 2/3, which should be examined by in vivo studies.
Synaptic efficacy.
The size of the unitary EPSP evoked by a single presynaptic AP is given by V
=
nbqSpr with nb, qS and pr as defined above. The unitary EPSP in L2/3-to-L2/3 connections is on average around 1 mV, which is larger than that of unitary EPSPs at the L4-to-L2/3 connections (0.7 mV; Feldmeyer et al. 2002). In pairs with morphologically identified synaptic contacts, the mean EPSP amplitude was almost identical (0.5 mV and 0.4 mV for L4–L2/3 and L2/3–L2/3 connections, respectively) with the number of contacts being 4.5 and their mean distance from the soma being 69 µm for L4–L2/3 connections and 2.8 contacts and a mean distance of 97 µm for L2/3–L2/3 connections (the value of 55 µm reported by Koester & Johnston (2005) is likely to be an underestimate as this study was biased towards contacts close to the soma. The release probability for individual contacts has been estimated to be 0.79 at the L4–L2/3 (Silver et al. 2003) and 0.46 at the L2/3–L2/3 connection in somatosensory cortex (Koester & Johnston, 2005), respectively. Since both the number and the geometric distance of contacts are not vastly different for the two connection types, this may suggest that the quantal EPSP amplitude qS for the L2/3–L2/3 connection is on average somewhat larger than at the L4–L2/3 connection.
Architecture of inputs to L2/3 pyramidal cells
In vivo whole cell recordings from barrel-related pyramidal cells in layer 2/3 have indicated that L2/3 pyramidal cells have broad subthreshold RFs, but narrow suprathreshold RFs (Moore & Nelson, 1998; Margrie et al. 2002; Brecht et al. 2003). The subthreshold RFs reflect the structure of the network of synaptic inputs to L2/3 pyramidal cells. Importantly, these RFs are dynamic as they expand rapidly 20–30 ms after stimulus onset before collapsing during the following 100–200 ms (Brecht et al. 2003).
The barrel-related L2/3 pyramidal cells are elements of the supragranular network that receives direct input from the thalamus (VPM), the deeper layers L4 and L5A as well as horizontal input from within layer 2/3 (Fig. 10; Feldmeyer et al. 1999, 2005; Shepherd & Svoboda, 2005; Shepherd et al. 2005); some input from L5B pyramidal cells may exist as well (Thomson & Bannister, 1998). The degree of excitation of L2/3 pyramidal cells, as measured by subthreshold RFs, thus depends firstly on the anatomical convergence of the axonal arbours projecting from these neurones into layer 2/3, secondly on the efficacy of these connections in eliciting APs in their target L2/3 pyramidal cells, and thirdly on the synchrony of synaptic inputs of a particular type of projection. Together the time dependent PSP and AP patterns in layer 2/3 ‘represent’ a sensory stimulus as a cortical ‘map’. The results of the present experiments relevant for constructing such a map are the contours of the innervation domains of L4 and L2/3 afferents (Fig. 10), the size of unitary EPSPs of L2/3-to-L2/3 connections and the relative independence of unitary EPSP amplitudes on the distance between synaptically connected neurones (at least within the innervation domain; but see Holmgren et al. 2003).
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Anatomical convergence: estimate of L2/3 pyramidal cells targeting a L2/3 pyramidal cell in a column.
A rough estimate of the number of L2/3 pyramidal cells that innervate a L2/3 pyramidal cell in the same PW column can be derived from the number of synaptic boutons of the pyramidal cell axon that is located within the ‘innervation-domain’ of the column. The mean number of 0.3 boutons per micrometre axon length, and an axonal length of 2881 µm yields a total number of 900 boutons in the (barrel-centred) innervation domain of each pyramidal cell. When the number of boutons in the innervation domain is divided by the average number of synaptic contacts made in a L2/3-to-L2/3 pyramidal cell pair (3 contacts established per connection assuming a single release site per contact: Silver et al. 2003; Biro et al. 2005), a single L2/3 pyramidal cell should innervate about 300 postsynaptic neurones. Assuming that a 10% fraction of the boutons establishes synaptic contacts on inhibitory interneurones (numbers vary between 5% and 25%; see, e.g. DeFelipe & Farinas, 1992; Beaulieu, 1993; DeFelipe et al. 1999; see also Supplemental Online Material; Supplemental Fig. 4), the number of L2/3 pyramidal cells targeted by a single L2/3 pyramidal cell is probably in the order of 270 barrel-related pyramidal cells. For symmetry reasons, this is also the number of L2/3 pyramidal cells in a column by which a single L2/3 pyramidal cell is innervated, i.e. that converge on a single pyramidal cell. Thus, the numbers of barrel-related L2/3 pyramidal cells and L4 spiny neurones innervating a single L2/3 pyramidal cell is comparable (300–400, Lübke et al. 2003
versus 270, this report). This estimate differs significantly from that of Holmgren et al. (2003) who calculated about 60 inputs within a distance of ±200 µm, a region about the size of the innervation domain. In part this may be due to the larger mean distance between synaptically coupled neurones in their study, but even for short distances between somata (< 25 µm) the connectivity estimates were low compared to this and other studies (Mason et al. 1991; Hardingham & Larkman, 1998; Atzori et al. 2001; Thomson et al. 2002). Furthermore, it is unlikely that 60 inputs can sustain AP firing in the L2/3 network given the sparse AP activity reported from in vivo studies (Brecht et al. 2003).
Functional convergence: estimate of active L2/3 pyramidal cell inputs.
One can roughly estimate the amplitude of the late compound EPSP in a L2/3 pyramidal cell following deflection of the PW. The late EPSP is evoked by the columnar L2/3-to-L2/3 circuit after the L4-to-L2/3 input has generated early compound EPSPs and an initial spatially distributed train of APs in layer 2/3. We assume that each pyramidal cell in layer 2/3 is innervated by 270 other barrel-related pyramidal cells. As a lower estimate, 3% of these pyramidal cells generate an AP upon deflection of a single whisker (Brecht et al. 2003). Hence, each L2/3 pyramidal cell in the PW-column would receive about eight additional unitary synaptic inputs (because 3% of the 270 anatomical inputs are active) from other pyramidal cells located in the L2/3 network of the same column. Since a single L2/3 input generates a unitary EPSP size of about 1 mV, the maximal peak of the late compound EPSP is 8 mV. Because of the jitter of APs in layer 2/3 the late depolarization is, however, much smaller. If the single cell response probability for L2/3 pyramidal cells is 0.11, i.e. 10% (upper estimate; C.P.J. de Kock & B. Sakmann, unpublished observation), the late compound EPSP could be substantially higher. Thus, the L2/3-to-L2/3 connections could amplify the excitation evoked by feed-forward excitatory input from layer 4 (Douglas & Martin, 2004).
Vertical excitatory projections of L2/3 pyramidal cells in infragranular layers
Anatomical reconstructions of connected cell pairs (Feldmeyer et al. 2002; Lübke et al. 2003) indicate that L2/3 axonal arbours spread laterally across PW column borders also in infragranular layers 5 and 6. These are collaterals, which branch off from the vertically orientated main axon of the L2/3 pyramidal cells. The main axons project vertically to the subcortical white matter and give rise to axon bundles projecting to the contralateral hemisphere, to S2 and to the motor cortex (Hoffer et al. 2003, 2005). The infragranular projection tangential to the pial surface of L2/3 pyramidal cells is most dense in layer 5A. The overlap between L2/3 axonal arbours and L5A dendritic arbours is forming an innervation domain with the highest density of potential L2/3-to-L5A synaptic contacts underneath a barrel wall. Presumably it is part of an excitatory cortical feedback loop connecting reciprocally layer 2/3 and 5A (Feldmeyer et al. 2005; Shepherd & Svoboda, 2005; Schubert et al. 2006).
Conclusions
The major aim of the present study in conjunction with our previous work on the anatomical and functional connectivity of different classes of neurones in the barrel cortex is to delineate how a simple sensory stimulus, a brief whisker deflection, is encoded by PSPs and APs in L2/3 and to quantify the anatomical and functional determinants of the respective representational maps.
Figure 11 illustrates schematically part of a pattern of feed-forward vertical input combined with intralaminar (reciprocal) feedback excitation examined so far by paired recordings in layers 4, 2/3, 5A and 5B (Markram et al. 1997; Feldmeyer et al. 1999, 2002, 2005; Bruno & Sakmann, 2006). Here vertical thalamic input from VPM excites spiny cells in layer 4 which excite other cells within layer 4 to generate early APs. Via the intralaminar reciprocal excitatory connections the AP activity will be amplified provided the early APs are synchronous. A similar pattern of vertical feed-forward and horizontal feed-back excitation applies to layer 2/3 and 5A. Both are excited by feed-forward input from layer 4 that can be amplified by the intralaminar feed-back excitation. Surprisingly, all L2/3 pyramidal cells in the principal column respond, upon a single PW whisker deflection, with an early compound EPSP (Brecht et al. 2003). These early EPSPs reflect the high divergence of L4-to-L2/3 connections. The later compound EPSPs reflect the high divergence of connections between L2/3 pyramidal cells. Functionally both L4-to-L2/3 and L2/3-to-L2/3 connections are of high reliability but of relatively low efficacy. APs generated by these two connections signal to virtually every barrel-related cell in layer 2/3 the deflection of a whisker. In other words, the input to (and subthreshold excitation within) layer 2/3 is ‘dense’. However, only a small fraction, 3–11%, of L2/3 pyramidal cells respond with APs, and thus the output from layer 2/3 to other cortical areas like S2 or M1 is ‘sparse’. This pattern of dense coding at the input to a layer (meaning that in a large fraction of cells in a layer, PSPs are generated reliably) and sparse output from a layer (meaning in a small fraction of neurones APs are generated) is seen in layers 4, 2/3 and layer 5. The intralaminar feed-forward connections observed in each layer could in certain circumstances selectively amplify excitation in a particular layer and thus enhance its output to the specific target cells.
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