Activity-Dependent Patterning of Retinogeniculate Axons Proceeds with a Constant Contribution from AMPA and NMDA Receptors

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 (14)

Citing Articles via Google Scholar

Google Scholar

Articles by Hohnke, C. D.

Articles by Sur, M.

Search for Related Content

PubMed

PubMed Citation

Articles by Hohnke, C. D.

Articles by Sur, M.

Previous Article  |  Next Article

The Journal of Neuroscience, November 1, 2000, 20(21):8051-8060

Activity-Dependent Patterning of Retinogeniculate Axons Proceeds with a Constant Contribution from AMPA and NMDA Receptors
Carsten D. Hohnke, Serkan Oray, and Mriganka Sur
Department of Brain and Cognitive Sciences, Massachusetts Institute of Technology, Cambridge, Massachusetts 02139

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Neural activity is critical for the refinement of neural circuitry during development, although the mechanisms involved instabilizing appropriate connectivity remain unclear. It has beenproposed that the insertion of AMPA receptors at synapses withonly NMDA receptors ("silent synapses") mediates this stabilization,leading to an increasing contribution from AMPA receptors as developmentproceeds. Here we show in a mammalian system known to undergoactivity-dependent development [the segregation of retinal afferentsinto ON/OFF sublaminae in the ferret lateral geniculate nucleus(LGN)] that the refinement of the neural circuitry occurs in thepresence of a constant functional contribution from AMPA and NMDAreceptors. Although we detected a small number of silent synapseson LGN cells, their proportion did not decrease with age. Thesize and kinetics of NMDA-mediated spontaneous EPSCs (sEPSCs)were also stable over this period. Together with previous resultsreporting the stability of unitary AMPA-mediated EPSCs, the constancyof NMDA-mediated sEPSCs indicates an unchanging AMPA/NMDA contribution.Additionally, the CNQX-sensitivity did not increase for eithersEPSCs or optic tract-evoked EPSCs. Likewise, the anatomical AMPA/NMDAratio, as assayed by quantifying the colocalized expression ofAMPA and NMDA receptor subunits, was fixed throughout ON/OFF sublamination.In particular, the colocalization of AMPA receptor subunits (GluR1or GluR4) and NMDA receptor subunit NR1 opposite identified retinogeniculateterminals was stable during this period. These results add tothe view of the population of retinogeniculate synapses as robustlystable or normalized during a period when retinogeniculate axonsare undergoing dramatic activity-dependentrefinement.

Key words: visual system development; silent synapses; electrical activity; NMDA receptors; AMPA receptors; lateral geniculate nucleus

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In many sensory systems, the development of appropriate neural circuitry depends critically on the presence of patterned neuralactivity. In the mammalian visual system, for example, both thalamicand cortical circuits are refined in an activity-dependent mannerduring early development (Goodman and Shatz, 1993; Cramer andSur, 1995; Katz and Shatz, 1996; Hohnke and Sur, 1999a). However,it is not well understood how neural activity provides instructionfor changes in the neural circuitry. Given the similarities betweenthe mechanisms involved in activity-dependent development andthose involved in changes of synaptic efficacy [such as long-termpotentiation (LTP) or long-term depression ], it has been proposedthat the latter phenomenon mediates the former (Constantine-Patonet al., 1990; Kandel and O'Dell, 1992; Goodman and Shatz, 1993;Cramer and Sur, 1995; Katz and Shatz, 1996; Constantine-Patonand Cline, 1998). More specifically, it has been proposed thatthe conversion of so-called silent synapses to functional onesmight be involved in the maintenance of LTP (Isaac et al., 1995;Liao et al., 1995), as well as in the establishment of appropriateconnectivity during development (Durand et al., 1996; Wu et al.,1996; Isaac et al., 1997; Li and Zhuo, 1998; Rumpel et al., 1998;Liao et al., 1999; Petralia et al., 1999). That is, before a periodof activity-dependent development, all axon branches, appropriatelyand inappropriately placed, make a significant number of synapseswith NMDA receptors alone, and those branches are stabilized onwhich synapses incorporate AMPA receptors; the others areretracted.

Yet, although silent synapses may play a role in activity-dependent refinement during development, they have not been investigatedin a developing mammalian system that undergoes a well characterizedaxonal reorganization. The majority of reports of silent synapsescome from the hippocampus (Isaac et al., 1995; Liao et al., 1995;Durand et al., 1996; Liao et al., 1999; Petralia et al., 1999);however, to our knowledge, the activity-dependence of axonal developmentin that region has not been reported. Likewise, in other mammalianbrain regions, the role of activity in shaping the relevant axonarbors containing precisely the synapses that were examined isunclear (see Discussion). Silent synapses have also been foundin the tadpole optic tectum (Wu et al., 1996) in which activityis known to alter retinotectal afferents (Debski et al., 1990;Cline, 1991; Renteria and Constantine-Paton, 1996).

We have been investigating the development of synaptic efficacy in the ferret lateral geniculate nucleus (LGN). In the ferret,retinal projections from each eye initially overlap in the LGNbut segregate within the first 2 postnatal weeks into laminaethat receive inputs from only one or the other eye. In the subsequent2 weeks, within each of the eye-specific layers, retinogeniculateaxons from ON-center and OFF-center retinal ganglion cells (RGCs)segregate further to form ON/OFF sublaminae (Hahm et al., 1991,1999). This segregation is activity-dependent and relies on componentsthat are also required for the modification of synaptic strength(Cramer and Sur, 1995; Hohnke and Sur, 1999a). Here we investigatethe development of silent synapses and, more generally, the AMPA/NMDAcontribution during ON/OFF sublamination. Our results show thatsublamination proceeds with a stable AMPA/NMDA contribution, asassessed through multiplemeasures.

Parts of this work have been published previously in abstract form (Hohnke and Sur, 1999b; Oray et al., 1999).

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Electrophysiology. Thalamic slices (400-µm-thick) were prepared from young [postnatal day 14 (P14) to P31] ferrets. Animalswere deeply anesthetized with sodium pentobarbital (35 mg/kg,i.p.) and decapitated. A block of tissue including the thalamuswas rapidly removed and placed in a cold solution (4°C) containing(in mM): 210-252 sucrose, 3 KCl, 2-3 MgSO₄, 25 NaHCO₃, 1 NaHPO₄,1-2.5 CaCl₂, 10 dextrose, and 0.5-5 kynurenic acid, saturatedwith 95% O2-5%CO₂, pH 7.4. The cortex was dissected away, andthe remaining thalamus was sliced in the horizontal plane witha Vibratome (model 1000; Ted Pella Inc., Redding, CA). Sliceswere allowed to recover at room temperature in artificial CSF(ACSF) containing (in mM): 126 NaCl, 3 KCl, 2 MgSO₄, 25 NaHCO₃,1 NaHPO₄, 2.5 CaCl₂, and 10 dextrose, saturated with 95% O2-5%CO₂,pH 7.4. Slices were transferred to a submersion chamber and continuouslyperfused with ACSF. Recordings were performed at room temperatureunder visual control with infrared-differential interference contrastmicroscopy and were made from relay cells in the A and A1 laminae,the borders of which were clearly visible. In all experiments,50 µM bicuculline methiodide (Sigma, St. Louis, MO) was presentin the ACSF. 6-Cyano-7-nitroquinoxaline-2,3-dione (CNQX) (10 µM;Sigma) and 50 µM D-2-amino-5-phosphonopentanoic acid (Sigma) wereused to block AMPA and NMDA currents, respectively. Patch pipettescontained (in mM): 105 cesium gluconate, 10 HEPES, 1 sodium EGTA,0.1 CaCl₂, 2 MgCl₂, 2 Na-ATP, 0.1 Na-GTP, and 5 QX-314; the pHwas adjusted to 7.3. Retinal afferents were stimulated at 0.2Hz by delivering constant current through a bipolar stimulatingelectrode positioned in the optic tract at the lateral edge ofthe slice. For minimal stimulation, appropriate stimulus intensitieswere based on those used in previous investigations of minimalor single-fiber stimulation (Raastad et al., 1992; Stevens andWang, 1994). Briefly, a stimulus intensity was sought that (1)initially resulted in both EPSCs and failures, (2) produced constantEPSC latencies, and (3) did not produce EPSCs of significantlydifferent amplitudes than those intensities just less than orgreater to it [that is, the minimal response was stable over arange (~5-10%) of stimulus intensities]. For nonminimal stimulation,stimulus strength was set at the value just greater than thatwhich produced no failures. Recordings, voltage-clamped at $-$ 60or +40 mV, were obtained with an Axopatch-200 amplifier (AxonInstruments, Foster City, CA), and data were acquired with pClamp(Axon Instruments) and analyzed using Matlab (MathWorks Inc.,Natick, MA). Series resistances were 19.8 ± 10.0 M $Omega$ . Cells thatshowed overshooting action potentials and that had resting membranepotentials more hyperpolarized than $-$ 40 mV were considered foranalysis. Spontaneous EPSCs (sEPSCs) were automatically detectedand analyzed as described previously (Hohnke and Sur, 1999b).Evoked EPSCs were analyzed similarly. Data are expressed as median,mean ± SEM. The Mann-Whitney U test, Spearman rank correlation,and Kruskal-Wallis nonparametric ANOVA were used for tests ofsignificance unless otherwisenoted.

Eye injections. Animals were treated subcutaneously with atropine (0.1 mg/kg in 9% saline) and then deeply anesthetized withisoflurane (2%) in a nitrous oxide (60%) and oxygen (40%) mixture.A small surgical blade was used to separate the eyelids to exposethe conjunctiva on the lateral side of the eye. A 50 µl Hamiltonmicrosyringe was then used to inject 10 µl of the anterogradetracer cholera toxin subunit B (CTB) (1% H₂O; List Biologic, Campbell,CA) into the eye. After eye injection, the eyelids were allowedto reclose, and an antibiotic ophthalmic ointment was applied.A 2 d survival period was allowed for axonal transport of theCTB to theLGN.

Immunostaining. Animals were deeply anesthetized with sodium pentobarbital (35 mg/kg) and perfused transcardially with isotonicsaline, followed by 4% paraformaldehyde. The brain was removed,post-fixed for 24 hr, transferred to 30% sucrose for 24 hr, andthen sectioned horizontally at 50 µm. Sections were blocked andpermeabilized with 0.5% Triton X-100 for 30 min in normal sera,incubated with primary antibodies for 48 hr at 4°C, and subsequentlyincubated with secondary antibodies for 2 hr at room temperature.Sections were then mounted in buffer, coverslipped, and sealed.The following antibodies were used: mouse anti-NMDA receptor subunit1 (NR1) (1:250; PharMingen, San Diego, CA) (Catalano et al., 1996),rabbit anti-glutamate receptor subunit 1 (GluR1) (1:1000; UpstateBiotechnology, Lake Placid, NY) (Carder, 1997), rabbit anti-GluR4(1:100; Chemicon, Temecula, CA) (Jones et al., 1998), goat anti-CTB(1:1000; List Biologic) (Angelucci et al., 1996), mouse anti-synaptophysin(1:10; Boehringer Mannheim, Indianapolis, IN) (Voigt et al., 1993),horse anti-mouse FITC (1:200; Vector Laboratories, Burlingame,CA), goat anti-rabbit Texas Red (1:200; Vector Laboratories),and donkey anti-goat Cy5 (1:200; Chemicon). The specificity ofthe secondary antibodies was confirmed by omitting the primaryantibodies; in all such control experiments, no fluorescence wasobserved.

Confocal microscopy. Confocal scanning microscopy was performed using a Bio-Rad (Hercules, CA) MRC 1024ES system on a Zeiss(Oberkochen, Germany) Axioplan microscope. All images were collectedwith a Zeiss Plan-Neofluar 100× oil-immersion objective with numericalaperture 1.3. Fluorescence images were obtained with a krypton-argonlaser with three standard lines of excitation at 488 (FITC), 568(Texas Red), and 647 (Cy5) nm with standard filters. The theoreticalanalog focal resolution limit (using the full-width half-maximumcriterion) for our confocal apparatus at these wavelengths was0.16, 0.19, and 0.21 µm, respectively (Stelzer, 1995). Becausewe extensively used long wavelengths of light (for visualizingTexas Red and Cy5), we chose to limit our images to a pixel resolutionof 0.21 µm. Electron microscopy studies in the A and A1 laminaeof the cat LGN (Wilson et al., 1984; Hamos et al., 1987) suggestthat the distance between the closest excitatory glutamatergicsynapses of retinal or cortical origin is on the order of 1 µm,indicating that a pixel resolution of 0.21 µm is adequate to resolveadjacent excitatory synapses even with discrete sampling of theimage. Similarly, the z-resolution (axial resolution) is limitedby numerical aperture and wavelength (for instance, at an excitationwavelength of 488 nm, the z-resolution limit is 0.42 µm and getspoorer at longer wavelengths). By reducing the iris aperture,we were able to reduce the optical section thickness to 0.38 µm.This axial resolution was chosen to maximize signal intensityand minimize optical thickness. Thus, each confocal image representeda focal region of 108.3 × 108.3 µm with an axial thickness of0.38 µm (512 × 512 pixels with eight-bit pixel depth). Imagesin the separate fluorescent channels were collected sequentiallyand were the average of five frames at a single focal plane. Allimages were taken from the A or A1 layers of theLGN.

Image analysis. For double-labeling experiments, each image was analyzed independently for high-intensity activity in theFITC and Texas Red channels by a thresholding procedure. Colocalizationof the two fluorescent signals was quantified as the number ofpixels that had high-intensity values in both the FITC and TexasRed channels. Black and white colocalization images were generatedto show the spatial distribution of colocalization with each blackpixel representing a colocalization event. In triple-labelingexperiments, the Cy5 signal (corresponding to CTB labeling ofretinogeniculate terminals) was thresholded and used to restrictthe region of analysis for the FITC and Texas Red signals. Thiswas accomplished by discarding from the analysis all pixels thatwere more than three pixels (0.63 µm) distant from the edge ofhigh-intensity (thresholded) CTB staining. These restricted imageswere then analyzed for colocalization by counting the number ofpixels with high-intensity values in both the FITC and Texas Redchannels. Clustering was assessed by sliding a window across thecolocalization image and calculating the distance of a randomdata point from its nearest neighbor and comparing it with thedistance between a random nondata point and its nearest data point.The clustering index was generated by taking the median of theratio of these two numbers after multiple iterations (Ruthazerand Stryker, 1996).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Silent synapses on LGN cells

To examine the development of silent synapses, we used minimal stimulation techniques to compare failure rates at hyperpolarized( $-$ 60 mV) and depolarized (+40 mV) membrane potentials. Additionally,we compared the frequency of sEPSCs in the two conditions. Becausesilent synapses are active only at depolarized potentials, thefailure rates at those potentials should decrease relative tofailure rates at hyperpolarized potentials if silent synapsesare present (Isaac et al., 1995; Liao et al., 1995). Likewise,the frequency of sEPSCs would be expected to increase at depolarizedpotentials. Figure 1 shows the results from a typical experiment.Responses at $-$ 60 mV were fast with no extended decay that wouldresult from the activation of NMDA receptors (Fig. 1C). Indeed,responses at $-$ 60 mV were completely blocked by CNQX (data notshown). At $-$ 60 mV, stimulation of the optic tract resulted infailures on 60% of the trials, whereas at +40 mV failures occurredon 50% of the trials (Fig. 1B). This particular example suggeststhat any systematic difference in the reliability of transmissionat the two potentials is likely to be slight.

View larger version (29K):
[in this window]
[in a new window]
Figure 1. Typical minimal stimulation recording. A, Diagram of the experimental preparation. The stimulating electrode was placed in the optic tract along the lateral edge of horizontal LGN slices. Recordings were made in the A or A1 laminae. B, Individual single-fiber EPSC amplitudes at hyperpolarized and depolarized membrane potentials (indicated at the top). The gray horizontal band indicates the approximate range of noise; EPSC amplitudes falling within it are considered failures. Note the small reduction in the number of failures at +40 mV. C, Five consecutive responses at $-$ 60 (bottom) and +40 (top) mV. Responses were easily detectable over the noise. Same cell as in B. The filled circle represents the removal of the stimulus artifact for clarity.

More generally, the population data show a slight but significant decrease in the failure rate at +40 mV (39.7 ± 2.0%) relativeto $-$ 60 mV (64.4 ± 2.0%; n = 14; p < 0.05) (Fig. 2A). The differencebetween failure rates at the two potentials (Fig. 2B) was equivalentbefore ON/OFF sublamination at P14-P17 (26.7 ± 3.5%; n = 5) andafter its completion at P28-P31 (23.6 ± 4.1%; n = 9; p > 0.05).Whereas the decrease in the failure rate at +40 mV at either theyounger or older ages indicates the presence of some silent synapsesat all ages, we find no evidence for a greater proportion at theyounger ages. Figure 2C shows example recordings from the samecell presented in Figure 1. The absence of a significant increasein the sEPSC frequency at +40 mV suggests that the number of silentsynapses onto that cell is relatively small. In neither the youngernor the older cells was sEPSC frequency increased at +40 mV. Ata holding potential of $-$ 60 mV, the sEPSC frequencies in youngercells was 0.53 Hz (0.59 ± 0.04 Hz; n = 7) and in older cells was0.38 Hz (0.53 ± 0.04 Hz; n = 9). These frequencies were no differentfrom those recorded at +40 mV for either the younger (0.40, 0.45± 0.03 Hz; p > 0.05) or the older (0.35, 0.37 ± 0.02 Hz; p > 0.05)cells (Fig. 2D). The sEPSC frequency data thus do not indicatethe presence of silent synapses and further indicate that thereis no change in the efficacy of voltage-dependent synaptic transmissionas ON/OFF sublamination is established.

View larger version (25K):
[in this window]
[in a new window]
Figure 2. A small number of silent synapses are present during ON/OFF sublamination, but their proportion is constant before and after sublamination. A, Failure rates at $-$ 60 and +40 mV for individual cells. The outside markers are the means for the two conditions. B, Failure rates by age at $-$ 60 and +40 mV. The slight decrease in failure rates at +40 mV is equivalent at P14-P17 (at the onset of sublamination; filled bars) and P28-P31 (after its completion; open bars). C, Spontaneous EPSCs recorded at $-$ 60 (bottom) and +40 (top) mV. Note the absence of a dramatic increase in the number of sEPSCs at +40 mV. Same cell as in Figure 1. D, The frequency of sEPSCs was not significantly decreased at +40 mV, suggesting that the results from B are attributable to a small rather than large number of silent synapses. Data are mean ± SEM. Denotes *p < 0.05.

Silent synapses may be an extreme example of a mechanism that modulates synaptic strength by changing the receptor complementat synapses. A probe limited to the detection of silent synapseswould not detect a more subtle change in the AMPA/NMDA contribution.Previously we have shown that the AMPA component, as assayed byAMPA receptor-mediated sEPSCs, remains stable throughout ON/OFFsublamination (Hohnke and Sur, 1999c). Here we extend those resultsby examining the development of NMDA receptor-mediated sEPSCsduring this period to obtain a finer assessment of the developmentof the AMPA/NMDAcontribution.

EPSCs mediated by NMDA receptors

By depolarizing cells to +40 mV and adding the AMPA receptor blocker CNQX to the bath, we recorded NMDA-mediated sEPSCs fromanimals between P14 and P31, spanning the period of ON/OFF sublamination.Typical distributions of areas and the averaged NMDA-mediatedsEPSCs from single cells before and after ON/OFF sublaminationare shown in Figure 3. Although variable, the NMDA-mediated sEPSCproperties of our cell population were stable throughout ON/OFFsublamination. The charge transfer of NMDA-mediated sEPSCs (Fig.4A), for example, was not correlated with age (r = $-$ 0.24; n =16; p > 0.05). More specifically, NMDA-mediated sEPSC area inthe younger cells (age less than P21) was 366 fC (426 ± 83 fC;n = 9) and in the older cells (age more than P28) was 373 fC (477± 116 fC; n = 7; p > 0.05). Neither was the frequency of NMDA-mediatedsEPSCs correlated with age during retinogeniculate axon reorganization(r = $-$ 0.23; p > 0.05). Whereas the frequency showed a slight upwardtrend toward the end of sublamination, the frequency in the youngercells (0.28, 0.16 ± 0.06 Hz) was not significantly different fromthat in older cells (0.50, 0.19 ± 0.04 Hz; p > 0.05) (Fig. 4B).

View larger version (16K):
[in this window]
[in a new window]
Figure 3. Representative histograms of NMDA-mediated sEPSC areas (recorded at +40 mV with CNQX in the bath) for a P14 (A, left) and a P31 (B, left) cell; diamonds indicate the median values. Note the similar appearance and median values of the distributions. Short and long time scale recordings from the same cells (right) show similar amplitudes and shapes at the two ages that are before and after ON/OFF sublamination, respectively.

View larger version (15K):
[in this window]
[in a new window]
Figure 4. The properties of NMDA-mediated sEPSCs are stable throughout ON/OFF sublamination. Scatter plots of the size (A), frequency (B), and kinetics (C, D) of NMDA-mediated sEPSCs throughout ON/OFF sublamination. None of the properties are correlated with age during this period (p > 0.05).

Similarly, the kinetics of NMDA-mediated sEPSCs that are present at the completion of ON/OFF sublamination have been establishedbefore its onset. Rise times (r = 0.16), half-widths (r = $-$ 0.18),and decay times (r = $-$ 0.16) were fixed throughout this periodand did not correlate with age (p > 0.05 for all measures). Risetimes in younger cells (4.0, 5.1 ± 0.9 msec) were not significantlydifferent from those in older cells (4.6, 4.7 ± 0.6 msec; p >0.05) (Fig. 4C). Likewise, half-widths in the younger cells (114,116 ± 14 msec) were unchanged in older cells (97, 98 ± 9 msec;p > 0.05). Finally, the long decay times characteristic of NMDA-mediatedcurrents were similar in the younger (124, 147 ± 19 msec) andolder (118, 123 ± 13 msec; p > 0.05) (Fig. 4D) cells. Togetherwith previous results describing a uniform AMPA receptor-mediatedcomponent during this same period (Hohnke and Sur, 1999c), thestability of NMDA-mediated sEPSCs suggests an unvarying contributionof AMPA and NMDA receptors to synaptic transmission during ON/OFFsublamination.

For a more direct assessment of the AMPA/NMDA contribution, we compared the AMPA and NMDA components of sEPSCs in the samecell. We recorded sEPSCs at +40 mV in control and CNQX solutionsand measured their CNQX-sensitivity during and after ON/OFF sublamination.Blocking AMPA receptors would leave NMDA receptor-mediated responsesand hence would be expected to reduce spontaneous (or evoked,see below) EPSC amplitude and increase the rise time; if thereare proportionately more AMPA receptors in older animals, theeffect of blocking AMPA receptors would be greater. SpontaneousEPSCs showed the expected effects in the presence of CNQX (Fig.5A), but these effects were not age-dependent. Considering allcells, normalized sEPSC rise times (rise time/amplitude, whichis the inverse of EPSC slope) in CNQX were 114% (137 ± 22%), andamplitudes were 91% (91 ± 9%) of control. In younger (P14-P16)cells, normalized sEPSC rise times in CNQX were 125% (160 ± 51%;n = 9) and in older (P28-P31) cells were 110% (109 ± 15%; n =7) of control. However, there was no significant difference inthe effect of CNQX, and therefore in the AMPA/NMDA ratio, betweenthe younger and older cells (p > 0.05) (Fig. 5B).

View larger version (18K):
[in this window]
[in a new window]
Figure 5. NMDA-mediated sEPSC and evoked EPSC rise times do not change during ON/OFF sublamination. EPSCs were recorded at +40 mV. A, Average sEPSCs from a P16 cell (top) and a P29 cell (bottom) in control (black trace) and CNQX (gray trace) conditions. B, The normalized rise time (rise time/amplitude) of sEPSCs is slightly increased in the presence of CNQX; however, the effect is similar in both younger (filled bar) and older (open bar) cells. C, Optic tract-evoked EPSCs from a P16 cell (top) and a P28 cell (bottom). D, The normalized rise time of optic tract-evoked EPSCs is increased under CNQX, but the effect is again similar in the younger (filled bar) and older (open bar) cells. Diamonds indicate median values.

Relay cells in the LGN receive input from several sources other than retinal ganglion cell axons, although the principal glutamatergicinputs are retinal or cortical in origin (Sherman and Koch, 1986,1998). Although it has been demonstrated that evoked, miniature,retinogeniculate EPSCs are indistinguishable from sEPSCs in thissystem (Hohnke and Sur, 1999c), it is not clear whether the sEPSCsrecorded in the present study arise from corticogeniculate orretinogeniculate inputs. Replacing calcium with strontium in theextracellular solution to evoke miniature EPSCs (mEPSCs) of identifiedorigin (Miledi, 1966; Goda and Stevens, 1994; Oliet et al., 1996),as we have done in our examination of AMPA-mediated retinogeniculatemEPSCs (Hohnke and Sur, 1999c), is problematic when investigatingNMDA currents because their decay times are longer than the intervalsbetween asynchronous transmitter release. To more specificallyassay the AMPA/NMDA contribution at retinogeniculate synapses,we investigated the CNQX-sensitivity of optic tract-evoked EPSCs.Optic tract stimulation in control and CNQX conditions also suggeststhat no developmental change occurs in the AMPA/NMDA contributionduring ON/OFF sublamination. After the addition of CNQX, normalizedrise times of evoked EPSCs in the younger (n = 5) cells were 159%(182 ± 54%) and in the older (n = 4) cells were 204% (205 ± 26%)of control. As with sEPSCs (but based on a small population ofcells in each group), there was no significant difference betweenthe younger and older cells in the effect of CNQX (p > 0.05),consistent with no change in the NMDA-mediated response with ageand in the AMPA/NMDA contribution (Fig. 5D).

Colocalization of AMPA and NMDA receptor subunits

To further investigate the development of the AMPA/NMDA contribution during ON/OFF sublamination, we examined the colocalizedexpression of AMPA and NMDA glutamate receptor subunits. If AMPAreceptors are progressively inserted at NMDA-only synapses, wewould observe an increase in the colocalization of AMPA and NMDAreceptors. At P14, we observed labeling of both NR1, an obligatoryNMDA receptor subunit, and GluR1, an AMPA receptor subunit, whichcontinued through P28 (Fig. 6A). There was significant overlapof the label for both subunits, and their colocalization was constantthroughout sublamination (n = 51 images from 9 animals; p > 0.05)(Fig. 6B).

View larger version (80K):
[in this window]
[in a new window]
Figure 6. AMPA and NMDA receptor subunit colocalization is stable over ON/OFF sublamination. A, NR1 (NMDA) and GluR1 (AMPA) subunit expression and colocalization at P14 (n = 15 images from 2 animals), P21 (n = 22 images from 4 animals), and P28 (n = 14 images from 3 animals). Top row shows examples of labeling of NR1 (green) and GluR1 (red) through ON/OFF sublamination. Colocalized labeling is shown in yellow. Bottom row shows only the colocalized labeling from the corresponding row above. B, Colocalization remains constant from P14 to P28 (p > 0.05). C, The clustering of colocalized pixels is similar before and after sublamination (p > 0.05), although it increases during the third postnatal week (p < 0.05). Scale bar (in this and all subsequent figures), 25 µm.

Our immunostaining technique does not differentiate between intracellular and extracellular subunit expression (Mammen etal., 1997). Consequently, colocalization values may be skewedby changes in production of the various subunits at locationsnearby one another (e.g., the cell body). That is, an increasein colocalization at synapses may be masked by a decrease in receptorsubunit translation in the nucleus. If this were the case, onewould expect to see a decrease in the clustering of colocalizedpixels, corresponding to the decrease at the soma. To addressthis issue, we performed a cluster analysis (see Materials andMethods). The clustering of GluR1 and NR1 is similar before andafter ON/OFF sublamination (p > 0.05), although it increases fromP14 to P21 (p < 0.05) (Fig. 6C).

Unlike NMDA receptors, AMPA receptors do not include an obligatory subunit. Consequently, to determine whether the patternof colocalization that we observed was in some way unique to theGluR1 subunit, we repeated the double-labeling experiments withantibodies to the GluR4 subunit. The development of GluR4-NR1colocalization during ON/OFF sublamination was similar to thatobserved with GluR1-NR1 labeling (Fig. 7A). That is, colocalizationof GluR4 and NR1 at P14, P21, and P28 was stable (n = 38 imagesfrom 9 animals; p > 0.05) (Fig. 7B). As with GluR1-NR1 labeling,GluR4-NR1 clustering at the end of sublamination was not significantlychanged from that before its onset (p > 0.05), although it didincrease at P21 (p < 0.05) (Fig. 7C). Interestingly, at laterages (P21 and P28), we observed neurons that expressed NR1 butdid not express high levels of the GluR1 subunit. In contrast,we observed no neurons at any age that expressed NR1 but did notexpress GluR4. This may suggest that GluR4 is a more stable andubiquitous AMPA receptor subunit in the developing ferret LGN.

View larger version (80K):
[in this window]
[in a new window]
Figure 7. The pattern of AMPA-NMDA colocalization is not unique to GluR1. A-C, Same convention as in Figure 6. GluR4-NR1 colocalization is stable across ON/OFF sublamination (p > 0.05). P14 (n = 14 images from 2 animals), P21 (n = 13 images from 4 animals), and P28 (n = 11 images from 3 animals). Clustering of colocalized pixels is similar before and after sublamination (p > 0.05), although it increases during the third postnatal week (p < 0.05).

Finally, we were interested in examining NR1, GluR1, and GluR4 staining that was closely associated with retinal terminals.That is, given the concern noted above that both intracellularand extracellular subunits were labeled, we wanted to characterizecolocalization directly opposite retinogeniculate boutons (i.e.,at presumptive retinal synapses). To that end, we performed triple-labelingexperiments. We labeled retinogeniculate afferents with CTB injectedinto the eye and subsequently also labeled GluR1 and NR1 subunits(Fig. 8A). These experiments also distinguished between retinogeniculateand corticogeniculate inputs and allowed for the determinationof whether an increase in AMPA-NMDA colocalization at retinogeniculatesynapses was being masked by the more extensive corticogeniculateinput. Colocalization opposite CTB-stained retinogeniculate fibersrevealed a pattern that was not significantly different from thatseen with the more general double labeling. Both colocalizationand clustering were no different after ON/OFF sublamination thanbefore (n = 13 images from 2 animals; p > 0.05) (Fig. 8B,C). Triple-labelingof retinogeniculate terminals, GluR4, and NR1 (Fig. 9A) showedthe same results as with GluR1; colocalization and clusteringopposite retinogeniculate terminals were similar before and afterON/OFF sublamination (n = 10 images from 2 animals; p > 0.05)(Fig. 9B,C).

View larger version (80K):
[in this window]
[in a new window]
Figure 8. The pattern of AMPA-NMDA colocalization opposite retinogeniculate terminals is not different from the global pattern of colocalization in the LGN. A, NR1 (green) and GluR1 (red) labeling opposite CTB-labeled retinogeniculate terminals (blue). Left column shows examples of triple labeling at P14 and P28. Middle column shows pixels just opposite CTB labeling (for details, see Materials and Methods). Right column shows only the colocalized labeling at pixels derived from the corresponding column to the left. B, Colocalization at P28 (n = 5 images from 1 animal) is unchanged from P14 (n = 8 images from 1 animal; p > 0.05). C, Likewise, the clustering of colocalized pixels is similar before and after sublamination (p > 0.05).

View larger version (82K):
[in this window]
[in a new window]
Figure 9. The pattern of AMPA-NMDA colocalization opposite retinogeniculate terminals is not unique to GluR1. A-C, Same convention as in Figure 8. GluR4-NR1 colocalization at P28 (n = 7 images from 1 animal) is unchanged from P14 (n = 3 images from 1 animal; p > 0.05). Clustering of colocalized pixels opposite retinogeniculate terminals is stable across ON/OFF sublamination (p > 0.05). D, CTB label overwhelmingly represents synaptic boutons, marked by synaptophysin, rather than fibers of passage. The vast majority of CTB label (blue) is colocalized with synaptophysin (green); colocalized label is shown in pink. There is also a significant amount of synaptophysin labeling independent of CTB, reflecting the nonretinal innervation of the LGN.

In separate experiments, we confirmed that primarily synaptic boutons at retinal terminals rather than fibers of passage werelabeled by the CTB injections. In conjunction with CTB injections,we labeled synaptophysin, a synaptic vesicle protein. The vastmajority of CTB label (98%) was colocalized with synaptophysin(Fig. 9D), indicating that the periphery of CTB label was an appropriateconstraint for examining presumptive postsynaptic locations forGluR1 (or GluR4)-NR1 colocalization. Whereas there was very littleCTB label that was not colocalized with synaptophysin, there was,of course, synaptophysin labeling that was not colocalized withCTB (52% of the label in Fig. 9D), reflecting the nonretinal inputto the LGN (e.g., cortical and brainstemterminals).

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The results presented here, obtained using a variety of techniques, demonstrate that, although a small number of silent retinogeniculatesynapses are present at the onset of ON/OFF sublamination, anoverall change in the AMPA/NMDA contribution is unlikely to beinvolved in the maturation of sublamination. Using minimal stimulationof the optic tract, we show that failure rates of responses atdepolarized potentials do not change with age. We show that NMDA-mediatedsEPSCs maintain their size and kinetics and have shown previouslythe same for AMPA-mediated sEPSCs (Hohnke and Sur, 1999c). Wedemonstrate that the rise time and amplitude of the NMDA-mediatedcomponent of spontaneous and optic tract-evoked EPSCs is constantthroughout ON/OFF sublamination. Using immunocytochemistry toidentify AMPA and NMDA receptor subunits, we show that AMPA-NMDAcolocalization is stable throughout the LGN and opposite retinogeniculateterminals inparticular.

Three caveats to our data should be noted. First, it is possible that NMDA-only currents are not attributable to the existenceof NMDA-only synapses but rather to the spillover of glutamatefrom an active synapse into an inactive one (Kullmann and Asztely,1998). The low concentration of transmitter that would resultfrom spillover would preferentially activate NMDA receptors, whichhave a higher affinity for glutamate (Patneau and Mayer, 1990).However, recent evidence suggests that AMPA and NMDA receptorshave similar affinities (Dube and Liu, 1999). Additionally, immunocytochemicaldata show that some hippocampal synapses have no detectable AMPAreceptors (Liao et al., 1999; Petralia et al., 1999). Recordingsfrom autapses also reveal silent synapses (Gomperts et al., 1998),and the kinetics of NMDA receptor activation at functional andsilent synapses are similar (Rumpel et al., 1998). Whatever thesource of NMDA-only currents, our results indicate that theircontribution to retinogeniculate transmission is held fixed throughoutON/OFFsublamination.

Second, we recorded from a heterogeneous population of cells in the A layers of the LGN that include X cells, Y cells, andinterneurons. It is unlikely that we recorded from many interneurons;recordings from cells with small somas [which are characteristicof interneurons (Friedlander et al., 1981)] were avoided, andall cells included in the analysis displayed easily evoked low-thresholdcalcium spikes, a characteristic of LGN relay cells (McCormickand Pape, 1988). However, although we observed no systematic variationsin our data that might correlate with different LGN cell types,such a relationship cannot beexcluded.

A third caveat is that, ideally, our immunostaining technique would target extracellular receptor proteins opposite retinogeniculateterminals. Antibodies to extracellular domains are available (Mammenet al., 1997), of course, that specificity would be lost in thesectioned LGNs that we used in this study because of the permeabilityof cell membranes attributable to tissue sectioning. As a result,trends in the colocalization of subunits at synapses may be maskedby the characteristics of intracellular colocalization. Indeed,in spinal cultures, the percentage of surface GluR1 increasesas cells mature during the first 1-2 weeks (Mammen et al., 1997).However, our cluster analysis indicates, albeit indirectly, thatin P14-P28 ferret LGN there is no trend in the density of colocalizationat particular loci (e.g., the nuclei) that would obscure an increasein colocalization after ON/OFF sublamination relative to beforeit. A more direct analysis of colocalization just opposite identifiedretinogeniculate fibers gives the same results, i.e., stable colocalizationthroughout ON/OFF sublamination. We did observe an increase inclustering during the middle of sublamination that may reflecta transient increase in receptor subunit production in thesoma.

Silent synapses and their role in development of connections

Our findings present a counterweight to recent evidence suggesting that the conversion of silent to functional synapses mayplay an important role in the development and refinement of inputs(Durand et al., 1996; Wu et al., 1996; Isaac et al., 1997; Liand Zhuo, 1998; Rumpel et al., 1998; Liao et al., 1999; Petraliaet al., 1999). Of that evidence, only one previous study (Isaacet al., 1997) has investigated the development of silent synapsesin a mammalian system, the rat primary somatosensory cortex, inwhich activity-dependent plasticity has been systematically explored.Yet, even in that system, the role of activity in reshaping thethalamocortical afferents that were probed for silent synapsesis unresolved (Feldman et al., 1999; Wallace and Fox, 1999). Thedevelopment of the ON/OFF sublaminae, and more specifically, thedevelopment of individual retinogeniculate axons, are known todepend on retinal activity (Cramer and Sur, 1997), NMDA receptorson LGN cells (Hahm et al., 1991, 1999), and the presence of nitricoxide (Cramer et al., 1996; Cramer and Sur, 1999). The presentresults demonstrate that, although the structure of retinogeniculatearbors is altered during sublamination in an activity-dependentmanner, the functional efficacy of retinogeniculate synapses doesnot appear to change during thisperiod.

Why might the results at retinogeniculate and thalamocortical synapses differ? It is possible that there are simply differentmechanisms of plasticity at work in these two systems. Even withinone system, distinct forms of plasticity can be found (Zalutskyand Nicoll, 1991; Johnston et al., 1992). It is also possiblethat differences between the cellular environments of 1-week-oldrat cortex and 4-week-old ferret thalamus recruit the same elements(silent synapses) for different purposes (Constantine-Paton andCline, 1998; Lin and Constantine-Paton, 1998). Indeed, in amphibiansin which the activity-dependence of retinotectal afferents hasbeen extensively described previously (Debski et al., 1990; Cline,1991; Renteria and Constantine-Paton, 1996), it has been proposedthat silent synapses provide a mechanism for the continued, faithfultransmission of information during the period when topographymust be continually updated (Wu et al., 1996). Perhaps the rapidlydeveloping body surface of neonatal rats places demands on thalamocorticalafferents in the somatosensory cortex that are similar to thoseplaced on retinotectal afferents in Xenopus tadpoles in responseto the addition of RGCs. In the ferret, retinal ganglion cellbirth is completed by P3 (Johnson and Casagrande, 1993), and ganglioncell numbers reach adult values by P6 (Henderson et al., 1988;Johnson and Casagrande, 1993), well before the onset of ON/OFFsublamination.

However, it is also possible that the results presented here and those reported from thalamocortical synapses (Isaac et al.,1997) do not, in fact, differ greatly. These authors note thatthe reduction in the percentage of silent synapses that they observemay be the result of a sampling bias at later ages after significant(functional) synaptogenesis has occurred. That is, if the newterminations that form during late axon growth primarily containboth AMPA and NMDA receptors, then the percentage of silent synapseswould decrease. The width of thalamocortical axon arbors in thesomatosensory cortex increases by 80% or more during the periodinvestigated (Catalano et al., 1996). In contrast, retinogeniculatearbors do not increase significantly in size during ON/OFF sublamination,although they do become progressively restricted to an LGN sublayer(Hahm et al., 1999).

Consistent with our finding that the AMPA/NMDA contribution is held constant during ON/OFF sublamination in the LGN are reportsthat silent synapses persist during early development in anotherpart of the thalamus, the ventroposterior nucleus (Golshani andJones, 1999), and in the dorsal horn of the rat spinal cord (Bardoniet al., 1998) (but see Li and Zhuo, 1998). Additionally, likethe results reported here, sEPSCs in the rat cortex consist ofboth AMPA and NMDA receptor-mediated currents, and their ratiois constant throughout early development (Burgard and Hablitz,1993). In rat cortical neurons in culture, the ratio of quantalAMPA/NMDA currents is similar at different synapses on the sameneuron, and the ratio is preserved after activity-dependent changesin synaptic strength (Watt et al., 2000). In some systems AMPAreceptors develop earlier than NMDA receptors (Gordon et al.,1997; Colwell et al., 1998; Rohrbough and Spitzer, 1999). Perhapsmore analogously to our data, NMDA-mediated sEPSC amplitudes andrise times show no age-dependent changes in the rat superior colliculusduring the time when retinocollicular axons are refining (Hestrin,1992; Shi et al., 1997). However, in that system, NMDA-mediatedsEPSC decay times decrease during map refinement, although ourresults show no such change in the ferret. This difference islikely attributable to the difference in timing of a developmentalshift from NR2B to NR2A NMDA receptor subunits. Our study encompassesthe entirety of ON/OFF sublamination, but the NR2B to NR2A shiftin the LGN does not occur until well thereafter (Ramoa and Prusky,1997), in parallel with the decrease in the decay times of evokedNMDA-mediated EPSCs (Ramoa and McCormick, 1994b). In contrast,the NR2B to NR2A shift in the rat superior colliculus, and a paralleldecrease in the decay times of NMDA-mediated sEPSCs, occur withinthe time period examined in those studies (Shi et al., 1997).

If not as mediators of axon branch stabilization, what then is the role of NMDA-only synapses? Silent synapses may not infact be silent; extracellular glutamate concentrations (Lermaet al., 1986) and low-threshold activation of NMDA receptors invivo (Fox et al., 1990) suggest that they may be a functionalelement of developing or mature circuits (Constantine-Paton andCline, 1998). Alternatively, if NMDA-only synapses are primarilysilent, they may act as synapses-in-reserve or as mediators ofgain control (Malgaroli, 1999). In any case, the results presentedhere reinforce the assessment of the function of the populationof retinogeniculate synapses as remarkably stable during a periodof intense anatomical reorganization of their input (Hohnke andSur, 1999c). Synaptic properties of geniculocortical afferentsin the cat also show surprising conservation during an intenseperiod of reorganization (Silver and Stryker, 1999), and in themouse visual cortex, normal plasticity occurs despite defectsin the ability to potentiate synaptic efficacy (Hensch et al.,1998). The developing visual system may rely on cues other thanchanges in synaptic efficacy, perhaps via neurotrophic regulation(Castren et al., 1992; Allendoerfer et al., 1994; Cabelli et al.,1995; Riddle et al., 1995; McAllister et al., 1996), to mediateaxon branch withdrawal and stabilization. Alternatively, synapticefficacy may be modulated indirectly. Recent evidence suggeststhat absolute synaptic efficacy could remain constant, whereasrelative synaptic efficacy is modulated by activity-dependentchanges in the intrinsic excitability of neurons (Desai et al.,1999; Stemmler and Koch, 1999) or in the connectivity of cellpairs (Hsia et al., 1998). Indeed, the development of retinogeniculateconnections is accompanied by significant changes in the intrinsicmembrane properties of LGN neurons (White and Sur, 1992; Ramoaand McCormick, 1994a; Hohnke and Sur, 1999c).

  FOOTNOTES

Received July 28, 2000; revised Aug. 16, 2000; accepted Aug. 18, 2000.

The work was supported by National Institutes of Health Grants EY 11512 and EY 07023. We thank Adrienne Sacatos for assistancewith data collection in NR1/GluR1 immunocytochemistry experimentsand Michael O'Boyle for assistance with confocalmicroscopy.
Correspondence should be addressed to Mriganka Sur, Massachusetts Institute of Technology, E25-235, 45 Carleton Street, Cambridge,MA 02139. E-mail: msur{at}ai.mit.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Allendoerfer K, Cabelli R, Escandon E, Kaplan D, Nikolics K, Shatz C (1994) Regulation of neurotrophin receptors during the maturation of the mammalian visual system. J Neurosci 14:1795-1811[Abstract].
Angelucci A, Clasca F, Sur M (1996) Anterograde axonal tracing with the subunit B of cholera toxin: a highly sensitive immunohistochemical protocol for revealing fine axonal morphology in adult and neonatal brains. J Neurosci Methods 65:101-112[ISI][Medline].
Bardoni R, Magherini PC, MacDermott AB (1998) NMDA EPSCs at glutamatergic synapses in the spinal cord dorsal horn of the postnatal rat. J Neurosci 18:6558-6567[Abstract/Free Full Text].
Burgard E, Hablitz J (1993) NMDA receptor-mediated components of miniature excitatory synaptic currents in developing rat neocortex. J Neurophysiol 70:1841-1852[Abstract/Free Full Text].
Cabelli R, Hohn A, Shatz C (1995) Inhibition of ocular dominance column formation by infusion of NT-4/5 of BDNF. Science 267:1662-1666[Abstract/Free Full Text].
Carder R (1997) Immunocytochemical characterization of AMPA-selective glutamate receptor subunits: laminar and compartmental distribution in macaque striate cortex. J Neurosci 17:3352-3363[Abstract/Free Full Text].
Castren E, Zafra F, Thoenen H, Lindholm D (1992) Light regulates expression of brain-derived neurotrophic factor mRNA in rat visual cortex. Proc Natl Acad Sci USA 89:9444-9448[Abstract/Free Full Text].
Catalano S, Robertson R, Killackey H (1996) Individual axon morphology and thalamocortical topography in developing rat somatosensory cortex. J Comp Neurol 367:36-53[ISI][Medline].
Cline H (1991) Activity-dependent plasticity in the visual systems of frogs and fish. Trends Neurosci 14:104-111[ISI][Medline].
Colwell CS, Cepeda C, Crawford C, Levine MS (1998) Postnatal development of glutamate receptor-mediated responses in the neostriatum. Dev Neurosci 20:154-163[ISI][Medline].
Constantine-Paton M, Cline HT (1998) LTP and activity-dependent synaptogenesis: the more alike they are, the more different they become. Curr Opin Neurobiol 8:139-148[ISI][Medline].
Constantine-Paton M, Cline H, Debski E (1990) Patterned activity, synaptic convergence, and the NMDA receptor in developing visual pathways. Annu Rev Neurosci 13:129-154[ISI][Medline].
Cramer KS, Sur M (1995) Activity-dependent remodeling of connections in the mammalian visual system. Curr Opin Neurobiol 5:106-111[Medline].
Cramer KS, Sur M (1997) Blockade of afferent impulse activity disrupts on/off sublamination in the ferret lateral geniculate nucleus. Dev Brain Res 98:287-290[Medline].
Cramer KS, Sur M (1999) The neuronal form of nitric oxide synthase is required for pattern formation by retinal afferents in the ferret lateral geniculate nucleus. Brain Res Dev Brain Res 116:79-86[Medline].
Cramer KS, Angelucci A, Hahm JO, Bogdanov MB, Sur M (1996) A role for nitric oxide in the development of the ferret retinogeniculate projection. J Neurosci 16:7995-8004[Abstract/Free Full Text].
Debski EA, Cline HT, Constantine-Paton M (1990) Activity-dependent tuning and the NMDA receptor. J Neurobiol 21:18-32[ISI][Medline].
Desai N, Rutherford L, Turrigiano G (1999) Plasticity in the intrinsic excitability of cortical pyramidal neurons. Nat Neurosci 2:515-520[ISI][Medline].
Dube G, Liu G (1999) AMPA and NMDA receptors display similar affinity during rapid synaptic-like glutamate applications. Soc Neurosci Abstr 25:992.
Durand GM, Kovalchuk Y, Konnerth A (1996) Long-term potentiation and functional synapse induction in developing hippocampus. Nature 381:71-75[Medline].
Feldman DE, Nicoll RA, Malenka RC (1999) Synaptic plasticity at thalamocortical synapses in developing rat somatosensory cortex: LTP, LTD, and silent synapses. J Neurobiol 41:92-101[ISI][Medline].
Fox K, Sato H, Daw N (1990) The effect of varying stimulus intensity on NMDA-receptor activity in cat visual cortex. J Neurophysiol 64:1413-1428[Abstract/Free Full Text].
Friedlander M, Lin G, Stanford L, Sherman S (1981) Morphology of functionally identified neurons in the lateral geniculate nucleus of the cat. J Neurophysiol 46:80-129[Free Full Text].
Goda Y, Stevens C (1994) Two components of transmitter release at a central synapse. Proc Natl Acad Sci USA 91:12942-12946[Abstract/Free Full Text].
Golshani P, Jones E (1999) Synchronized paroxysmal activity in the developing thalamocortical network mediated by corticothalamic projections and "silent" synapses. J Neurosci 19:2865-2875[Abstract/Free Full Text].
Gomperts S, Rao A, Craig A, Malenka R, Nicoll R (1998) Postsynaptically silent synapses in single neuron cultures. Neuron 21:1443-1451[ISI][Medline].
Goodman C, Shatz C (1993) Developmental mechanisms that generate precise patterns of neuronal connectivity. Cell 72:77-98.
Gordon B, Kinch G, Kato N, Keele C, Lissman T, Fu LN (1997) Development of MK-801, kainate, AMPA, and muscimol binding sites and the effect of dark rearing in rat visual cortex. J Comp Neurol 383:73-81[Medline].
Hahm JO, Langdon RB, Sur M (1991) Disruption of retinogeniculate afferent segregation by antagonists to NMDA receptors. Nature 351:568-570[Medline].
Hahm JO, Cramer KS, Sur M (1999) Pattern formation by retinal afferents in the ferret lateral geniculate nucleus: developmental segregation and the role of N-methyl-D-aspartate receptors. J Comp Neurol 411:327-345[ISI][Medline].
Hamos JE, Van Horn SC, Raczkowski D, Sherman SM (1987) Synaptic circuits involving an individual retinogeniculate axon in the cat. J Comp Neurol 259:165-192[ISI][Medline].
Henderson Z, Finlay B, Wikler K (1988) Development of ganglion cell topography in ferret retina. J Neurosci 8:1194-1205[Abstract].
Hensch TK, Gordon JA, Brandon EP, McKnight GS, Idzerda RL, Stryker MP (1998) Comparison of plasticity in vivo and in vitro in the developing visual cortex of normal and protein kinase A RI $beta$ -deficient mice. J Neurosci 18:2108-2117[Abstract/Free Full Text].
Hestrin S (1992) Developmental regulation of NMDA receptor-mediated synaptic currents at a central synapse. Science 357:686-689.
Hohnke C, Sur M (1999a) Development of the visual pathways: effects of neural activity. Ment Retard Dev Disabil Res Rev 5:51-59.
Hohnke C, Sur M (1999b) The number and efficacy of single retinal axon inputs to cells in the ferret lateral geniculate nucleus during the development of ON/OFF sublamination. Soc Neurosci Abstr 25:1267.
Hohnke C, Sur M (1999c) Stable properties of spontaneous EPSCs and miniature retinal EPSCs during the development of ON/OFF sublamination in the ferret lateral geniculate nucleus. J Neurosci 19:236-247[Abstract/Free Full Text].
Hsia A, Malenka R, Nicoll R (1998) Development of excitatory circuitry in the hippocampus. J Neurophysiol 79:2013-2024[Abstract/Free Full Text].
Isaac J, Nicoll R, Malenka R (1995) Evidence for silent synapses: implications for the expression of LTP. Neuron 15:427-434[ISI][Medline].
Isaac J, Crair M, Nicoll R, Malenka R (1997) Silent synapses during development of thalamocortical inputs. Neuron 18:269-280[ISI][Medline].
Johnson J, Casagrande V (1993) Prenatal development of axon outgrowth and connectivity in the ferret visual system. Vis Neurosci 10:117-130[ISI][Medline].
Johnston D, Williams S, Jaffe D, Gray R (1992) NMDA-receptor-independent long-term potentiation. Annu Rev Physiol 54:489-505[ISI][Medline].
Jones E, Tighilet B, Tran B, Huntsman M (1998) Nucleus- and cell-specific expression of NMDA and non-NMDA receptor subunits in monkey thalamus. J Comp Neurol 397:371-393[ISI][Medline].
Kandel E, O'Dell T (1992) Are adult learning mechanisms also used for development? Science 258:243-245[Free Full Text].
Katz L, Shatz C (1996) Synaptic activity and the construction of cortical circuits. Science 274:1133-1138[Abstract/Free Full Text].
Kullmann D, Asztely F (1998) Extrasynaptic glutamate spillover in the hippocampus: evidence and implications. Trends Neurosci 21:8-14[ISI][Medline].
Lerma J, Herranz AS, Herreras O, Abraira V, Martin del Rio R (1986) In vivo determination of extracellular concentration of amino acids in the rat hippocampus. A method based on brain dialysis and computerized analysis. Brain Res 384:145-155[ISI][Medline].
Li P, Zhuo M (1998) Silent glutamatergic synapses and nociception in mammalian spinal cord. Nature 393:695-698[Medline].
Liao D, Hessler N, Malinow R (1995) Activation of postsynaptically silent synapses during pairing-induced LTP in CA1 region of hippocampal slice. Nature 375:400-404[Medline].
Liao D, Zhang X, O'Brien R, Ehlers M, Huganir R (1999) Regulation of morphological postsynaptic silent synapses in developing hippocampal neurons. Nat Neurosci 2:37-43[ISI][Medline].
Lin SY, Constantine-Paton M (1998) Suppression of sprouting: an early function of NMDA receptors in the absence of AMPA/kainate receptor activity. J Neurosci 18:3725-3737[Abstract/Free Full Text].
Malgaroli A (1999) Silent synapses: I can't hear you! Could you please speak aloud? Nat Neurosci 2:3-5[ISI][Medline].
Mammen AL, Huganir RL, O'Brien RJ (1997) Redistribution and stabilization of cell surface glutamate receptors during synapse formation. J Neurosci 17:7351-7358[Abstract/Free Full Text].
McAllister A, Katz L, Lo D (1996) Neurotrophin regulation of cortical dendritic growth requires activity. Neuron 17:1057-1064[ISI][Medline].
McCormick D, Pape H (1988) Acetylcholine inhibits identified interneurons in the cat lateral geniculate nucleus. Nature 334:246-248[Medline].
Miledi R (1966) Strontium as a substitute for calcium in the process of transmitter release at the neuromuscular junction. Nature 212:1233-1234.
Oliet SH, Malenka RC, Nicoll RA (1996) Bidirectional control of quantal size by synaptic activity in the hippocampus. Science 271:1294-1297[Abstract].
Oray S, Hohnke C, Sur M (1999) The ratio of AMPA to NMDA receptors in the ferret lateral geniculate nucleus during the development of ON/OFF sublamination. Soc Neurosci Abstr 25:1267.
Patneau D, Mayer M (1990) Structure-activity relationships for amino acid transmitter candidates acting at N-methyl-D-aspartate and quisqualate receptors. J Neurosci 10:2385-2399[Abstract].
Petralia R, Est