Postsynaptic Calcium Transients Evoked by Activation of Individual Hippocampal Mossy Fiber Synapses

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 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 Web of Science (24)

Citing Articles via Google Scholar

Google Scholar

Articles by Reid, C. A.

Articles by Fine, A.

Search for Related Content

PubMed

PubMed Citation

Articles by Reid, C. A.

Articles by Fine, A.

Previous Article  |  Next Article

The Journal of Neuroscience, April 1, 2001, 21(7):2206-2214

Postsynaptic Calcium Transients Evoked by Activation of Individual Hippocampal Mossy Fiber Synapses
Christopher A. Reid¹, Ruth Fabian-Fine², and Alan Fine¹^,³
¹ Division of Neurophysiology, National Institute for Medical Research, London NW7 1AA, United Kingdom, ² Department of Biological Sciences, The Open University, Milton Keynes MK7 6AA, United Kingdom, and ³ Department of Physiology and Biophysics, Faculty of Medicine, Dalhousie University, Halifax, Nova Scotia B3H 4H7, Canada

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Control of Ca²⁺ within dendritic spines is critical for excitatory synaptic function and plasticity, but little is known aboutCa²⁺ dynamics at thorny excrescences, the complex spines on hippocampalCA3 pyramidal cells contacted by mossy fiber terminals of dentategranule cell axons. We have monitored subthreshold stimulus-dependentpostsynaptic Ca²⁺ transients in optically and ultrastructurally characterized complexspines and find that such spines can act as discrete units ofCa²⁺ response. In contrast to the more common "simple" spines, synapticallyevoked Ca²⁺ transients at complex spines have only a small NMDA receptor-dependentcomponent and do not involve release of calcium from internalstores. Instead, they result mainly from AMPA receptor-gated Ca²⁺ influx through voltage-activated calcium channels on the spine;these channels provide graded amplification of the response ofthorny excrescences to individual mossy fiber synapticevents.

Key words: hippocampus; dendritic spine; mossy fiber synapse; CA3 pyramidal neuron; calcium dynamics; subthreshold stimulation; active spine membrane; voltage-activated calcium channels; thorny excrescence; electron microscopy

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Most excitatory synapses within the CNS are made on dendritic spines. The precise role of these structures is unknown, althoughthey are thought to act as compartments for postsynaptic integrationof biochemical signals (Segal, 1995; Denk et al., 1996; Shepherd,1996; Svoboda et al., 1996). Ca²⁺ acts as a key second messenger in many biochemical cascades,and the control of Ca²⁺ dynamics within spines is critical for certain forms of synapticplasticity (Bliss and Collingridge, 1993). Through the use ofintracellular fluorescent Ca²⁺ indicators, it is now possible to monitor the synaptic activationof individual dendritic spines (Müller and Connor, 1991; Malinowet al., 1994; Yuste and Denk, 1995; Emptage et al., 1999; Mainenet al., 1999), permitting the study of these processes with hithertounattainable spatialresolution.

Hippocampal CA3 pyramidal neurons have two quite different classes of spines. Commissural-associational and recurrent collateralinputs contact the more common form of structurally simple dendriticspines, found in abundance throughout most of the dendritic arbor.In contrast, dentate granule cell axons (mossy fibers) synapseon large and complex dendritic spines, known as thorny excrescences(Ramon y Cajal, 1911), located mainly on the proximal apical dendriteand soma (Chicurel and Harris, 1992). Multiple protrusions ofthese spines are interdigitated with protrusions of the largemossy fiber terminals, with discrete postsynaptic densities apposedto multiple presynaptic releasesites.

Several studies have described subthreshold stimulus-dependent postsynaptic Ca²⁺ transients at simple spines on hippocampal (Malinow et al., 1994;Yuste and Denk, 1995; Emptage et al., 1999; Mainen et al., 1999;Yuste et al., 1999; Kovalchuk et al., 2000) and neocortical (Koesterand Sakmann, 1998) pyramidal neurons. These Ca²⁺ transients appear primarily dependent on NMDA receptor-mediatedglutamatergic transmission (Emptage et al., 1999; Yuste et al.,1999), although the relative contributions of other sources ofCa²⁺, including voltage-activated calcium channels (VACCs) (Mageeet al., 1995; Schiller et al., 1998) and calcium-induced calciumrelease (CICR) from internal stores (Emptage et al., 1999; Kovalchuket al., 2000), iscontroversial.

Less is known about the control of postsynaptic Ca²⁺ dynamics at the complex mossy fiber synapse. Here, we show that complexspines at mossy fiber synapses can act as discrete units of Ca²⁺ response. Using pharmacological manipulations to establish therelative contributions of potential Ca²⁺ sources, we demonstrate that, in contrast to simple spines, synapticallyevoked Ca²⁺ transients at complex spines are only partially dependent onNMDA receptor activation and appear to result mainly from Ca²⁺ influx through VACCs activated by AMPA receptor-mediateddepolarization.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Preparation of organotypic hippocampal cultures. Transverse 350-µm-thick slices of hippocampus were cut from 8-d-old maleWistar rat pups and cultured on Millicell CM (Millipore, Bedford,MA) membranes at a gas-liquid interface (Stoppini et al., 1991)for 10-21 d beforeuse.

Electrophysiological and optical recording. Cultures on their supporting membrane were transferred to a recording chamberin which they were continually superfused with oxygenated (95%O₂-5% CO₂) artificial CSF (ACSF) maintained at 30°-32°C (temperaturecontroller; Scientific System Design, Montclair, NJ). A translationstage permitted the chamber and micromanipulators to be movedsmoothly as a unit. Except where noted, the ACSF contained (inmM): 120 NaCl, 3 KCl, 2 MgSO₄, 3 CaCl₂, 1.2 NaHPO₄, 23 NaHCO₃,11 glucose, and 1 of the anti-oxidant Trolox. Slices were viewedthrough a Leica (Wetzlar, Germany) DMLSF upright microscope usingan Olympus Optical (Tokyo, Japan) water-immersion 60× numericalaperture 0.9 objective and a Bio-Rad (Hercules, CA) MRC600 confocallaser scan head. Pyramidal cells in the CA3 region of organotypichippocampal cultures were impaled with sharp microelectrodes (100-180M $Omega$ , with filament) tip filled with 0.5-1 mM Oregon Green 488 BAPTA-1(Molecular Probes, Eugene, OR) in 200 mM potassium acetate andbackfilled with 4 M potassium acetate; N-(2,6-dimethylphenylcarbamoylmethyl)triethylammoniumbromide (QX-314) (50 mM) was included in some experiments. Tofacilitate subsequent preparation for electron microscopy (seebelow), microelectrodes in some cases also contained 2% CascadeBlue biocytin (Molecular Probes). The indicator was injected intothe cell by applying hyperpolarizing current (0.05-0.1 nA) for5-20 min via an Axoclamp 2B amplifier (Axon Instruments, FosterCity, CA). Stimuli (single 40-100 µsec square pulses, or pairsseparated by 70-75 msec) were delivered via a sharpened monopolartungsten stimulating electrode (A-M Systems, Carlsborg, WA) placedin the cell body layer of the dentate gyrus. The proximal regionof the apical dendrite of the CA3 pyramidal neuron was searchedwhile stimulating at ~0.05 Hz, until a spine exhibiting stimulus-evokedcalcium transients was found. Two-dimensional confocal scans lackthe temporal resolution required for accurate measurement of thesecalcium transients, so the confocal microscope was used in linescan mode. Line scans consisted of 256 successive sweeps, at 2msec intervals, across a single line in the field of view. Theorientation of the line was optimized using a scan rotator (ScientificSystem Design), and a custom-made time stamp was used to marka white line in the line scan, which coincided with the precisetime of stimulation. Electrophysiological data were captured usingA/DVANCE software (McKeller Designs, Vancouver, Canada), and imageswere collected using COMOS software (Bio-Rad). Images and electrophysiologicaldata were analyzed using NIH Image and Axograph (Axon Instruments)software, respectively. The calcium transient amplitudes wereexpressed as percent fractional change in fluorescence, calculatedas 100(F $-$ F_initial)/(F_initial $-$ F_background). To improve thesignal-to-noise ratio, we measured $Delta$ F/F over a 30 msec windowat the peak of the Ca²⁺ transient. Changes in $Delta$ F/F after drug manipulations were expressedas normalized percent relative to $Delta$ F/F before drug application(baseline); controls were exposed to ACSF changes at the correspondingtimes. Statistical comparisons were made with Student's t test,two-tailed except where indicated. 6-Cyano-7-nitroquinoxaline-2,3-dione(CNQX), D-( $-$ )-2-amino-5-phosphonovaleric acid (D-APV), (2S,2'R,3'R)-2-(2',3'-dicarboxycyclopropyl)glycine(DCG-IV), N-(4-hydroxyphenylpropanoyl)spermine trihydrochloride(HPP-spermine), (+)-5-methyl-10,11-dihydro-5H-dibenzo [a,d] cyclohepten-5,10-iminemaleate (MK-801), and QX-314 were obtained from Tocris Cookson(Ballwin, MO), Trolox was obtained from Aldrich (Milwaukee, WI),and all other reagents were obtained from Sigma (St. Louis,MO).

Electron microscopic visualization of characterized synapses. Cascade Blue-coinjected preparations were, after imaging andelectrophysiological recording, fixed in 3% paraformaldehyde-0.3%glutaraldehyde in 0.1 M PBS, pH 7.4, for 20 min at 4°C. Beforeosmication and embedding, the preparation was trimmed under fluorescencemicroscopic observation to include only the filled neuron andits immediate environs. The reduced preparation was rinsed inPBS (four times for 5 min each) and osmicated (0.5% OsO₄ in PBS)for 4-7 min. After subsequent rinsing in PBS (three times for5 min each), preparations were dehydrated in a graded series ofethanol and embedded in Araldite (Agar Scientific, Stansted, UK).The resin was polymerized overnight in embedding molds at 60°C.Serial ultrathin sections (75 nm) were cut with a Reichert Ultracutand collected on pioloform-coated single slot grids. Sectionswere contrasted with uranyl acetate and Reynold's lead citrateaccording to standard EM methods and were examined using a Jeol(Peabody, MA) JEM-1010 electronmicroscope.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of complex dendritic spines postsynaptic to mossy fiber terminals

Individual pyramidal cells in the CA3 region of organotypic hippocampal slice cultures were filled with the high-affinityfluorescent Ca²⁺ indicator Oregon Green 488 BAPTA-1 and imaged by laser-scanningconfocal microscopy (Fig. 1A). Visual criteria were used to identifydendritic spines postsynaptic to mossy fiber terminals; spineswere located on the proximal apical dendrite within 100 µm ofthe soma and were large, with heads 2-5 µm in diameter (Chicureland Harris, 1992). Furthermore, many of the spines investigatedhere could be seen by confocal microscopy to have a complex, lobularappearance (Fig. 2B). To maximize the likelihood of stimulatingmossy fibers, the extracellular stimulating electrode was placedin the dentate granule cell body layer (Fig. 1B) to elicit EPSPsin the impaled cell. The mossy fiber origin of the EPSP was supportedby its short latency and, pharmacologically, by inhibition ofthe synaptic response using DCG-IV (1 µM), a selective group IImetabotropic glutamate receptor (mGluR) agonist (EPSP amplitudesreduced to 8 ± 1% of control; p < 0.05; n = 3) (Fig. 1C); groupII mGluRs are expressed exclusively on mossy fiber terminals inCA3 (Kamiya et al., 1996; Shigemoto et al., 1997).

View larger version (26K):
[in this window]
[in a new window]
Figure 1. Identification of complex dendritic spines at mossy fiber synapses. A_i, A living CA3 pyramidal neuron in an organotypic hippocampal slice, after filling with the calcium indicator Oregon Green 488 BAPTA-1. The arrow indicates a complex spine on the primary apical dendrite of the CA3 pyramidal neuron. A_ii, Enlarged view showing the location, large size, and shape of the complex spine. B, Illustration of electrode placement in the organotypic hippocampal cultures. The stimulating electrode was positioned in the dentate granule cell body layer to maximize the likelihood of selectively stimulating the mossy fibers projecting from these cells to the proximal dendrites of CA3 pyramidal neurons. C, DCG-IV (1 µM), a selective group II metabotropic glutamate receptor agonist, significantly reduces the EPSP-IPSP, confirming its mossy fiber origin (*p < 0.05, significantly different from control). Inset traces show EPSP-IPSPs in the absence and presence of DCG-IV; resting potential, $-$ 76 mV.

View larger version (35K):
[in this window]
[in a new window]
Figure 2. Confocal imaging of calcium transients in individual complex spines, elicited by subthreshold EPSPs. A, Left, Calcium indicator-filled proximal dendritic segment of a CA3 pyramidal neuron. Two line scans along the trajectory indicated by the arrows are shown in A_i and A_ii. Below each line scan are the synchronously recorded somatic membrane potential (bottom black traces; note the compound synaptic response in A_i and A_ii, with a small EPSP immediately followed by a large IPSP) and the Ca²⁺ transients (top traces; expressed as fractional change in fluorescence, $Delta$ F/F) in the spine (black) and in the immediately subjacent dendritic shaft (red) at the levels of the top and bottom fiducial marks, respectively, in the left panel. The vertical white lines (time stamps) in the line scans mark the delivery of a single stimulus via the stimulating electrode in the granule cell layer to activate mossy fibers projecting to the imaged cell. The line scan in A_i shows an EPSCaT that is restricted to one thorny excrescence without spread to the dendritic shaft compartment. The line scan in A_ii illustrates a failure of afferent stimulation to elicit an EPSCaT, presumably attributable to the failure of transmitter release at the investigated spine. B, Left, Calcium indicator-filled region of a CA3 pyramidal cell body and proximal apical dendrite. Line scans along the trajectory indicated by the arrows demonstrate an EPSCaT, evoked by a subthreshold EPSP, restricted to a single thorny excrescence (B_i) at the level of the fiducial mark and a generalized Ca²⁺ transient in all structures in response to a suprathreshold EPSP (B_ii). C, Additional examples of EPSCaTs, evoked by single (C_i) or paired (C_ii; 75 msec interval) stimuli, restricted to a single thorny excrescence (top black traces; as measured at the level of the top fiducial mark in the left panel) without affecting Ca²⁺ fluorescence in the immediately subjacent dendritic shaft (red traces and bottom fiducial mark); figure elements as in A. In the example in C_ii, transmission at this synapse failed in response to the first of the paired stimuli. In the false color "thermal" lookup table used in these confocal images, increasing fluorescence is denoted by colors from black through red to yellow and white. Vertical calibration bar: top traces, A, 70% $Delta$ F/F; B, 100%; C, 50%; bottom traces, A, 5 mV; B_i, 2 mV; B_ii, 30 mV; C, 3 mV. The resting membrane potential was $-$ 77 mV for the cell in A, $-$ 77 mV for the cell in B, and $-$ 66 mV for the cell in C.

Single synaptic events elicit calcium transients within individual complex spines

Stimulation in the dentate granule cell layer resulting in subthreshold EPSPs in the indicator-filled CA3 pyramidal neuronswas typically found to be associated with a rapid increase inCa²⁺ indicator fluorescence in one or a few complex dendritic spines,as illustrated in Figure 2. The line scan trajectories, markedby the pairs of arrows, pass through a number of spines, of whichonly one in each case exhibited a rapid increase in fluorescenceafter some (Fig. 2Ai,Bi,Ci) but not all (Fig. 2Aii,Cii) afferentstimuli. In contrast, when the stimulus strength was increasedto elicit an action potential, all imaged spines (as well as thedendrite and soma) exhibited a simultaneous increase in fluorescence(Fig. 2Bii). The synaptically evoked postsynaptic Ca²⁺ transients (EPSCaTs) at these complex spines are large (fractionalchange in intensity, $Delta$ F/F = 84 ± 7%; n = 31), with a rapid rise(<8 msec) and slower decay ( $tau$ = 168 ± 16; n = 12). EPSCaT amplitudeswere not limited by saturation of the high-affinity Ca²⁺ indicator because, when stronger stimuli elicited action potentials(presumably by recruitment of additional fibers synapsing elsewhereon the cell) (Fig. 2Bii), this in all cases resulted in largerCa²⁺ transients at the interrogated spine (% $Delta$ F/F = 111 ± 14% for suprathresholdEPSPs vs 67 ± 9% for subthreshold EPSPs; p < 0.0005; n =13).

In over 90% of spines studied, the EPSCaT was restricted to the spine (Fig. 2Ai,Ci,Cii); in 11 cases in which the scan pathwas perpendicular to the long axis of the dendrite, the mean fluorescencetransient ( $Delta$ F/F) in the dendritic shaft directly beneath the spinewas 3.2 ± 1.6% compared with 92 ± 14% in the spine head. Theseobservations indicate that, as with more simple spines, the complex"thorny excrescence" spine is a discrete compartment of postsynapticCa²⁺response.

Calcium transients at thorny excrescences were not invariably evoked by every stimulus (Fig. 2Aii,Cii). We have demonstratedpreviously (Emptage et al., 1999) that the probability of obtainingan EPSCaT (p_Ca) can be used to estimate the transmitter releaseprobability (p_r) at simple synapses. Mossy fiber boutons displaymultiple discrete active zones (potential transmitter releasesites) opposite postsynaptic densities on CA3 complex spines (Chicureland Harris, 1992), so that the effective p_r at these synapsesis an aggregate probability reflecting both p_r at each releasesite and the total number of these sites. Paired-pulse facilitation,the phenomenon in which the EPSP to a second closely-followingstimulus is larger than that to the first, is believed to reflectan increase in p_r to the second stimulus when residual Ca²⁺ from the first impulse sums with Ca²⁺ from the second (Wu and Saggau, 1994). In general, mossy fibersynapses exhibited a high p_Ca; in 3 mM extracellular Ca²⁺, the average p_Ca was 0.84 ± 0.05 (n = 31 synapses). At six mossyfiber synapses in which p_Ca to single stimuli was <1, p_Ca increasedfrom the first stimulus to the second stimulus (0.31 ± 0.1 vs0.98 ± 0.02; p < 0.002) when paired stimuli were administeredwith a 70-75 msec interval (Fig. 2Cii). This demonstration ofpaired-pulse facilitation suggests that, in parallel with ourobservations at simple spines, p_Ca measured at complex spinesreflects p_r, the aggregate probability of transmitter releaseby all of the inputs to the imagedspine.

Ultrastructural confirmation of identification of complex spines as thorny excrescences postsynaptic to mossy fiber terminals

To confirm the identification of the optically characterized complex spines as thorny excrescences postsynaptic to mossy fibers,preparations were fixed after optical and electrophysiologicalrecording and processed for electron microscopy. Comparison withconfocal images allowed unambiguous identification of opticallycharacterized spines in serial ultrathin sections (Fig. 3). Thesespines (n = 3 preparations) all displayed complex lobular morphologyand received multiple synaptic contacts from presynaptic terminalscontaining clear round and dense-cored vesicles (Fig. 3D), characteristicof mossy fiber synapses in organotypic culture (Frotscher andGähwiler, 1988). These observations, in conjunction with theelectrophysiological and pharmacological observations describedabove, establish unambiguously that the complex spines monitoredhere by confocal microscopy are indeed thorny excrescences postsynapticto mossy fiber terminals.

View larger version (127K):
[in this window]
[in a new window]
Figure 3. The identity of optically characterized complex spines as postsynaptic to mossy fibers is confirmed by electron microscopy. A, Line scan (right) along the trajectory indicated by arrows in the left confocal image shows an EPSCaT in one complex spine (black-white arrowhead and fiducial mark) in response to dentate gyrus stimulation. Two adjacent complex spines (black arrowheads) are not activated. B, Electron micrograph of an ultrathin section through the same cell; correspondence with the optical images (inset and A) is evident. C, Higher magnification view of the region in B corresponding to the region outlined by white boxes in A and inset in B. The three complex spines labeled by arrowheads in A and B are indicated by corresponding arrowheads. D, Higher magnification image of an adjacent serial section, showing the activated spine indicated by the black-white arrowhead in A-C. Black-white arrowheads indicate two synapses onto the complex spine, made by terminals containing both clear and dense-cored vesicles. Scale bar: A, 9.5 µm; B, 6 µm; C, 1.8 µm; D, 0.5 µm; inset in B, 12 µm.

Contribution of ionotropic glutamate receptors to the calcium transient

Several mechanisms could underlie the rapid rise in Ca²⁺ at thorny excrescences. To establish the glutamatergic nature of theresponse, we examined the effect of the AMPA/kainate receptorantagonist CNQX (20 µM). CNQX abolished both the EPSP (7.1 ± 1.2mV reduced to $-$ 1.5 ± 1.2 mV; p < 0.005; n = 5) and the EPSCaT(0.6 ± 0.2% of initial, "baseline," amplitude; n = 5; p < 0.005)(Fig. 4A,C). This indicates that a CNQX-sensitive, presumablyAMPA receptor-mediated, local depolarization is essential forevoking EPSCaTs in complex spines. This depolarization could serveto open VACCs or to remove the voltage-dependent Mg²⁺ block of NMDA receptors. To test whether the activation of NMDAreceptors is responsible for the Ca²⁺ transient, we applied two different NMDA receptor antagonists.Both the irreversible NMDA receptor open-channel blocker MK-801(20 µM) and the competitive antagonist D-APV (20 µM) significantly,but only partially, reduced the Ca²⁺ transient (53 ± 14%, n = 4 and 58 ± 6%, n = 4 of baseline, respectively;p < 0.05 for the combined data compared with control) (Fig. 4B,C).These values, implying that up to 47% of the Ca²⁺ transient is NMDA-mediated, are overestimates, because simplyresampling without drugs leads to a small reduction in EPSCaTamplitude (87 ± 10% of baseline) (Fig. 4C, Control), presumablya consequence of indicator bleaching. Correction for this resamplingreduction suggests the NMDA-mediated component represents only~35% of the EPSCaT. In three cells in which APV was applied andstability maintained through drug washout, recovery of the Ca²⁺ transient was achieved after wash (to 87 ± 12% of baseline, i.e.,to control values for resampling) (Fig. 4Bii).

View larger version (24K):
[in this window]
[in a new window]
Figure 4. Ionotropic glutamate receptors mediate the Ca²⁺ signal seen at complex mossy fiber dendritic spines. A_i, The EPSCaT amplitude (% $Delta$ F/F) at an investigated thorny excrescence, and synchronously recorded somatic membrane potential (resting potential, $-$ 66 mV), in response to a single stimulus. The AMPA/kainate receptor antagonist CNQX (20 µM) abolishes both the EPSP and the Ca²⁺ signal; the IPSP component persists. A_ii, Summary histogram of the mean EPSCaT amplitude before, during, and after application of CNXQ (n = 5). Error bars represent SEM. B_i, The irreversible NMDA receptor antagonist MK 801 (20 µM) partially reduces the Ca²⁺ signal at the mossy fiber spines but does not significantly change the EPSP (resting potential, $-$ 73 mV). B_ii, Summary histogram of the mean EPSCaT amplitude before and after application of MK 801 (n = 4) and the reversible NMDA receptor antagonist APV (25 µM; n = 5), illustrating partial block of the signal by both drugs. C, Summary histogram of mean EPSCaT amplitudes (normalized to initial baseline EPSCaT amplitude) after different treatments. D, Mean peak synaptic response amplitude for the same series of experiments, normalized similarly. CNQX blocks the EPSP component of the compound synaptic waveform, whereas the other manipulations have no significant effect. Numbers in brackets indicate the number of experiments done for each group. *p < 0.05, significantly different from control.

What other sources could contribute to EPSCaTs at complex spines? One possibility is other ionotropic glutamate receptors;AMPA receptors lacking Q/R-edited GluR2 subunits are known tobe Ca²⁺-permeable (Hollmann et al., 1991; Jia et al., 1996). A possiblecontribution of this source to the EPSCaT was investigated byusing HPP-spermine (10 µM), a specific antagonist of Ca²⁺-permeable AMPA receptors (Washburn and Dingledine, 1996). Thisdrug had no effect on EPSCaT amplitudes (88.7 ± 17% of baseline)(Fig. 4C), consistent with previous reports that Ca²⁺-permeable AMPA receptors are not present at mossy fiber-CA3 pyramidalsynapses (Toth and McBain, 1998). Kainate receptors containingunedited versions of GluR5 and GluR6 subunits are also known tobe Ca²⁺-permeable (Hollmann et al., 1991). However, kainate-mediatedEPSCs at mossy fiber synapses have current-voltage relationshipsthat are linear or show slight outward rectification (Castilloet al., 1997; Vignes and Collingridge, 1997), characteristic ofCa²⁺-impermeable kainate receptors and in contrast to the strong inwardrectification exhibited by Ca²⁺-permeable kainate receptors (Burnashev et al., 1996). Furthermore,kainate receptor activation at the mossy fiber synapse requireshigh-frequency stimulation (Castillo et al., 1997; Vignes andCollingridge, 1997). Thus, it is unlikely that Ca²⁺-permeable kainate receptors contribute to the unitary EPSCaTsdescribedhere.

Contribution of voltage-activated calcium channels to the calcium transient

The local depolarization resulting from activation of AMPA receptors could generate the EPSCaT by opening VACCs. To test whetherVACCs contribute to the transient, we tested the effects of severalsubstances. The application of Ni²⁺ (100 µM), which blocks low-threshold T-type and high-thresholdR-type VACCs (Wu et al., 1998), reduced the amplitude of the Ca²⁺ signal slightly but not significantly (74 ± 3% of baseline; n= 4; p = 0.20) (Fig. 5B), indicating that these channels are unlikelyto contribute more than ~15% of the EPSCaT (after correcting forresampling). Nifedipine, at a concentration (20 µM) sufficientto reduce action potential-evoked Ca²⁺ transients at the soma by 49 ± 14% (n = 3), did not significantlyreduce EPSCaT amplitudes (89 ± 6% of baseline; n = 3; p = 0.46)(Fig. 5A), suggesting that L-type VACCs also do not contributesignificantly to the synaptically evoked Ca²⁺ transients in complex spines.

View larger version (19K):
[in this window]
[in a new window]
Figure 5. L-, T-, and R-type voltage-activated calcium channels are not major contributors to EPSCaTs at mossy fiber synapses. Summary histograms of mean EPSCaT amplitudes at complex spines (% $Delta$ F/F, normalized as in Fig. 4) (A) and synchronously recorded mean peak synaptic response amplitudes (normalized as percent of initial baseline synaptic response, as in Fig. 4) (B) after control change of ACSF or after application of the L-type VACC antagonist nifedipine (20 µM) or the T- and R-type VACC antagonist Ni²⁺ (100 µM). Both substances are without significant effect on either the EPSP or the Ca²⁺ transient.

Three additional VACCs remained to be considered: the high-voltage activated N-, P-, and Q-types. Because these channels areknown also to support transmitter release at mossy fiber terminals(Castillo et al., 1994), a direct evaluation of their effectson complex spine EPSCaTs is difficult. Therefore, to determinewhether high-threshold VACCs are present on complex spines, backpropagatingaction potentials were elicited by injecting a current pulse (40-80msec, 1 nA) into the CA3 pyramidal cell (Fig. 6B). The resultantCa²⁺ transient is independent of transmitter release and thereforeamenable to pharmacological manipulations that disrupt synaptictransmission. In all cases, the Ca²⁺ transient within the complex spine had the same onset latencyand kinetics as the transient generated in the dendritic shaft(Fig. 6A). This suggests that action potential-evoked Ca²⁺ influx into the spine results from the activation of channelson the spine itself rather than from diffusion of Ca²⁺ from the dendritic shaft (Svoboda et al., 1996), in agreementwith previous observations (Jaffe and Brown, 1997). The nonselectiveVACC blocker Cd²⁺ (50 µM) completely eliminated action potential-evoked Ca²⁺ transients at complex spines (0.2 ± 1% of baseline; n = 6; p< 0.0005) (Fig. 6B,C); the effect was seen even at complex spinesadjacent to the soma in which the block cannot be attributableto interference with action potential propagation. The wide-spectrumblocker of N-, P-, and Q-type VACCs, $omega$ -conotoxin MVIIC (2 µM)(McDonough et al., 1996), also substantially reduced the actionpotential-evoked Ca²⁺ transients at complex spines (49.0 ± 8% of baseline; n = 4; p< 0.02), providing additional evidence that these channels arepresent and functional at complex spines.

View larger version (17K):
[in this window]
[in a new window]
Figure 6. High-threshold voltage-activated calcium channels are present at thorny excrescences and are major contributors to the EPSCaT. A, Ca²⁺ indicator-filled complex spines on the proximal apical dendritic shaft of a CA3 pyramidal neuron (left). A line scan (right) along the trajectory indicated by the arrows in the left shows the Ca²⁺ transients elicited by an action potential triggered by a suprathreshold EPSP (stimulus to dentate gyrus at time marked by the vertical white line). The quantified transients in the spine (black) and subjacent dendritic shaft (red), at the levels in the left indicated by the top and bottom fiducial marks, respectively, are shown below the line scan, scaled to the same peak amplitude. The two traces are temporally indistinguishable, indicating that the Ca²⁺ transient arises independently in the spine and not by diffusion of Ca²⁺ from the dendritic shaft. B, The Ca²⁺ transient in an individual complex spine evoked by intrasomatic current injection (left top trace; % $Delta$ F/F) is entirely blocked by the broad-spectrum VACC antagonist Cd²⁺ (50 µM; right top trace); the synchronously recorded action potentials (bottom traces) are unaffected. The dotted line indicates the onset of the depolarizing current injection. Note that the second action potential at left is reflected in a second peak in the fluorescence trace, establishing that single action potentials do not saturate the indicator in these spines. The resting membrane potential was $-$ 73 mV for this cell. C, Summary histogram of amplitudes of action potential-evoked Ca²⁺ transients in complex spines (% $Delta$ F/F) showing reduction in the presence of Cd²⁺ (n = 6; p < 0.0005). D, EPSCaTs are wholly NMDA receptor-dependent at depolarized membrane potentials. Summary histograms comparing effects of APV on mean EPSCaT amplitudes (% $Delta$ F/F, normalized as in Fig. 4) with the cell at resting membrane potential and the greater reduction by APV during injection of depolarizing current to inactivate VACCs (*p < 0.005).

As an additional test of the involvement of VACCs in mediating complex spine EPSCaTs, VACCs were inactivated by depolarizingthe CA3 pyramidal cell. We reasoned that if VACCs are responsiblefor the NMDA receptor-independent component of the EPSCaT, thenunder experimental conditions in which VACCs are inactivated NMDAreceptor antagonists should entirely block the EPSCaT. Positivecurrent (0.05-0.2 nA) was injected into the neuron (with 50 mMQX-314 in the microelectrode to suppress action potentials), depolarizingthe membrane to $-$ 10 to $-$ 15 mV to inactivate VACCs. At these depolarizedmembrane potentials, APV completely blocked the EPSCaT ( $-$ 0.7 ±5% of baseline amplitude; n = 3; p < 0.005; compared with thesmaller APV block at resting membrane potentials, 58 ± 6% of baseline)(Fig. 6D). In conjunction with the lack of effect of Ni²⁺ and nifedipine, these experiments taken together support theconclusion that N-, P-, and/or Q-type high-threshold VACCs onthorny excrescences are activated by single synaptic events andare the major generators of EPSCaTs at thesespines.

Contribution of Ca²⁺ release from internal stores

Our previous observations on simple spines in CA3 and CA1 pyramidal cells indicated that EPSCaTs result from amplificationof NMDA receptor-mediated Ca²⁺ influx by the release of Ca²⁺ from internal stores within the spine (Emptage et al., 1999).To determine whether a similar amplification mechanism functionsat the mossy fiber synapse, we added ryanodine (20 µM) to thebathing medium. Ryanodine at this concentration binds to ryanodinereceptors (RyRs), blocking CICR from internal stores (McPhersonet al., 1991). In contrast to its nearly complete abolition ofEPSCaTs at simple spines, ryanodine had no effect on EPSCaTs atcomplex spines (% $Delta$ F/F = 100 ± 29% of baseline; n = 4; p = 0.40)(Fig. 7A), indicating that RyR-mediated CICR does not contributeto these Ca²⁺ transients. However, internal stores may also release Ca²⁺ via activation of IP₃ receptors by either IP₃ or Ca²⁺ (Berridge, 1993). To test this possibility, cyclopiazonic acid(CPA) (15-30 µM), a selective blocker of sarcoplasmic-endoplasmicreticulum Ca²⁺/ATPase (SERCA pumps) (Seidler et al., 1989), was used to depletethe smooth endoplasmic reticulum-derived Ca²⁺ stores. In contrast to simple spines, in which CPA abolishedEPSCaTs (Emptage et al., 1999), this drug did not decrease EPSCaTamplitudes at complex spines. Indeed, in striking contrast, CPAsignificantly increased EPSCaT amplitudes at complex spines [to124 ± 4% of baseline (equivalent to ~140% after correction forresampling); p < 0.05; n = 3] (Fig. 7A), presumably reflectinga role of stores in buffering synaptically evoked Ca²⁺ transients in the spines.

View larger version (19K):
[in this window]
[in a new window]
Figure 7. Ca²⁺-induced Ca²⁺ release from internal stores does not contribute to EPSCaTs at mossy fiber synapses. Summary histograms of mean EPSCaT amplitudes at complex spines (% $Delta$ F/F, normalized as in Fig. 3) (A) and synchronously recorded mean peak synaptic response amplitudes (normalized as percent of initial baseline synaptic response, as in Fig. 4) (B) after control change of ACSF or after application of CPA (20 µM), or the ryanodine receptor antagonist ryanodine (20 µM). Neither drug reduced EPSCaTs or influenced synaptic electrical responses, but CPA significantly increased the EPSCaT amplitude (*p < 0.05), indicating a role of store Ca²⁺ uptake in buffering Ca²⁺ transients within thorny excrescences.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Morphological studies including electron microscopy and Zn²⁺ histochemistry (Timm's staining) have demonstrated that mossy fiberterminals in organotypic hippocampal cultures maintain their normalcomplex structure and restricted distribution on CA3 pyramidalneurons (Robain et al., 1994; Pozzo Miller et al., 1996). Themorphology, location, and ultrastructure of the complex spinesstudied here and the DCG-IV sensitivity of the EPSP suggest thatthe anatomy and physiology of mossy synapses in these organotypiccultures parallels that in the intact brain. Strong, tetanic synapticstimulation has been shown previously to evoke Ca²⁺ transients in the proximal apical dendrite of these cells (PozzoMiller et al., 1996; Jaffe and Brown, 1997). Here, we have demonstratedthat subthreshold activation of mossy fiber synapses by singlestimuli produces postsynaptic Ca²⁺ transients restricted to the spine. Thus, these complex spines,like the morphologically simple spines more commonly found onhippocampal pyramidal neurons, can be considered minimal compartmentsof postsynaptic Ca²⁺ response (Yuste and Denk, 1995; Denk et al., 1996; Svoboda etal., 1996). The precise role of these localized Ca²⁺ transients is unresolved, but they are likely to mediate plasticas well as homeostatic processes in the spine. The increased resolutionof our observations has permitted a characterization of the pharmacologyof these Ca²⁺ transients, revealing that, in contrast to EPSCaTs at simplespines, single synaptically evoked Ca²⁺ transients at complex spines can be detected even in the absenceof NMDA receptor activation and have no calcium store component.This ancillary role of NMDA receptors in generating postsynapticCa²⁺ transients at mossy fiber synapses is consistent with the lowdensity of NMDA receptors found on complex spines (Monaghan etal., 1983; Jonas et al., 1993; Spruston et al., 1995) and, togetherwith the other results presented here, implies that EPSCaTs atthese synapses result mainly from AMPA-gated opening ofVACCs.

VACCs are known to be present on dendritic spines (Mills et al., 1994; Segal, 1995) and to be activated by backpropagatingaction potentials (Jaffe et al., 1994; Yuste and Denk, 1995),but whether they can be activated by subthreshold synaptic inputhas been controversial. The presence of VACCs endows the spinewith excitable membrane, and it has been suggested that excitatorysynaptic input may initiate action potentials in such excitablespines (Segev and Rall, 1998). The present results indicate thatVACCs on complex spines are indeed activated not only by backpropagatingaction potentials but also by subthreshold synaptic activation.However, the former generate larger amplitude calcium transientsin the spines than do the latter, implying that synaptic activationof spine VACCs is graded rather than all-or-none as has been suggestedpreviously on theoretical grounds (Segev and Rall, 1998).

We have not been able to specify the VACCs responsible for the mossy fiber EPSCaT. The failure of nifedipine to affect theseresponses while reducing somatic Ca²⁺ transients caused by action potentials is consistent with immunohistochemicalevidence that L-type VACCs occur predominantly on the soma, ratherthan dendrites, of CA3 neurons (Elliott et al., 1995). A substantialrole for low-threshold T-type and high-threshold R-type VACCswas eliminated by the lack of significant effect of Ni²⁺ on the EPSCaT. A definitive test of the selective involvementof the remaining VACCs, P-, Q-, and N-type, in generating thecomplex spine EPSCaT was precluded by the involvement of thesechannels in transmitter release from the mossy fiber terminal(Castillo et al., 1994). It was possible, however, to confirmthe presence of functional high-threshold VACCs on complex spines,because Cd²⁺ abolished, and $omega$ -conotoxin MVIIC reduced, action potential-elicitedCa²⁺ transients whose onset was too rapid to be attributable to diffusionof Ca²⁺ into the spines from the dendritic shaft (Svoboda et al., 1997).Furthermore, depolarization of the neuron to levels that shouldinactivate VACCs rendered EPSCaTs fully blockable by the NMDA-receptorantagonistAPV.

CPA increases the EPSCaT amplitude at complex spines, indicating that these spines contain internal calcium stores that function(at least at low-stimulation frequencies) mainly in buffering,rather than generating, these EPSCaTs. The considerable differencebetween sources of the synaptic Ca²⁺ transient at thorny excrescences (in which the Ca²⁺ comes mainly from VACCs, less from NMDA receptors, and not atall from CICR) and at simple spines [in which the transient arisesfrom NMDA receptor-mediated CICR, with minimal contribution fromVACCs (Emptage et al., 1999)] in the same CA3 pyramidal cellspresumably reflects a genuine difference between these types ofsynapse rather than a peculiarity of organotypic cultures (Kovalchuket al., 2000). Why spines on the same cell should differ in thisway is unclear. Activation of the mossy synapse, however, elicitsa much larger EPSP than does activation of commissural or collateralsynapses; this has led to the suggestion that mossy fiber inputmay serve as a "teacher" controlling plasticity at more distal,simple spine synapses (Marr, 1971; Carnevale et al., 1997; Henzeet al., 2000). The more proximal location of the mossy synapsemay contribute to its stronger effect on the postsynaptic cell(particularly in triggering action potentials), but so may amplificationof the response by the excitable complex spine. The greater synapticactivation of VACCs in thorny excrescences than in simple spinesmay in turn reflect the different geometry of these spines (Segevand Rall, 1988; Rusakov et al., 1996) or differences in densityor subtype of channels. Changes in the properties or deploymentof postsynaptic VACCs, no less than of glutamate receptors, couldcontribute to long-lasting synaptic plasticity (Shepherd et al.,1985).

  FOOTNOTES

Received Oct. 20, 2000; revised Dec. 15, 2000; accepted Dec. 22, 2000.

This work was supported by the Medical Research Council of the United Kingdom and the Human Frontier Science Program. C.A.R.is a Howard Florey Fellow of the Royal Society. We thank T. Bliss,N. Emptage, D. Rusakov, and M. Takahashi for helpful comments,and S. Dhanjal, G.-L. Raimondi, G. Roalfe, and the MechanicalEngineering Section of the National Institute for Medical Researchfor technicalassistance.
Correspondence should be addressed to Alan Fine, Division of Neurophysiology, National Institute for Medical Research, TheRidgeway, Mill Hill, London NW7 1AA, UK. E-mail: afine{at}nimr.mrc.ac.uk.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Berridge MJ (1993) Inositol trisphosphate and calcium signalling. Nature 361:315-325[Medline].
Bliss TV, Collingridge GL (1993) A synaptic model of memory: long-term potentiation in the hippocampus. Nature 361:31-39[Medline].
Burnashev N, Villarroel A, Sakmann B (1996) Dimensions and ion selectivity of recombinant AMPA and kainate receptor channels and their dependence on Q/R site residues. J Physiol (Lond) 496:165-173[Abstract/Free Full Text].
Carnevale NT, Tsai KY, Claiborne BJ, Brown TH (1997) Comparative electrotonic analysis of three classes of rat hippocampal neurons. J Neurophysiol 78:703-720[Abstract/Free Full Text].
Castillo PE, Weisskopf MG, Nicoll RA (1994) The role of Ca²⁺ channels in hippocampal mossy fiber synaptic transmission and long-term potentiation. Neuron 12:261-269[Web of Science][Medline].
Castillo PE, Malenka RC, Nicoll RA (1997) Kainate receptors mediate a slow postsynaptic current in hippocampal CA3 neurons. Nature 388:182-186[Medline].
Chicurel ME, Harris KM (1992) Three-dimensional analysis of the structure and composition of CA3 branched dendritic spines and their synaptic relationships with mossy fiber boutons in the rat hippocampus. J Comp Neurol 325:169-182[Web of Science][Medline].
Denk W, Yuste R, Svoboda K, Tank DW (1996) Imaging calcium dynamics in dendritic spines. Curr Opin Neurobiol 6:372-378[Web of Science][Medline].
Elliott EM, Malouf AT, Catterall WA (1995) Role of calcium channel subtypes in calcium transients in hippocampal CA3 neurons. J Neurosci 15:6433-6444[Abstract/Free Full Text].
Emptage N, Bliss TV, Fine A (1999) Single synaptic events evoke NMDA receptor-mediated release of calcium from internal stores in hippocampal dendritic spines. Neuron 22:115-124[Web of Science][Medline].
Frotscher M, Gähwiler BH (1988) Synaptic organization of intracellularly stained CA3 pyramidal neurons in slice cultures of rat hippocampus. Neuroscience 24:541-551[Web of Science][Medline].
Henze DA, Urban NN, Barrionuevo G (2000) The multifarious hippocampal mossy fiber pathway: a review. Neuroscience 98:407-427[Web of Science][Medline].
Hollmann M, Hartley M, Heinemann S (1991) Ca²⁺ permeability of KA-AMPA-gated glutamate receptor channels depends on subunit composition. Science 252:851-853[Abstract/Free Full Text].
Jaffe DB, Brown TH (1997) Calcium dynamics in thorny excrescences of CA3 pyramidal neurons. J Neurophysiol 78:10-18[Abstract/Free Full Text].
Jaffe DB, Fisher SA, Brown TH (1994) Confocal laser scanning microscopy reveals voltage-gated calcium signals within hippocampal dendritic spines. J Neurobiol 25:220-233[Web of Science][Medline].
Jia ZP, Agopyan N, Miu P, Xiong ZG, Henderson J, Gerlai R, Taverna FA, Velumian A, MacDonald J, Carlen P, Abramow-Newerly W, Roder J (1996) Enhanced LTP in mice deficient in the AMPA receptor GluR2. Neuron 17:945-956[Web of Science][Medline].
Jonas P, Major G, Sakmann B (1993) Quantal components of unitary EPSCs at the mossy fibre synapse on CA3 pyramidal cells of rat hippocampus. J Physiol (Lond) 472:615-663[Abstract/Free Full Text].
Kamiya H, Shinozaki H, Yamamoto C (1996) Activation of metabotropic glutamate receptor type 2/3 suppresses transmission at rat hippocampal mossy fibre synapses. J Physiol (Lond) 493:447-455[Abstract/Free Full Text].
Koester HJ, Sakmann B (1998) Calcium dynamics in single spines during coincident pre- and postsynaptic activity depend on relative timing of back-propagating action potentials and subthreshold excitatory postsynaptic potentials. Proc Natl Acad Sci USA 95:9596-9601[Abstract/Free Full Text].
Kovalchuk Y, Eilers J, Lisman J, Konnerth A (2000) NMDA receptor-mediated subthreshold Ca(2+) signals in spines of hippocampal neurons. J Neurosci 20:1791-1799[Abstract/Free Full Text].
Magee JC, Christofi G, Miyakawa H, Christie B, Lasser-Ross N, Johnston D (1995) Subthreshold synaptic activation of voltage-gated Ca²⁺ channels mediates a localized Ca²⁺ influx into the dendrites of hippocampal pyramidal neurons. J Neurophysiol 74:1335-1342[Abstract/Free Full Text].
Mainen ZF, Malinow R, Svoboda K (1999) Synaptic calcium transients in single spines indicate that NMDA receptors are not saturated. Nature 399:151-155[Medline].
Malinow R, Otmakhov N, Blum KI, Lisman J (1994) Visualizing hippocampal synaptic function by optical detection of Ca²⁺ entry through the N-methyl-D-aspartate channel. Proc Natl Acad Sci USA 91:8170-8174[Abstract/Free Full Text].
Marr D (1971) Simple memory: a theory for archicortex. Phil Trans Roy Soc Lond B Biol Sci 262:23-81[Abstract/Free Full Text].
McDonough SI, Swartz KJ, Mintz IM, Boland LM, Bean BP (1996) Inhibition of calcium channels in rat central and peripheral neurons by omega-conotoxin MVIIC. J Neurosci 16:2612-2623[Abstract/Free Full Text].
McPherson PS, Kim YK, Valdivia H, Knudson CM, Takekura H, Franzini-Armstrong C, Coronado R, Campbell KP (1991) The brain ryanodine receptor: a caffeine-sensitive calcium release channel. Neuron 7:17-25[Web of Science][Medline].
Mills LR, Niesen CE, So AP, Carlen PL, Spigelman I, Jones OT (1994) N-type Ca²⁺ channels are located on somata, dendrites, and a subpopulation of dendritic spines on live hippocampal pyramidal neurons. J Neurosci 14:6815-6824[Abstract].
Monaghan DT, Holets VR, Toy DW, Cotman CW (1983) Anatomical distributions of four pharmacologically distinct 3H-L-glutamate binding sites. Nature 306:176-179[Medline].
Müller W, Connor JA (1991) Dendritic spines as individual neuronal compartments for synaptic Ca²⁺ responses. Nature 354:73-76[Medline].
Pozzo Miller LD, Petrozzino JJ, Golarai G, Connor JA (1996) Ca²⁺ release from intracellular stores induced by afferent stimulation of CA3 pyramidal neurons in hippocampal slices. J Neurophysiol 76:554-562[Abstract/Free Full Text].
Ramon Y, Cajal S (1911) In: Histologie du Systeme Nerveux de l'Homme et des Vertebres. Paris: Maloine.
Robain O, Barbin G, Billette de Villemeur T, Jardin L, Jahchan T, Ben-Ari Y (1994) Development of mossy fiber synapses in hippocampal slice culture. Brain Res Dev Brain Res 80:244-250[Medline].
Rusakov DA, Stewart MG, Korogod SM (1996) Branching of active dendritic spines as a mechanism for controlling synaptic efficacy. Neuroscience 75:315-323[Web of Science][Medline].
Schiller J, Schiller Y, Clapham DE (1998) NMDA receptors amplify calcium influx into dendritic spines during associative pre- and postsynaptic activation. Nat Neurosci 1:114-118[Web of Science][Medline].
Segal M (1995) Dendritic spines for neuroprotection: a hypothesis. Trends Neurosci 18:468-471[Web of Science][Medline].
Segev I, Rall W (1988) Computational study of an excitable dendritic spine. J Neurophysiol 60:499-523[Abstract/Free Full Text].
Segev I, Rall W (1998) Excitable dendrites and spines: earlier theoretical insights elucidate recent direct observations. Trends Neurosci 21:453-460[Web of Science][Medline].
Seidler NW, Jona I, Vegh M, Martonosi A (1989) Cyclopiazonic acid is a specific inhibitor of the Ca²⁺-ATPase of sarcoplasmic reticulum. J Biol Chem 264:17816-17823[Abstract/Free Full Text].
Shepherd GM (1996) The dendritic spine: a multifunctional integrative unit. J Neurophysiol 75:2197-2210[Free Full Text].
Shepherd GM, Brayton RK, Miller JP, Segev I, Rinzel J, Rall W (1985) Signal enhancement in distal cortical dendrites by means of interactions between active dendritic spines. Proc Natl Acad Sci USA 82:2192-2195[Abstract/Free Full Text].
Shigemoto R, Kinoshita A, Wada E, Nomura S, Ohishi H, Takada M, Flor PJ, Neki A, Abe T, Nakanishi S, Mizuno N (1997) Differential presynaptic localization of metabotropic glutamate receptor subtypes in the rat hippocampus. J Neurosci 17:7503-7522[Abstract/Free Full Text].
Spruston N, Jonas P, Sakmann B (1995) Dendritic glutamate receptor channels in rat hippocampal CA3 and CA1 pyramidal neurons. J Physiol (Lond) 482:325-352[Abstract/Free Full Text].
Stoppini L, Buchs PA, Muller D (1991) A simple method for organotypic cultures of nervous tissue. J Neurosci Methods 37:173-182[Web of Science][Medline].
Svoboda K, Tank DW, Denk W (1996) Direct measurement of coupling between dendritic spines and shafts. Science 272:716-719[Abstract].
Svoboda K, Denk W, Kleinfeld D, Tank DW (1997) In vivo dendritic calcium dynamics in neocortical pyramidal neurons. Nature 385:161-165[Medline].
Toth K, McBain CJ (1998) Afferent-specific innervation of two distinct AMPA receptor subtypes on single hippocampal interneurons. Nat Neurosci 1:572-578[Web of Science][Medline].
Vignes M, Collingridge GL (1997) The synaptic activation of kainate receptors. Nature 388:179-182[Medline].
Washburn MS, Dingledine R (1996) Block of alpha-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid (AMPA) receptors by polyamines and polyamine toxins. J Pharmacol Exp Ther 278:669-678[Abstract/Free Full Text].
Wu LG, Saggau P (1994) Presynaptic calcium is increased during normal synaptic transmission and paired-pulse facilitation, but not in long-term potentiation in area CA1 of hippocampus. J Neurosci 14:645-654[Abstract].
Wu LG, Borst JG, Sakmann B (1998) R-type Ca²⁺ currents evoke transmitter release at a rat central synapse. Proc Natl Acad Sci USA 95:4720-4725[Abstract/Free Full Text].
Yuste R, Denk W (1995) Dendritic spines as basic functional units of neuronal integration. Nature 375:682-684[Medline].
Yuste R, Majewska A, Cash SS, Denk W (1999) Mechanisms of calcium influx into hippocampal spines: heterogeneity among spines, coincidence detection by NMDA receptors, and optical quantal analysis. J Neurosci 19:1976-1987[Abstract/Free Full Text].

Copyright © 2001 Society for Neuroscience 0270-6474/01/2172206-09$05.00/0

This article has been cited by other articles:

E. R. Kandel
The Biology of Memory: A Forty-Year Perspective
J. Neurosci., October 14, 2009; 29(41): 12748 - 12756.
[Abstract] [Full Text] [PDF]

M. T.-W. Ho, K. A. Pelkey, L. Topolnik, R. S. Petralia, K. Takamiya, J. Xia, R. L. Huganir, J.-C. Lacaille, and C. J. McBain
Developmental Expression of Ca2+-Permeable AMPA Receptors Underlies Depolarization-Induced Long-Term Depression at Mossy Fiber CA3 Pyramid Synapses
J. Neurosci., October 24, 2007; 27(43): 11651 - 11662.
[Abstract] [Full Text] [PDF]

C. A. Reid, D. B. Dixon, M. Takahashi, T. V. P. Bliss, and A. Fine
Optical Quantal Analysis Indicates That Long-Term Potentiation at Single Hippocampal Mossy Fiber Synapses Is Expressed through Increased Release Probability, Recruitment of New Release Sites, and Activation of Silent Synapses
J. Neurosci., April 7, 2004; 24(14): 3618 - 3626.
[Abstract] [Full Text] [PDF]

M. Tsukamoto, T. Yasui, M. K Yamada, N. Nishiyama, N. Matsuki, and Y. Ikegaya
Mossy fibre synaptic NMDA receptors trigger non-hebbian long-term potentiation at entorhino-CA3 synapses in the rat
J. Physiol., February 1, 2003; 546(3): 665 - 675.
[Abstract] [Full Text] [PDF]

W. Kakegawa, N. Yamada, M. Iino, K. Kameyama, T. Umeda, K. Tsuzuki, and S. Ozawa
Postsynaptic Expression of a New Calcium Pathway in Hippocampal CA3 Neurons and Its Influence on Mossy Fiber Long-Term Potentiation
J. Neurosci., June 1, 2002; 22(11): 4312 - 4320.
[Abstract] [Full Text] [PDF]

R. Fabian-Fine, P. Skehel, M. L. Errington, H. A. Davies, E. Sher, M. G. Stewart, and A. Fine
Ultrastructural Distribution of the {alpha}7 Nicotinic Acetylcholine Receptor Subunit in Rat Hippocampus
J. Neurosci., October 15, 2001; 21(20): 7993 - 8003.
[Abstract] [Full Text] [PDF]

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 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 Web of Science (24)

Citing Articles via Google Scholar

Google Scholar

Articles by Reid, C. A.

Articles by Fine, A.

Search for Related Content

PubMed

PubMed Citation

Articles by Reid, C. A.

Articles by Fine, A.