Presynaptic R-Type Calcium Channels Contribute to Fast Excitatory Synaptic Transmission in the Rat Hippocampus

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 (34)

Citing Articles via Google Scholar

Google Scholar

Articles by Gasparini, S.

Articles by Cherubini, E.

Search for Related Content

PubMed

PubMed Citation

Articles by Gasparini, S.

Articles by Cherubini, E.

Previous Article  |  Next Article

The Journal of Neuroscience, November 15, 2001, 21(22):8715-8721

Presynaptic R-Type Calcium Channels Contribute to Fast Excitatory Synaptic Transmission in the Rat Hippocampus
Sonia Gasparini¹, Alexander M. Kasyanov¹, Daniela Pietrobon², Leon L. Voronin³, and Enrico Cherubini¹
¹ Neuroscience Program and Istituto Nazionale Fisica della Materia Unit, International School for Advanced Studies, 34014 Trieste, Italy, ² Department of Biomedical Sciences, 35121 Padova, Italy, and ³ Brain Research Institute, Russian Academy of Medical Sciences, 103064 Moscow, Russia

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The possibility that R-type calcium channels contribute to fast glutamatergic transmission in the hippocampus has been assessedusing low concentrations of NiCl₂ and the peptide toxin SNX 482,a selective antagonist of the pore-forming $alpha$ _1E subunit of R-typecalcium channel. EPSPs or EPSCs were recorded in the whole-cellconfiguration of the patch-clamp technique mainly from CA3 hippocampalneurons. Effects of both NiCl₂ and SNX 482 were tested on large(composite) EPSCs evoked by mossy and associative-commissuralfiber stimulation. NiCl₂ effects were also tested on minimal EPSPs-EPSCs.Both substances reduced the amplitude of EPSPs-EPSCs. This effectwas associated with an increase in the number of response failuresof minimal EPSPs-EPSCs, an enhancement of the paired-pulse facilitationratios of both minimal and composite EPSCs, and a reduction ofthe inverse squared coefficient of variation (CV²). The reduction of CV² was positively correlated with the decrease in EPSC amplitude.The inhibitory effect of NiCl₂ was occluded by SNX 482 but notby $omega$ -conotoxin-MVIIC, a broad-spectrum antagonist thought to interactwith N- and P/Q-type calcium channels, supporting a specific actionof low concentrations of NiCl₂ on R-type calcium channels. Together,these observations indicate that both NiCl₂ and SNX 482 act atpresynaptic sites and block R-type calcium channels with pharmacologicalproperties similar to those encoded by the $alpha$ _1E gene. These channelsare involved in fast glutamatergic transmission at hippocampalsynapses.

Key words: hippocampus; mossy fibers; associative-commissural fibers; single-fiber EPSPs; single-fiber EPSCs; composite EPSC; $omega$ -conotoxin-MVIIC; SNX 482

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Synaptic transmission is triggered by calcium entry through voltage-dependent calcium channels (VDCCs) into presynaptic nerveterminals (Katz, 1969). Using type-specific calcium channel blockers,it has been found that most VDCCs involved in transmitter releasein the mammalian CNS belong to N- and P/Q-type channels (Takahashiand Momiyama, 1993; Wheeler et al., 1994; Dunlap et al., 1995).These channels are localized at presynaptic release sites at whichthey synergistically control synaptic function. The relationshipbetween presynaptic calcium concentration ([Ca²⁺]) and transmitter release is nonlinear and can be approximatedby a power function with the exponent that typically varies between3 and 4 in different synapses (Dodge and Rahamimoff, 1967; Augustineand Charlton, 1986; Takahashi and Momiyama, 1993; Wu and Saggau,1997). The relative contribution of VDCCs to transmitter releasecan be estimated by monitoring changes in [Ca²⁺] in presynaptic nerve endings, loaded with calcium indicatorsin the presence of selective VDCC antagonists. Using this method,Wu and Saggau (1995) have found that, at hippocampal CA3-CA1 synapses,complete block of both N- and P/Q-type VDCCs with $omega$ -conotoxin-MVIIC( $omega$ -CTx-MVIIC) does not completely suppress presynaptic calciumtransient. This indicates that, in addition to N- and P/Q-type,other VDCC types contribute to presynaptic calcium entry and fastglutamatergic synaptic transmission (Luebke et al., 1993; Takahashiand Momiyama, 1993; Wu and Saggau, 1995). Approximately one-quarterof presynaptic calcium influx is resistant to $omega$ -CTx-MVIIC in bothhippocampus (Wu and Saggau, 1995) and cerebellum (Mintz et al.,1995). The residual $omega$ -CTx-MVIIC-resistant calcium transient mightbe mediated by T- or R-type VDCCs (Wu and Saggau, 1994, 1995;Mintz et al., 1995, 1997). However, the involvement of T-typeVDCC seems unlikely because this channel type is localized mainlyon the soma and dendrites (Huguenard, 1996; Craig et al., 1999).A possible candidate is the R-type VDCC first described by Zhanget al. (1993) and involved in excitation-secretion coupling inboth central neurons and chromaffin cells (Wu et al., 1998; Wanget al., 1999; Albillos et al., 2000).

In the present experiments, we have investigated whether R-type calcium channels contribute to trigger transmitter releaseat hippocampal mossy and associative-commissural fibers synapses.To this aim, we have used low concentrations of NiCl₂ and thepolypeptide toxin SNX 482, a selective antagonist of recombinant $alpha$ _1E channels (Newcomb et al., 1998), which inhibits some nativeR-type channels (Wang et al., 1999; Tottene et al., 2000). Wefound that, at these synapses, R-type calcium channels constitutea significant fraction of presynaptic VDCCs controlling fast glutamatergictransmission.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Slice preparation. Experiments were performed on hippocampal slices obtained from postnatal day 14 (P14) to P19 Wistar ratsas described previously (Gasparini et al., 2000). Briefly, animalswere decapitated after being anesthetized with an intraperitonealinjection of urethane (2 gm/kg). The brain was quickly removedfrom the skull and placed in an ice-cold artificial CSF (ACSF)containing (in mM): 130 NaCl, 3.5 KCl, 1.2 NaH₂PO₄, 25 NaHCO₃,1.3 MgCl₂, 2 CaCl₂, and 11 glucose (saturated with 95% O₂ and5% CO₂), pH 7.3-7.4. Transverse hippocampal slices (300-400 µmthick) were cut with a vibratome and stored at room temperaturein a holding bath containing the same saline solution as above.After a recovery period of at least 1 hr, an individual slicewas transferred to the recording chamber in which it was continuouslysuperfused with oxygenated ACSF at a rate of 2-3 ml/min.

Electrophysiological recordings. EPSPs or EPSCs were recorded at 32°C from CA1 or CA3 pyramidal neurons using the patch-clamptechnique in the whole-cell configuration. Patch pipettes werefilled with a solution containing (in mM): 125 Cs-methanesulphonate,10 CsCl, 10 HEPES, 0.6 EGTA, 5 N-(2,6-dimethylphenylcarbamoylmethyl)triethylammonium-bromide(Alomone Labs, Jerusalem, Israel), 2 MgATP, and 0.3 NaGTP (resistanceof 3-5 M $Omega$ ). Bicuculline methiodide (5-10 µM) (Sigma-Aldrich, Milan,Italy), 3-[(R)-2-carboxypiperazin-4-yl]-propyl-1-phosphonic acid(20 µM; Tocris Cookson, Bristol, UK), and tetrodotoxin (10 nM;Affiniti Research Products, Exeter, UK) were routinely added tothe bathing solution to block GABA_A and NMDA receptors and toreduce polysynaptic activity, respectively. Bipolar twisted NiCr-insulatedelectrodes were placed in stratum radiatum to activate Schaffercollaterals in the CA1 region and associative-commissural fibersin the CA3 area or in stratum lucidum to stimulate mossy fibers(MFs). Paired stimuli (50 msec interval, 100 µsec duration) wereusually applied at 0.05 Hz (or 0.1 Hz in the case of pressureapplication of drugs). Two sets of experiments were performedwith recordings of large (composite) EPSCs and minimal EPSPs-EPSCs,respectively. In the first set of experiments, stimulation intensitywas adjusted to evoke composite (multifibers) EPSCs with no responsefailures. In another set, minimal afferent stimulation was usedto activate one or few fibers. The minimal EPSPs-EPSCs were associatedwith occasional response failures. Their number was usually estimatedby visual discrimination. MF-EPSCs were characterized by theirfast rise time and by their sensitivity to (2S,2'R,3'R)-2-(2',3'-dicarboxycyclopropyl)glycine(DCG-IV) (1 µM; Tocris Cookson), a selective agonist of metabotropicglutamate receptors (mGluRs) 2/3, known to selectively block mossyfibers transmission (Kamiya et al., 1996), whereas associative-commissuralfiber EPSPs were characterized by their slower rise time and theirresistance to DCG-IV (Berretta et al., 2000). Because the effectsof NiCl₂ on MF-EPCSs and associative-commissural fiber-EPSCs werevery similar, data obtained from activation of these two inputswere pooledtogether.

NiCl₂ was applied either in the bath via a three-way tap system or by pressure (5-10 psi) from a glass pipette (outer diameter,5-10 µm) positioned close to the recording cell. In the bath,NiCl₂ was applied at concentrations of 30-50 µM and usually startedto produce an effect after 2-3 min. Therefore, responses obtainedduring bath application of NiCl₂ were averaged only starting fromthe third minute of NiCl₂ application. Lower concentrations ofNiCl₂ (10 µM) did not produce any effect. We did not use higher(100 µM) concentrations of this divalent cation to avoid interferencewith other types of channels. Pressure application facilitatedaccessibility of NiCl₂ to the cell membrane and reduced the applicationtime (Miledi and Thies, 1971). In these experiments, the concentrationof NiCl₂ in the pipette was raised 10 times to obtain the sameblocking effect as with bath application. $omega$ -Conotoxin-MVIIC (BachemAG, Bubendorf, Switzerland) and SNX 482 (gift of G. Miljanichand L. Nadasdi, Elan Pharmaceuticals Inc., Menlo Park, CA) wereapplied by pressure. In some of these experiments, when two inputs(MFs and associative-commissural fibers) were alternatively activated,drugs delivered through the pressure pipette were found to affect,in the majority of the cases, only EPSCs evoked by stimulationof nerve fibers running closer to the tip of the pipette. A subsequentdisplacement of the pipette closer to the other afferent pathwaywas able to suppress EPSCs elicited by stimulation of the secondinput.

Rise and decay time constants were evaluated on average responses, using a single exponential fit. Paired-pulse facilitation(PPF) was measured as the ratio between the amplitude of the secondand first response before and during drug application after averagingall respective traces. In some (n = 21) experiments, the coefficientof variation (CV) of response amplitude was determined as CV =SD/mean, and its inverse squared value (CV²) was calculated. This measure is traditionally used to detectchanges in presynaptic transmitter release (Katz, 1969; Voronin,1993; Chavez-Noriega and Stevens, 1994) (for limitations, seeFaber and Korn, 1991).

Data are presented as mean ± SEM. Statistical comparisons were made with the use of paired t test or Wilcoxon signed ranktest (p < 0.05 was taken assignificant).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

NiCl₂ reduces composite EPSCs evoked by stimulation of mossy or associative-commissural fibers

Bath application of NiCl₂ at concentrations (30-50 µM) known to block some R-type calcium channels (Randall and Tsien, 1995;Tottene et al., 2000) significantly (p < 0.005) depressed themean peak amplitude of composite EPSCs, elicited by stimulationof mossy or associative-commissural fibers in CA3 pyramidal neuronsfrom 77.0 ± 12.6 to 45.9 ± 9.0 pA (n = 5) (Fig. 1). NiCl₂ inducedalso a significant (p < 0.05) increase in the paired-pulse facilitationratio from 1.62 ± 0.22 to 2.14 ± 0.30 (n = 4) (Fig. 1D). The effectof NiCl₂ was not associated with significant changes in holdingcurrent (values before and during NiCl₂ were $-$ 123.4 ± 14.8 and $-$ 130.9 ± 12.6 pA, respectively; p > 0.05) or membrane input resistance(293.5 ± 9.1 and 287.4 ± 14.8 M $Omega$ , before and during NiCl₂ application,respectively; p > 0.5). The kinetic properties of the EPSCs beforeand during NiCl₂ application were examined in five cells. As exemplifiedin Figure 1A, no significant (p > 0.5) modifications in the riseor decay time constants were detected (the mean rise and decaytime constants were 3.5 ± 0.5 and 3.4 ± 0.5 msec or 12.6 ± 2.3and 11.0 ± 1.2 msec before and during NiCl₂, respectively). Asillustrated in Figure 1B, the effects of NiCl₂ were only partiallyreversible.

View larger version (32K):
[in this window]
[in a new window]
Figure 1. NiCl₂ reduces the amplitude of composite EPSCs. A, Average of EPSCs evoked in a CA3 neuron by stimulation of mossy fibers in control conditions (40 traces; left) and in the presence of NiCl₂ (24 traces; middle). On the right, EPSCs (to the first stimulus) recorded in control conditions and in the presence of NiCl₂ have been averaged, normalized, and superimposed. B, Plot of EPSC1 (filled symbols) and EPSC2 (open symbols) amplitude versus time before, during (horizontal bar), and after application of NiCl₂. C, Mean peak amplitude of the first EPSC before (white column) and during (black column) superfusion of NiCl₂ (n = 5). D, Mean paired-pulse facilitation ratio in control conditions and during NiCl₂ application (n = 4). In this and the following figures, error bars refer to SEM. *p < 0.05; **p < 0.005.

In three cases in which NiCl₂ was tested on composite EPSCs evoked in CA1 neurons by stimulation of Schaffer collaterals,it reduced the mean amplitude EPSCs by 26.8 ± 14.7% (n =3).

Pressure application of NiCl₂ induces a reversible reduction of composite EPSCs

Poor accessibility of divalent cations to the cell membrane may account for the slow onset and the only partial washout ofNiCl₂ effects (Miledi and Thies, 1971). To facilitate accessibilityand to reduce the time of application, in another set of experiments,NiCl₂ was applied by pressure from a glass pipette positionedclose to the recording cell. To obtain the same inhibition aswith bath application, it was necessary to raise 10 times theconcentration of NiCl₂ in the pipette, which therefore was 300µM. In the example shown in Figure 2, pressure application ofNiCl₂ reduced the peak amplitude of the EPSCs evoked in a CA1pyramidal cell by stimulation of the Schaffer collateral by 45.3%,and this effect was almost completely reversed during washout.NiCl₂ produced also an increase in the paired-pulse facilitationratio from 1.4 to 2.1. On average, in three CA1 cells, NiCl₂ reducedthe peak amplitude of EPSCs evoked by Schaffer collateral stimulationby 40.5 ± 5.2% and increased the paired-pulse facilitation ratiofrom 1.7 ± 0.1 to 2.2 ± 0.3 (data not shown). In 10 CA3 neurons,NiCl₂ significantly (p < 0.001) reduced the mean amplitude ofEPSCs evoked by mossy fiber stimulation by 46.2 ± 2.4% and increasedthe paired-pulse facilitation ratio from 1.5 ± 0.1 to 1.8 ± 0.3(Fig. 2C,D).

View larger version (29K):
[in this window]
[in a new window]
Figure 2. Pressure application of NiCl₂ reversibly reduces the peak amplitude of composite EPSCs evoked in a CA1 pyramidal neuron by stimulation of the Schaffer collateral. A, Average of 10 EPSCs recorded in control conditions, in the presence of NiCl₂, and during washout. NiCl₂ reduced the amplitude of the first EPSC from 77.7 to 42.5 pA. B, The amplitudes of EPSC1 (filled symbols) and EPSC2 (open symbols) are plotted against time before, during (horizontal bar), and after application of NiCl₂. The concentration of NiCl₂ in the pressure pipette was 300 µM. C, Mean peak amplitude of EPSC1 evoked in CA3 neurons by stimulation of mossy fibers in control conditions (white column) and during (black column) superfusion of NiCl₂ (n = 10). D, Mean paired-pulse facilitation ratio of mossy fiber EPSCs in control conditions and during NiCl₂ application (n = 10). **p < 0.001.

The neurotoxin SNX 482 depresses EPSCs evoked by stimulation of the mossy and associative-commissural fibers

SNX 482, a toxin isolated from the tarantula Histerocrates gigas venom, at low concentrations, is a selective antagonist ofrecombinant VDCCs containing $alpha$ _1E subunits and inhibits some nativeR-type channels (Newcomb et al., 1998; Wang et al., 1999; Totteneet al., 2000). To see whether R-type calcium channels containingthe $alpha$ _1E subunit contribute to glutamate release in the hippocampus,SNX 482 at 0.3 or 1 µM was applied by pressure from a pipettelocated close to the mossy fibers in the vicinity of the patchedcell. These concentrations should be equivalent to 30 and 100nM toxin applied by bath perfusion (see Materials and Methods).Figure 3, A and C, shows the effects of SNX 482 (1 µM) on theamplitude of EPSCs evoked in a CA3 neuron by mossy fiber stimulation.The toxin reduced the peak amplitude of the EPSC by 62.7%. Theeffect of the toxin was localized; EPSCs evoked in the same neuronby stimulation of the associative-commissural fibers were unaffected(Fig. 3B,D). The mean peak amplitude of the associative-commissuralEPSC was 59.0 and 58.8 pA before and after SNX 482, respectively.However, when the pressure pipette was moved closer to the associative-commissuralfiber terminals, a 54.9% reduction of EPSCs amplitude was observed(data not shown). Overall, in seven CA3 cells, SNX 482 (1 µM)produced a reduction of the peak EPSC amplitude of 55.9 ± 4.5%.A slightly weaker effect on EPSC amplitude (42.3 ± 2.9% reduction)was induced by lower concentrations of SNX 482 (0.3 µM; n = 14).The blocking effect produced by the toxin was very similar tothat obtained with NiCl₂ and was irreversible. The decrease inthe mean EPSC amplitude produced by SNX 482 (1 µM) was accompaniedby an increase in the paired-pulse facilitation ratio in fourof seven cells tested. However, the mean increase in the PPF ratiodid not reach statistical significance (Fig. 3E). Therefore, tofurther test the involvement of presynaptic mechanisms in SNX482 action, an additional analysis based on calculation of theinverse squared coefficient of variation of response amplitude(CV²; see Materials and Methods) was performed. CV² decreased in all cells tested with 1 µM drug concentration (n= 7) and in the majority of the cells tested with 0.3 µM (n =11/14) (Fig. 3F). Importantly, the reduction of CV² produced by SNX 482 significantly correlated with the decreasein the mean amplitude of EPSCs (r = 0.43; n = 21; p < 0.05; one-tailedtest). These observations support a presynaptic site of actionof the toxin.

View larger version (28K):
[in this window]
[in a new window]
Figure 3. Pressure application of the toxin SNX 482 close to mossy fiber terminals reduces the peak amplitude of mossy but not associative-commissural fiber EPSCs. A, Average of composite EPSCs evoked in a CA3 neuron by stimulation of the mossy fibers before (left) and during (right) SNX 482 application. C, Plot of the peak amplitude of EPSC1 (filled symbols) and EPSC2 (open symbols) before and during application of SNX 482 (horizontal bar; concentration of SNX 482 into the pressure pipette, 1 µM). B, D, Similar presentation for EPSCs evoked in the same CA3 neuron by stimulation of associative-commissural fibers. Note that SNX 482 reduced the amplitude of mossy fiber EPSCs but did not affect associative-commissural EPSCs (mean peak amplitude values before and during SNX 482 were 76.7 and 26.5 pA for mossy fiber EPSCs and 59.0 and 58.8 pA for associative-commissural fiber EPSCs). Mean PPF ratio of mossy fiber EPSCs recorded in seven CA3 pyramidal cells before and during toxin application. F, Plot of the ratio of CV² (toxin over control) versus relative EPSC amplitudes (expressed as the ratio of the amplitude during SNX 482 application to the baseline amplitude). The regression line has been fitted through the data (least-square approximation; regression coefficient is 0.43; p < 0.05). Each symbol represents one cell (n = 21).

If NiCl₂ and SNX 482 act on the same target, namely on the $alpha$ _1E subunit of the R-type of calcium channel, application of NiCl₂(30 µM) after the toxin should not produce any additional effect.Indeed in five cases, bath application of NiCl₂ after the toxindid not significantly (p > 0.1) modify the EPSC amplitude, suggestingthat both the toxin and the divalent cation act on the same target.The mean peak amplitude reduction of the EPSCs was 37.8 ± 3.1%after application of SNX 482 (0.3 µM) and 50.4 ± 6.4% after additionof NiCl₂ (Fig. 4A).

View larger version (17K):
[in this window]
[in a new window]
Figure 4. Occlusion between the effects of SNX 482 and NiCl₂ indicates a common site of action. A, Examples of composite EPSC (average of 10 traces) evoked in a CA3 pyramidal neuron by stimulation of mossy fibers before (left) and during (middle) pressure application of SNX 482 (concentration in the pipette, 0.3 µM). Nine minutes after toxin application, superfusion of NiCl₂ (30 µM) did not affect the amplitude or shape of the EPSC (right). EPSC peak amplitude values were 94.5, 58.0, and 55.0 pA in control, in SNX 482 and in NiCl₂, respectively. B, Summary data from five cells. Differences in percentage block between SNX 482 and NiCl₂ are not statistically significant (p > 0.1). C, Composite EPSCs (average of 10 responses) evoked in a CA3 pyramidal neuron by stimulation of mossy fibers before (left) and during (middle) pressure application of $omega$ -CTx-MVIIC (concentration in the pipette, 10 µM). Ten minutes after the toxin, bath application of NiCl₂ (30 µM) produced an additional reduction of EPSC amplitude (right). EPSCs peak amplitude values were 103.4, 33.8, and 12.0 pA in control, in $omega$ -CTx-MVIIC, and in NiCl₂, respectively. D, Summary data from five cells. Differences in percentage block between $omega$ -CTx-MVIIC and NiCl₂ were statistically significant (p < 0.001).

As a control for the above occlusive interaction, we performed additional experiments (n = 5) using $omega$ -conotoxin-MVIIC knownto block N- and P/Q-type calcium channels (Wu and Saggau, 1995).In line with previous reports (Wu and Saggau, 1995), pressureapplication of the toxin (concentration in the pressure pipette,10 µM) produced a 66.1 ± 2.8% reduction of the peak amplitudeEPSC, which was irreversible. When NiCl₂ (30 µM) was applied inthe bath after $omega$ -conotoxin-MVIIC, an additional significant (p< 0.001) reduction of EPSC amplitude to 90.2 ± 3.6% was observed(Fig. 4B). This indicates that NiCl₂ at this concentration suppressesa set of channels different from that blocked by $omega$ -conotoxin-MVIIC.The small EPSC that remains after $omega$ -conotoxin-MVIIC and NiCl₂might be mediated by R-type calcium channels less sensitive toNiCl₂, as suggested by previous experiments at the calyx synapsesin the rat medial nucleus of the trapezoid body (Wu et al., 1998).

The data presented so far clearly show that presynaptic $alpha$ _1E channels contribute to glutamate release at mossy and associative-commissuralfiber synapses. The question then rises whether all presynapticterminals could have R-type channels commingled with N- and P/Q-typeor approximately half of all terminals could have only R-typechannels, whereas the other half posses only N- and P/Q-type.To address this point, another set of experiments using minimalstimulation, which presumably activates only a few afferent fibersor even a single fiber, were performed. In these experiments,we used NiCl₂ at concentrations (30-50 µM) known to block thesame R-type calcium channels inhibited by SNX 482 (see occlusionby SNX 482 on NiCl₂block).

NiCl₂ depresses EPSPs or EPSCs evoked by minimal stimulation of the mossy or associative-commissural fibers

Figure 5 (control) exemplifies EPSPs evoked by minimal stimulation of the associative-commissural fibers at resting membranepotentials (ranging from $-$ 58 to $-$ 63 mV). The EPSPs fluctuatedin amplitude from trial to trial with occasional failures. Whentwo stimuli were applied at 50 msec intervals, the second onetriggered higher-amplitude responses, with a reduced number offailures. EPSPs were completely blocked by CNQX (10 µM), indicatingthat they were generated by glutamate acting on non-NMDA receptors(data not shown). Bath application of NiCl₂ (30-50 µM) significantlyreduced the peak amplitude of the EPSPs evoked by mossy or associative-commissuralfibers by ~50% (Fig. 5D) in 13 of 15 recorded cells (in two cells,NiCl₂ was ineffective). Thus, during NiCl₂ application, the meanEPSP amplitudes changed from 0.77 ± 0.15 to 0.38 ± 0.11 mV (n= 13; p < 0.001) (Fig. 5D). This effect was associated with asignificant increase in the number of failures from 19 ± 3 to44 ± 6% (n = 13; p < 0.001) (Fig. 5E) and in the paired-pulsefacilitation ratio from 2.5 ± 0.4 to 3.5 ± 0.9 (n = 12; p < 0.05)(Fig. 5F). NiCl₂ did not affect membrane input resistance; itwas 220 ± 32 and 273 ± 28 M $Omega$ before and during NiCl₂ application,respectively (n = 13; p > 0.5).

View larger version (34K):
[in this window]
[in a new window]
Figure 5. NiCl₂ reduces the peak amplitude of EPSPs evoked in a CA3 pyramidal neuron by minimal stimulation of the associative-commissural fibers. A, Ten individual traces obtained by paired stimuli (50 msec interval) delivered to associative-commissural fibers at 0.05 Hz from $-$ 60 mV in control conditions, during NiCl₂ perfusion, and 13 min after wash. Note the increased number of response failures during NiCl₂ application. B, Averages of responses obtained before (n = 87), during (n = 60), and 13 min after wash (n = 40). C, Plot of EPSP amplitudes evoked by the first (EPSP1; filled symbols) and second (EPSP2; open symbols) pulse in the paired-pulse paradigm before, during (horizontal bar), and after application of NiCl₂. D, Mean peak amplitude of the first EPSP before (white column) and during (black column) superfusion of NiCl₂ (n = 13). E, Mean failure rates before (white column) and during (black column) application of NiCl₂ (n = 13). F, Mean paired-pulse facilitation ratio in control conditions and during NiCl₂ application (n = 12). *p < 0.05; **p < 0.001.

Similar blocking effect of NiCl₂ (~50%) was found in five of six cells clamped at a holding potential of $-$ 60 mV. In thesecells, EPSCs were evoked by minimal stimulation of MF or associative-commissuralfibers in stratum lucidum or radiatum, respectively (Fig. 6).In the presence of NiCl₂, a significant reduction in the meanpeak amplitude of the EPSCs was detected (from 23.4 ± 7.1 to 11.5± 3.7 pA; n = 5; p < 0.05) (Fig. 6D). A significant (p < 0.05)increase in the number of failures and paired-pulse facilitationratio was also found (from 30.6 ± 6.3 to 48.0 ± 6.1% and from1.67 ± 0.15 to 1.89 ± 0.16%, respectively) (Fig. 6E,F). All ofthese effects were rarely reversible.

View larger version (33K):
[in this window]
[in a new window]
Figure 6. NiCl₂ reduces the peak amplitude of EPSCs evoked in CA3 pyramidal neurons by minimal stimulation of the mossy fibers. A, Ten individual traces of EPSCs recorded from a holding potential of $-$ 60 mV, in control conditions and in the presence of NiCl₂. Note decreased EPSC amplitudes during NiCl₂ application and increased number of response failures after the first pulse. In this experiment, failure rate increased from 18.7 to 58.7%. B, Average EPSCs from the same experiment (n = 56 in control and n = 32 during application of NiCl₂). C, Plot of EPSC1 (filled symbols) and EPSC2 (open symbols) amplitude versus time before, during (horizontal bar), and after application of NiCl₂. D-F, Mean values of the EPSC1 amplitude (D), failure rate (E), and paired-pulse facilitation ratio (F) before (white columns) and during (black columns) NiCl₂ application (n = 5). *p < 0.05.

NiCl₂ was able to reduce to approximately the same extent EPSCs evoked in CA1 neurons by minimal stimulation of Schaffer collaterals(from 18.4 ± 8.6 to 7.7 ± 3.9 pA; n = 3/4; data notshown).

In conclusion, although a certain degree of variability of NiCl₂ block on single fiber EPSPs-EPSCs was observed in differentcells (on average, ~50%), a complete suppression was never achieved,suggesting that presynaptic terminals bearing only R-type channelsare highlyunlikely.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present experiments show that R-type VDCCs highly sensitive to both SNX 482 and NiCl₂ contribute to fast excitatory transmissionin the hippocampus, at mossy and associative-commissural fibersynapses. The first clue that presynaptic VDCCs of the R-typetrigger transmitter release has been provided by Wu et al. (1998)in the medial nucleus of the trapezoid body in brainstem slices(calyx of Held synapses). At these synapses, approximately one-quarterof calcium current evoked by a presynaptic action potential wasresistant to $omega$ -conotoxin-MVIIC but sensitive to relatively lowconcentrations of NiCl₂ (Randall and Tsien, 1995), supportingthe idea that R-type VDCCs cooperate with MVIIC-sensitive N- andP/Q-type to regulate synaptic transmission. In this preparation,the lower effectiveness of VDCC of R- and N-type in triggeringrelease compared with P/Q-type channels could be attributableto the distant location of a substantial fraction of R- and N-typechannels from the release sites (Wu et al., 1999). More recently,R-type VDCCs have been found to control both oxytocin releasein isolated neurohypophysial terminals (Wang et al., 1999) andthe rapid secretory response coupled to exocytotic release ofcatecholamines in mouse adrenal slice chromaffin cells (Albilloset al., 2000).

Native R-type VDCCs with different biophysical and pharmacological properties have been described in different types of neurons(Tottene et al., 1996; Hilaire et al., 1997; Magnelli et al.,1998; Wu et al., 1998; Wang et al., 1999) and have been shownto be coexpressed in the same type of neuron (Forti et al., 1994;Tottene et al., 1996; Wu et al., 1998; Tottene et al., 2000).Only some of the native R-type VDCCs are inhibited by SNX 482,the first selective (at concentrations <300-500 nM) antagonistof recombinant $alpha$ _1E (Ca_V 2.3) channels (Newcomb et al., 1998; Wanget al., 1999; Tottene et al., 2000). Tottene et al. (2000) haveshown that, in cerebellar granule cells, the component of R-typecalcium current inhibited by a low concentration of SNX 482 (fullyinhibited by 200 nM toxin) is also highly sensitive to NiCl₂ block(fully inhibited by 30 µM NiCl₂), whereas the R-type componentinhibited by larger concentrations of toxin [IC₅₀ of 500 nM, calledSNX 482-resistant component, because at these concentrations SNX482 is not a selective antagonist of $alpha$ _1E (Ca_V 2.3) channels] isalso less sensitive to NiCl₂ block. Both of these components areabsent in $alpha$ _1E knock-out mice (Wilson et al., 2000), because thecalcium current that remains in cerebellar granule cells of knock-outmice in the presence of $omega$ -agatoxin-IVA ( $omega$ -AgaIVA), $omega$ -conotoxin-GVIA,and nimodipine is not inhibited by 1 µM SNX 482 (a concentrationthat would completely inhibit the so called toxin-resistant componentof Tottene et al., 2000). Because both components are suppressedafter transfection of the neurons with specific $alpha$ _1E antisenseoligonucleotides (Tottene et al., 2000) and are completely absentin $alpha$ _1E knock-out mice (Wilson et al., 2000), the different R-typeVDCCs coexpressed in cerebellar granule cells appear to be allencoded by the $alpha$ _1E gene. Alternatively, spliced isoforms of the $alpha$ _1E subunit most likely account for their different biophysicaland pharmacological properties (Schramm et al., 1999; Totteneet al., 2000). The origin of the additional current componentnot inhibited by very high concentrations of SNX 482 describedby Wilson et al. (2000) remains unclear. It is possible that thiscurrent may actually be attributable to Q-type channels not completelyinhibited by 200 nM $omega$ -AgaIVA (Randall and Tsien, 1995).

In the present experiments, the observation that low concentrations of SNX 482 were able to reduce the amplitude of EPSCsto the same extent (~50%) as low concentrations of NiCl₂ stronglyfavors the conclusion that R-type calcium channels are involvedin transmitter release. Additional evidence in favor of R-typeVDCCs in fast synaptic transmission was provided by occlusionexperiments in which NiCl₂ was applied after SNX 482. No additionalsignificant reduction in EPSC amplitude was detected after additionof NiCl₂, suggesting that both NiCl₂ and the toxin act on thesame site. On the contrary, an additional reduction of EPSC amplitudewas observed when NiCl₂ was applied after $omega$ -CTx-MVIIC, at a saturatingconcentration known to completely inhibit N- and P/Q-type VDCCs(Castillo et al., 1994; Wu and Saggau, 1995), further supportinga specific action of NiCl₂ on R-type channels. These results contradictprevious findings that NiCl₂, at the same concentration, failedto modify field EPSPs evoked in the CA1 hippocampal region bySchaffer collateral stimulation (Oliet et al., 1997). This apparentdiscrepancy may be attributable to differences in the experimentalconditions. To obtain a mGluR form of long-term depression, aCa²⁺/Mg²⁺ ratio of 4:4 mM was used in experiments by Oliet et al. (1997)(instead of 2:1.3 mM used in the present experiments). This conditionthat reduces basal synaptic transmission to 62% may have affectedthe driving force for calcium and cooperativity within presynapticcalciumchannels.

Within the hippocampus, using in situ hybridization and immunocytochemical techniques, high levels of the $alpha$ _1E mRNA transcriptand protein have been detected mainly postsynaptically at thesomatic and dendritic level (Yokoyama et al., 1995; Day et al.,1996). The postsynaptic localization of the $alpha$ _1E protein is furthersupported by electrophysiological experiments showing the presenceof NiCl₂-sensitive R-type calcium channels on the dendrites ofCA1 pyramidal neurons. These channels together with the T-typeare supposed to contribute to action potential burst firing (Christieet al., 1995; Magee and Johnston, 1995; Kavalali et al., 1997;Magee and Carruth, 1999). However, immunoreactivity for classE calcium channels has been detected also presynaptically at thelevel of mossy fiber terminals in stratum lucidum, suggesting,in agreement with the present findings, a major role of thesechannels in cell communication (Day et al., 1996). Although wecannot entirely exclude that low concentrations of NiCl₂ or SNX482 may affect T- or R-type calcium channels located postsynaptically,the following observations support the conclusion that their blockingaction on EPSP-EPSC amplitude can be mostly accounted for by apresynaptic depression of transmitterrelease.

(1) NiCl₂ did not modify membrane potential, input resistance, or EPSCs kinetics. (2) NiCl₂ and SNX 482 reduced EPSPs-EPSCsevoked from $-$ 60 mV, a holding potential at which most low-voltage-activatedcalcium channels are inactivated. (3) In the case of alternativeactivation of two distinct inputs to the same cell, the toxinaffected preferentially EPSCs evoked by stimulation of fiberslocalized closer to the pressure pipette, leaving the others almostunaffected. In the case of a postsynaptic action, SNX 482 shouldhave affected EPSCs evoked by both inputs. (4) In the presenceof NiCl₂, the reduction of the amplitude of EPSPs-EPSCs evokedby minimal stimulation was associated with a significant increasein the number of failures. (5) In the presence of SNX 482, thedecrease in the amplitude of EPSC was accompanied by a reductionof CV², which is a traditional measure of transmitter release. (6) Thereduction of EPSP-EPSC amplitude by NiCl₂ and SNX 482 was associatedwith an increase in the paired-pulse facilitation ratio, anothertraditional index of changes in presynaptic releaseprobability.

Regarding the problem of whether R-type calcium channels are commingled or not with N and P/Q on the same presynaptic terminal,our data on single fiber EPSPs-EPSCs favor the hypothesis of acolocalization of multiple type of calcium channels on the samenerve ending. In fact, single fiber EPSP-EPSC reduction by NiCl₂varied from 51 to 59% but never achieved 100%, as expected forR-type calcium channels alone. Moreover, although the presentexperiments do not allow to reliably estimate the fraction ofpresynaptic calcium entry because of $alpha$ _1E channels, assuming thattransmitter release is proportional to [Ca²⁺]^m and m = 3.5 (according to Wu and Saggau, 1995, at least for CA3-CA1synapses), we can estimate that ~15% of R-type calcium channelscontribute to glutamate release. This value is slightly lowerthan that of 25% given by Wu and Saggau (1995) for $omega$ -CTx-MVIIC-resistantcalcium channels. This difference could be explained by severalfactors, including differences in m value that can vary from synapseto synapse and in the same synapse in relation to the localizationof calcium channels, more or less close to the active zones (Wuet al., 1999).

In conclusion, our data demonstrate that R-type calcium channels with pharmacological properties similar to those encodedby the $alpha$ _1E gene highly sensitive to NiCl₂ and to SNX 482 substantiallycontribute to fast glutamatergic synaptic transmission at mossyand associative-commissural fibersynapses.

  FOOTNOTES

Received March 21, 2001; revised Aug. 29, 2001; accepted Aug. 31, 2001.

This work was supported by grants from Ministero Università e Ricerca Scientifica e Tecnologica to E.C. and D.P., InternationalAssociation for the Promotion of Cooperation with Scientists fromthe New Independent States of the Former Soviet Union to E.C.and L.L.V., and Wellcome Trust to L.L.V. We thank H. Arechigafor participating in some experiments and J. C. Magee for carefullyreading thismanuscript.
Correspondence should be addressed to Enrico Cherubini, Neuroscience Program and Istituto Nazionale Fisica della Materia Unit,International School for Advanced Studies, Via Beirut 2-4, 34014Trieste, Italy. E-mail: cher{at}sissa.it.

S. Gasparini's present address: Louisiana State University Neuroscience Center, 2020 Gravier Street, New Orleans, LA70112.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Albillos A, Neher E, Moser T (2000) R-type Ca²⁺ channels are coupled to the rapid component of secretion in mouse adrenal slice chromaffin cells. J Neurosci 20:8323-8330[Abstract/Free Full Text].
Augustine GJ, Charlton MP (1986) Calcium dependence of presynaptic calcium current and postsynaptic response at the squid giant synapse. J Physiol (Lond) 381:619-640[Abstract/Free Full Text].
Berretta N, Rossokhin AV, Kasyanov AM, Sokolov MV, Cherubini E, Voronin LL (2000) Postsynaptic hyperpolarization increases the strength of AMPA-mediated synaptic transmission at large synapses between mossy fibres and CA3 pyramidal cells. Neuropharmacology 39:2288-2301[Web of Science][Medline].
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].
Chavez-Noriega LE, Stevens CF (1994) Increased transmitter release at excitatory synapses produced by direct activation of adenylate cyclase in rat hippocampal slices. J Neurosci 14:310-317[Abstract].
Christie BR, Eliot LS, Ito K, Miyakawa H, Johnston D (1995) Different Ca²⁺ channels in soma and dendrites of hippocampal pyramidal neurons mediate spike-induced Ca²⁺ influx. J Neurophysiol 73:2553-2557[Abstract/Free Full Text].
Craig PJ, Beattie RE, Folly EA, Banerjee MD, Reeves MB, Priestley JV, Carney SL, Sher E, Perez-Reyes E, Volsen SG (1999) Distribution of the voltage-dependent calcium channel $alpha$ 1G subunit mRNA and protein throughout the mature rat brain. Eur J Neurosci 11:2949-2964[Web of Science][Medline].
Day NC, Shaw AL, McCormack AL, Craig PJ, Smith W, Beattie R, Williams TL, Ellis SB, Ince PG, Harpold MM, Lodge D, Volsen SG (1996) Distribution of $alpha$ _1A, $alpha$ _1B and $alpha$ _1E voltage-dependent calcium channel subunits in the human hippocampus and parahippocampal gyrus. Neuroscience 71:1013-1024[Web of Science][Medline].
Dodge FA, Rahamimoff R (1967) Co-operative action of calcium ions in transmitter release at the neuromuscular junction. J Physiol (Lond) 193:419-432[Abstract/Free Full Text].
Dunlap K, Luebke JI, Turner TJ (1995) Exocytotic Ca²⁺ channels in mammalian central neurons. Trends Neurosci 18:89-98[Web of Science][Medline].
Faber DS, Korn H (1991) Applicability of the coefficient of variation method for analyzing synaptic plasticity. Biophys J 60:1288-1294[Web of Science][Medline].
Forti L, Tottene A, Moretti A, Pietrobon D (1994) Three novel types of voltage-dependent calcium channels in rat cerebellar neurons. J Neurosci 14:5243-5256[Abstract].
Gasparini S, Saviane C, Voronin LL, Cherubini E (2000) Silent synapses in the developing hippocampus: lack of functional AMPA receptors or low probability of glutamate release? Proc Natl Acad Sci USA 97:9741-9746[Abstract/Free Full Text].
Hilaire C, Diochot S, Desmadryl G, Richard S, Valmier J (1997) Toxin-resistant calcium currents in embryonic mouse sensory neurons. Neuroscience 80:267-276[Web of Science][Medline].
Huguenard JR (1996) Low-threshold calcium currents in central nervous system neurons. Annu Rev Physiol 58:329-348[Web of Science][Medline].
Kamiya H, Shinozaki H, Yamamoto C (1996) Activation of metabotropic glutamate receptors type 2/3 suppresses transmission at rat hippocampal mossy fiber synapses. J Physiol (Lond) 493:447-455[Abstract/Free Full Text].
Katz B (1969) In: The release of neural transmitter substance. Springfield, IL: Thomas.
Kavalali ET, Zhuo M, Bito H, Tsien RW (1997) Dendritic Ca²⁺ channels characterized by recordings from isolated hippocampal dendritic segments. Neuron 18:651-663[Web of Science][Medline].
Luebke J, Dunlap K, Turner TJ (1993) Multiple calcium channel types control glutamatergic synaptic transmission in the hippocampus. Neuron 11:895-902[Web of Science][Medline].
Magee JC, Carruth M (1999) Dendritic voltage-gated ion channels regulate the action potential firing mode of hippocampal CA1 pyramidal neurons. J Neurophysiol 82:1895-1901[Abstract/Free Full Text].
Magee JC, Johnston D (1995) Characterization of single voltage-gated Na⁺ and Ca²⁺ channels in apical dendrites of rat CA1 pyramidal neurons. J Physiol (Lond) 487:67-90[Abstract/Free Full Text].
Magnelli V, Baldelli P, Carbone E (1998) Antagonists-resistant calcium currents in rat embryo motoneurons. Eur J Neurosci 10:1810-1825[Web of Science][Medline].
Miledi R, Thies RE (1971) Tetanic and post-tetanic rise in frequency of miniature end-plate potentials in low calcium solution. J Physiol (Lond) 212:245-257[Abstract/Free Full Text].
Mintz IM, Sabattini BL, Regehr WG (1995) Calcium control of transmitter release at a cerebellar synapse. Neuron 15:675-688[Web of Science][Medline].
Newcomb R, Szoke B, Palma A, Wang G, Chen X, Hopkins W, Cong R, Miller J, Tarczy-Hornoch K, Loo JA, Dooley DJ, Nadasdi L, Tsien RW, Lemos JR, Miljanich G (1998) A selective peptide antagonist of the class E calcium channel from the venom of tarantula, Hysterocrates gigas. Biochemistry 37:15353-15362[Medline].
Oliet SHR, Malenka RC, Nicoll RA (1997) Two distinct forms of long term depression coexist in CA1 hippocampal pyramidal cells. Neuron 18:969-982[Web of Science][Medline].
Randall AD, Tsien RW (1995) Pharmacological dissection of multiple types of Ca²⁺ channel currents in rat cerebellar granule neurons. J Neurosci 15:2995-3012[Abstract].
Schramm M, Vajna R, Pereverzev A, Tottene A, Klockner U, Pietrobon D, Hescheler J, Schneider T (1999) Isoforms of $alpha$ 1E voltage-gated calcium channels in rat cerebellar granule cells: detection of major calcium channel $alpha$ 1-transcripts by reverse transcription-polymerase chain reaction. Neuroscience 92:565-575[Web of Science][Medline].
Takahashi T, Momiyama A (1993) Different types of calcium channels mediate central synaptic transmission. Nature 366:156-158[Medline].
Tottene A, Moretti A, Pietrobon D (1996) Functional diversity of P-type and R-type calcium channels in rat cerebellar neurons. J Neurosci 16:6353-6363[Abstract/Free Full Text].
Tottene A, Volsen S, Pietrobon D (2000) $alpha$ _1E subunits form the pore of three cerebellar R-type calcium channels with different pharmacological and permeation properties. J Neurosci 20:171-178[Abstract/Free Full Text].
Voronin LL (1993) On the quantal analysis of hippocampal long-term potentiation and related phenomena of synaptic plasticity. Neuroscience 56:275-304[Web of Science][Medline].
Wang G, Dayanithi G, Newcomb R, Lemos JR (1999) An R-type Ca²⁺ current in neurohypophysial terminals preferentially regulates oxytocin secretion. J Neurosci 19:9235-9241[Abstract/Free Full Text].
Wheeler DB, Randall A, Tsien RW (1994) Roles of N-type and Q-type Ca²⁺ channels in supporting hippocampal synaptic transmission. Science 264:107-111[Abstract/Free Full Text].
Wilson SM, Toth PT, Oh SB, Gillard SE, Volsen S, Ren D, Phipson LH, Lee EC, Fletcher CF, Tessarollo L, Copeland NG, Jenkins NA, Miller RJ (2000) The status of voltage-dependent calcium channels in $alpha$ _1E knock-out mice. J Neurosci 20:8566-8571[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, Saggau P (1995) Block of multiple presynaptic calcium channel types by $omega$ -conotoxin-MVIIC at hippocampal CA3 to CA1 synapses. J Neurophysiol 73:1965-1972[Abstract/Free Full Text].
Wu LG, Saggau P (1997) Presynaptic inhibition of elicited neurotransmitter release. Trends Neurosci 20:204-212[Web of Science][Medline].
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].
Wu LG, Westenbroek RE, Borst JG, Catterall WA, Sakmann B (1999) Calcium channel types with distinct presynaptic localization couple differentially to transmitter release in single calix-type synapses. J Neurosci 19:726-736[Abstract/Free Full Text].
Yokoyama CT, Westenbroek RE, Hell JW, Soong TW, Snutch TP, Catterall WA (1995) Biochemical properties and subcellular distribution of the neuronal class E calcium channel $alpha$ ₁ subunit. J Neurosci 15:6419-6432[Abstract/Free Full Text].
Zhang JF, Randall AD, Ellinor PT, Horne WA, Sather WA, Tanabe T, Schwarz TL, Tsien RW (1993) Distinctive pharmacology and kinetics of cloned neuronal Ca2+ channels and their possible counterparts in mammalian CNS neurons. Neuropharmacology 32:1075-1088[Web of Science][Medline].

Copyright © 2001 Society for Neuroscience 0270-6474/01/21228715-07$05.00/0

This article has been cited by other articles:

S. Dai, D. D. Hall, and J. W. Hell
Supramolecular Assemblies and Localized Regulation of Voltage-Gated Ion Channels
Physiol Rev, April 1, 2009; 89(2): 411 - 452.
[Abstract] [Full Text] [PDF]

P. Long, A. Mercer, R. Begum, G. J. Stephens, T. S. Sihra, and J. N. Jovanovic
Nerve Terminal GABAA Receptors Activate Ca2+/Calmodulin-dependent Signaling to Inhibit Voltage-gated Ca2+ Influx and Glutamate Release
J. Biol. Chem., March 27, 2009; 284(13): 8726 - 8737.
[Abstract] [Full Text] [PDF]

P. M. Joksovic, M. Weiergraber, W. Lee, H. Struck, T. Schneider, and S. M. Todorovic
Isoflurane-Sensitive Presynaptic R-Type Calcium Channels Contribute to Inhibitory Synaptic Transmission in the Rat Thalamus
J. Neurosci., February 4, 2009; 29(5): 1434 - 1445.
[Abstract] [Full Text] [PDF]

E. Calixto, E. J. Galvan, J. P. Card, and G. Barrionuevo
Coincidence detection of convergent perforant path and mossy fibre inputs by CA3 interneurons
J. Physiol., June 1, 2008; 586(11): 2695 - 2712.
[Abstract] [Full Text] [PDF]

L. Li, J. Bischofberger, and P. Jonas
Differential Gating and Recruitment of P/Q-, N-, and R-Type Ca2+ Channels in Hippocampal Mossy Fiber Boutons
J. Neurosci., December 5, 2007; 27(49): 13420 - 13429.
[Abstract] [Full Text] [PDF]

A. Gundlfinger, J. Bischofberger, F. W. Johenning, M. Torvinen, D. Schmitz, and J. Breustedt
Adenosine modulates transmission at the hippocampal mossy fibre synapse via direct inhibition of presynaptic calcium channels
J. Physiol., July 1, 2007; 582(1): 263 - 277.
[Abstract] [Full Text] [PDF]

U. Meza, A. Thapliyal, R. A. Bannister, and B. A. Adams
Neurokinin 1 Receptors Trigger Overlapping Stimulation and Inhibition of CaV2.3 (R-Type) Calcium Channels
Mol. Pharmacol., January 1, 2007; 71(1): 284 - 293.
[Abstract] [Full Text] [PDF]

A. E. Metz, T. Jarsky, M. Martina, and N. Spruston
R-Type Calcium Channels Contribute to Afterdepolarization and Bursting in Hippocampal CA1 Pyramidal Neurons
J. Neurosci., June 15, 2005; 25(24): 5763 - 5773.
[Abstract] [Full Text] [PDF]

A. Scheuber, R. Miles, and J. C. Poncer
Presynaptic Cav2.1 and Cav2.2 Differentially Influence Release Dynamics at Hippocampal Excitatory Synapses
J. Neurosci., November 17, 2004; 24(46): 10402 - 10409.
[Abstract] [Full Text] [PDF]

X. Bian, X. Zhou, and J. J. Galligan
R-type calcium channels in myenteric neurons of guinea pig small intestine
Am J Physiol Gastrointest Liver Physiol, July 1, 2004; 287(1): G134 - G142.
[Abstract] [Full Text] [PDF]

H. Daniel, A. Rancillac, and F. Crepel
Mechanisms underlying cannabinoid inhibition of presynaptic Ca2+ influx at parallel fibre synapses of the rat cerebellum
J. Physiol., May 15, 2004; 557(1): 159 - 174.
[Abstract] [Full Text] [PDF]

R. A. Bannister, K. Melliti, and B. A. Adams
Differential Modulation of CaV2.3 Ca2+ Channels by G{alpha}q/11-Coupled Muscarinic Receptors
Mol. Pharmacol., February 1, 2004; 65(2): 381 - 388.
[Abstract] [Full Text] [PDF]

A. Brandt, J. Striessnig, and T. Moser
CaV1.3 Channels Are Essential for Development and Presynaptic Activity of Cochlear Inner Hair Cells
J. Neurosci., November 26, 2003; 23(34): 10832 - 10840.
[Abstract] [Full Text] [PDF]

J. Breustedt, K. E. Vogt, R. J. Miller, R. A. Nicoll, and D. Schmitz
{alpha}1E-Containing Ca2+ channels are involved in synaptic plasticity
PNAS, October 14, 2003; 100(21): 12450 - 12455.
[Abstract] [Full Text] [PDF]

J. Bischofberger, J. R. P. Geiger, and P. Jonas
Timing and Efficacy of Ca2+ Channel Activation in Hippocampal Mossy Fiber Boutons
J. Neurosci., December 15, 2002; 22(24): 10593 - 10602.
[Abstract] [Full Text] [PDF]

W. J. Tyler, S. P. Perrett, and L. D. Pozzo-Miller
The Role of Neurotrophins in Neurotransmitter Release
Neuroscientist, December 1, 2002; 8(6): 524 - 531.
[Abstract] [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 (34)

Citing Articles via Google Scholar

Google Scholar

Articles by Gasparini, S.

Articles by Cherubini, E.

Search for Related Content

PubMed

PubMed Citation

Articles by Gasparini, S.

Articles by Cherubini, E.