GABA Activity Mediating Cytosolic Ca2+ Rises in Developing Neurons Is Modulated by cAMP-Dependent Signal Transduction

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 (31)

Citing Articles via Google Scholar

Google Scholar

Articles by Obrietan, K.

Articles by van den Pol, A. N.

Search for Related Content

PubMed

PubMed Citation

Articles by Obrietan, K.

Articles by van den Pol, A. N.

Previous Article  |  Next Article

Volume 17, Number 12, Issue of June 15, 1997 pp. 4785-4799
Copyright ©1997 Society for Neuroscience

GABA Activity Mediating Cytosolic Ca²⁺ Rises in Developing Neurons Is Modulated by cAMP-Dependent Signal Transduction

Karl Obrietan and Anthony N. van den Pol
Department of Biological Sciences, Stanford University, Stanford, California 94305, and Department of Neurosurgery, Yale University, School of Medicine, New Haven, Connecticut 06520

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

In the majority of developing neurons, GABA can exert depolarizing actions, thereby raising neuronal Ca²⁺. Ca²⁺ elevations can have broad consequences during development, inducinggene expression, altering neurite outgrowth and growth cone turning,activating enzyme pathways, and influencing neuronal survival.We used fura-2 and fluo-3 Ca²⁺ digital imaging to assess the effects of inhibiting or activatingthe cAMP signal transduction pathway on GABA activity mediatingCa²⁺ rises during the early stages of in vitro hypothalamic neuraldevelopment. Our experiments stemmed from the finding that stimulationof transmitter receptors shown to either activate or inhibit adenylylcyclase activity caused a rapid decrease in Ca²⁺ rises mediated by synaptically released GABA.
Both the adenylyl cyclase activator forskolin and the inhibitor SQ-22,536 reduced the Ca²⁺ rise elicited by the synaptic release of GABA. Bath applicationof the membrane-permeable cAMP analogs 8-bromo-cAMP (8-Br-cAMP)or 8-(4-chlorophenylthio)-cAMP (0.2-5 mM) produced a rapid, reversible,dose-dependent inhibition of Ca²⁺ rises triggered by synaptic GABA release. Potentiation of GABAergicactivity mediating Ca²⁺ rises was observed in some neurons at relatively low concentrationsof the membrane-permeable cAMP analogs (20-50 µM). In the presenceof tetrodotoxin (TTX), postsynaptic Ca²⁺ rises triggered by the bath application of GABA were only moderatelydepressed (13%) by 8-Br-cAMP (1 mM), suggesting that the inhibitoryeffects of 8-Br-cAMP were largely the result of a presynapticmechanism.
The protein kinase A (PKA) inhibitors H89 and Rp-3 $'$ ,5 $'$ -cyclic monophosphothioate triethylamine also caused a large reduction(>70%) in Ca²⁺ rises triggered by synaptic GABA release. Unlike the short-termdepression elicited by activation of the cAMP signal transductionpathway, Ca²⁺ depression elicited by PKA inhibition persisted for an extendedperiod (>30 min) after PKA inhibitor washout. Postsynaptic depressionof GABA-evoked Ca²⁺ rises triggered by H89 (in the presence of TTX) recovered rapidly,suggesting that the extended depression observed during synapticGABA release was largely through a presynaptic mechanism. Long-termCa²⁺ modulation by cAMP-regulating hypothalamic peptides may be mediatedthrough a parallel mechanism.
Together, these results suggest that GABAergic activity mediating Ca²⁺ rises is dependent on ongoing PKA activity that is maintainedwithin a narrow zone for GABA to elicit a maximal Ca²⁺ elevation. Thus, neuromodulator-mediated changes in the cAMP-dependentsignal transduction pathway (activation or inhibition) could leadto a substantial decrease in GABA-mediated Ca²⁺ rises during early development.
Key words: mediobasal hypothalamus; calcium; GABA; GABA excitation; protein kinase A; cAMP; development; digital imaging

INTRODUCTION

The role of GABA as an excitatory neurotransmitter during the early stages of neural development has been documented overthe past several years (for review, see Cherubini et al., 1991).Several studies have shown that GABA triggers neural excitabilityby activating the GABA_A receptor (Ben-Ari et al., 1989; Chen etal., 1996). Because of a relatively depolarized Cl reversal potential (Chen et al., 1996), opening of the GABA_Areceptor allows Cl to efflux from the neuron, triggering membrane potential depolarization,activation of voltage-sensitive Ca²⁺ channels, and, as a result, an increase in intracellular Ca²⁺ (Yuste and Katz, 1991; Yamashita and Fukuda, 1993; Obrietan andvan den Pol, 1995). Although glutamate receives a lot of attentionregarding its ability to elevate cytosolic Ca²⁺ levels in developing neurons, we found that many developing neuronsshow a greater Ca²⁺ elevation in response to GABA than to an equimolar concentrationof glutamate (Obrietan and van den Pol, 1995). As neurons mature,GABA becomes a predominantly inhibitory transmitter that decreasescytosolic Ca²⁺ levels (Obrietan and van den Pol, 1995). GABA has been shownto possess many of the effects of other, better characterized,fast excitatory neurotransmitters known to increase intracellularCa²⁺ during development. For example, GABA_A receptor activation cantrigger BDNF induction (Berninger et al., 1995) and alter theneural phenotype (Marty et al., 1996). In addition, DNA synthesisin cortical neural progenitor cells can be blocked by specificallyinhibiting GABA_A receptor activity (LoTurco et al., 1995). GABAcan increase Ca²⁺ levels in neurites and growth cones (Obrietan and van den Pol,1996a), which may alter growth cone motility and the rate of neuriteextension. In addition, GABA-mediated Ca²⁺ influx in growth cones leads to an increase in GAP43 and MARCKSprotein phosphorylation (Fukura et al., 1996). These results suggestthat the ability of GABA to raise intracellular Ca²⁺ levels may be central to its functional role during development.

The cAMP signal transduction pathway is a potent regulator of synaptic neural physiology (for review, see Anholt, 1994; Cooperet al., 1994). A primary mechanism by which cAMP regulates neuralexcitability is through the activation of cAMP-dependent proteinkinase A (PKA). The neuromodulatory actions of PKA have been documentedextensively and include altering ion channel activity (Nagel etal., 1992; Johnson et al., 1994; Surmeier et al., 1995), geneexpression (Impey et al., 1996), and neurotransmitter release(Sciancalepore and Cherubini, 1995; Huang et al., 1996). Althougha considerable amount of information is known about the effectsof PKA at the molecular and single channel levels, much remainsto be determined about how its actions at a variety of sites mayaffect cytosolic Ca²⁺ regulation in synaptically active neurons. For example, PKA hasbeen shown to reduce the amplitude of the GABA_A receptor conductance(Moss et al., 1992), to decrease voltage-gated Na⁺ channel currents (Smith and Goldin, 1996), and to potentiatekainate-induced currents (Gu and Moss, 1996). A question of particularinterest is how GABAergic activity mediating Ca²⁺ elevations may be regulated during early development by PKA.

Similar to GABA, PKA has also been shown to play an important role during development. The cAMP signal transduction pathwayhas been implicated in a variety of developmentally regulatedprocesses, including cell cycle regulation (Grieco et al., 1996),neural migration (Behar et al., 1995), and gene induction (Zhanget al., 1993). Additionally, many neurotransmitters and neuropeptidesthat affect neural physiology through the regulation of adenylylcyclase activity, including neuropeptide Y (NPY), dopamine, glutamate,and serotonin, are expressed in early development and could serveto modulate the Ca²⁺-elevating actions of GABA (Rajaofetra, 1989; Belin et al., 1991;Marti et al., 1992; van den Pol et al., 1995, 1996a; Lieb et al.,1996). Based on these findings, we studied the modulation of GABAergicCa²⁺ elevating activity by the cAMP-mediated signal transduction pathway.

Here we report that Ca²⁺ rises regulated by synaptic GABA release during early development are dramatically influenced by activationor inhibition of the cAMP-dependent signal transduction cascade.

MATERIALS AND METHODS
Tissue culture. The mediobasal hypothalamus was removed from embryonic day 18 Sprague Dawley rats. The tissue was enzymaticallydigested in a mild protease solution (10 U/ml papain and 0.2 mg/mlL-cysteine in Earl's balanced salt solution) for 30 min. Next,the tissue was pelleted, and the protease solution was removed.Tissue was then suspended in standard tissue culture medium (glutamate-and glutamine-free DMEM supplemented with 10% fetal bovine serum,100 U/ml penicillin/streptomycin, and 6 gm/l glucose) and thentriturated into a single-cell suspension. Cells were washed andpelleted an additional three times. The single-cell suspensionwas plated onto 22 mm² glass coverslips that had been coated with high-molecular-weight(540,000 Da) poly-D-lysine. High-density cultures (200,000/cm²) were used for all experiments. Hypothalamic neural cultureswere maintained in a Napco 3600 incubator (37°C and 5% CO₂) untilthey were ready for use. To limit non-neuronal cell proliferation,cytosine arabinofuranoside (1 µM) was added to the tissue culturemedium 1 d after plating.

Fura-2 and fluo-3 Ca²⁺ digital imaging. Cells were loaded for 20 min with either 5 µM fura-2 AM or fluo-3 AM in standard perfusionsolution (137 mM NaCl, 25 mM glucose, 10 mM HEPES, 5 mM KCl, 1mM MgCl₂, 3 mM CaCl₂, pH 7.4). The cells were then washed andallowed to recover for 15 min before the start of the experiment.Coverslips were then loaded into a laminar style perfusion chamber.Solutions rapidly moved as a straight wave through the perfusionchamber, and complete washout of the chamber occurred in ~5 sec.For fura-2, neurons were imaged using a 40× Olympus objectivewith high 340/380 nm transmittance on a Nikon Diaphot 300 invertedmicroscope. Fluo-3 experiments were performed using a 100× Olympusobjective. Unless noted otherwise, Ca²⁺ digital recordings were made from the cell soma. All experimentswere performed at room temperature.

A 486 PC clone was used to collect data, run Ca²⁺ analysis software (Fluor; Universal Imaging Corporation, West Chester, PA),and control the Lambda-10-filtered wheel driver (Sutter Instruments).Sixteen (500 msec) digital frames of data were collected every3 sec. Excitation light came from a 150 W Xenon lamp. The equation[Ca²⁺]i = K_d(R $-$ R_min)/(R_max $-$ R) was used to convert fura-2 ratiometricfluorescent Ca²⁺ values to free Ca²⁺ concentrations. R is the ratio of the two fluorescence intensities,R_min is the ratio in the absence of Ca²⁺, and R_max is the ratio in a saturating concentration of Ca²⁺. The K_d for binding of Ca²⁺ to fura 2 was taken to be 224 nM (Grynkiewicz et al., 1985).Data for fluo-3 fluorescence are represented on a 0-255 U scale.As standard protocol for both fura-2 and fluo-3 imaging, backgroundfluorescence values were subtracted.

To determine the effects of different receptor agonists or signal transduction modulators on Ca²⁺ rises triggered by the synaptic release of GABA, the mean Ca²⁺ rise from the Ca²⁺ level in the presence of the GABA_A receptor antagonist bicucullinewas determined over a 15 sec period just before the applicationof a receptor agonist or signal transduction modulator. The meanCa²⁺ rise was then determined over a 15 sec period 90 sec after administrationof the receptor agonist or signal transduction modulator. Datafor Ca²⁺ rises for the two conditions are reported as a mean (pooled)Ca²⁺ rise of all responsive neurons ± SEM. Thirty to 50% of the neuronsexhibited a Ca²⁺ rise on bicuculline removal. For assays that evoked a Ca²⁺ response, either through agonist administration to the perfusionsolution or through electrical stimulation, the maximal Ca²⁺ rise for individual neurons was determined by subtracting themean basal Ca²⁺ level for a 15 sec period just before stimulation from the peak-evokedCa²⁺ rise. Ca²⁺ responses from a total of 1165 neurons were recorded in the courseof these experiments. Modulation of GABA-related activity couldrefer to either a presynaptic or postsynaptic site of action,whereas modulation of GABA-evoked Ca²⁺ rises refers to a postsynaptic site of action.

Electrical stimulation. Electrodes from a Grass SD9 stimulator were placed at both ends of the perfusion chamber. Ca²⁺ rises were stimulated by passing 2-5 V/cm², at 20 Hz frequency and 2 msec duration, through the chamberfor 6 sec. Ca²⁺ rises were visible immediately and usually peaked 4 sec aftercurrent application. At these voltages, Ca²⁺ rises were inhibited by either the application of the voltage-dependentNa⁺ channel blocker tetrodotoxin (TTX; 1 µM) or the administrationof fast excitatory neurotransmitter antagonists. At voltages higherthan those used in this paper (>6 V/cm²), TTX did not block the Ca²⁺ response, suggesting an additional nonsynaptic mechanism forthe induction of Ca²⁺ rises.

Immunostaining. Neurons were fixed for 1 hr in cold ( $-$ 20°C) methanol and then treated for 30 min with 3% BSA and 0.1% TritonX-100 in PBS. Neurons were then washed and incubated with mouseanti-synapsin 1 antibody (1:100) (Chemicon, Temecula, CA). Thesynapsin antiserum recognized a band of the correct weight onWestern blots, and preabsorption with synapsin antigen blockedstaining (Smith et al., 1994). Rat anti- $alpha$ -tubulin antibody (SeraLab) was used at 1:200 for 30 min. Neurons were washed and incubatedwith FITC- and Texas Red-labeled secondary antibodies (JacksonLaboratory, Bar Harbor, ME) for 30 min. After washing, cell fluorescencewas visualized with the appropriate filter sets. In the fluorescentmicroscope, synapsin-immunostained boutons were green, and tubulinimmunoreactivity was red.

Reagents. SKF-38393, McN-A-343, cytosine arabinofuranoside, GABA, cAMP, 8-bromo-cAMP (8-Br-cAMP), 8-(4-chlorophenylthio)-cAMP(4-Cl-cAMP), and poly-D-lysine were acquired from Sigma (St. Louis,MO). SQ-22,536, forskolin, (±) $-$ 2-amino-5-phosphonopentanoic acid(AP5), 6-cyano-7-nitroquinoxaline-2,3-dione (CNQX), bicuculline,nimodipine, and TTX were acquired from Research Biochemicals (Natick,MA). NPY was acquired from Peninsula Labs. Papain was acquiredfrom Worthington (Freehold, NJ); DMEM was from Life Technologies(Gaithersburg, MD); and fura-2 AM and fluo-3 AM were from MolecularProbes (Eugene, OR).

RESULTS

cAMP signal transduction pathway activation
To address the possibility that activating the cAMP signal transduction pathway affects GABA activity that mediates Ca²⁺ elevations, membrane-permeable cAMP analogs that mimic the cellulareffects of cAMP were administered to synaptically active hypothalamicneurons. Figure 1A shows that the withdrawal of the GABA_A receptorantagonist bicuculline (20 µM) from the perfusion solution eliciteda rapid and stable Ca²⁺ rise, indicating that cytosolic Ca²⁺ was raised by synaptically released GABA. Addition of 8-Br-cAMP(1 mM) caused a rapid reduction in Ca²⁺ levels. The mean ± SEM Ca²⁺ rise after removal of bicuculline was 73 ± 6 nM. After the additionof 8-Br-cAMP the Ca²⁺ rise decreased to 28 ± 5 nM, representing a statistically significant(p < 0.0001, two-tailed t test) reduction in GABA-mediated Ca²⁺ rise of 62% (n = 68). Figure 1B shows that mean inhibition ofGABA activity regulating Ca²⁺ rises by 8-Br-cAMP was dose-dependent. GABA-mediated Ca²⁺ levels were increased in some neurons, but only at low 8-Br-cAMPconcentrations. Specifically, the Ca²⁺ level in 6 of 20 neurons was raised by 50 µM extracellular 8-Br-cAMP,and at 150 µM 8-Br-cAMP, the Ca²⁺ level was raised in 4 of 30 neurons. However, at higher concentrations(500 µM and 1 and 5 mM) 8-Br-cAMP only depressed Ca²⁺ levels and did not elevate Ca²⁺ levels in any neurons (n = 90).
Fig. 1. Membrane-permeable analogs of cAMP trigger reversible Ca²⁺ depression. A, The removal of bicuculline (BIC, 20 µM) from the perfusionsolution triggered a rapid and sustained Ca²⁺ rise in the two representative neurons. Repeated applicationof 8-Br-cAMP (1 mM) induced a rapid depression of the GABA-relatedCa²⁺ rises that lasted only as long as 8-Br-cAMP was applied. B, Dose-responseeffect of 8-Br-cAMP on the synaptically released GABA-mediatedCa²⁺ level. The Ca²⁺ rise from a bicuculline-defined baseline was determined overa 15 sec period just before and 90 sec after 8-Br-cAMP application.The white bar (set at 100%) is the normalized Ca²⁺ rise just before 8-Br-cAMP application. Error bars indicate SEM.N, Total number of neurons assayed. C, 8-Br-cAMP had no effecton neuronal Ca²⁺ levels if synaptic GABA release was inhibited by the administrationof the Na⁺ channel blocker TTX (1 µM). Neurons with only small baselineCa²⁺ fluctuations were shown, so that any effect of 8-Br-cAMP on basalCa²⁺ might be observed. D, Membrane-impermeable cAMP (1 mM) had littleextracellular effect on GABA-mediated Ca²⁺ levels. All experiments were performed in the presence of AP5(100 µM) and CNQX (10 µM). All synaptic release experiments wereperformed with embryonic day 18 neurons after 5 DIV. In A, C,D, the bar along the x-axis shows time in min, and the bar tothe left of each Ca²⁺ trace is the calibrated cytosolic Ca²⁺ value for each neuron.
[View Larger Version of this Image (34K GIF file)]

Another membrane-permeable cAMP analog, 4-Cl-cAMP (2 mM), also triggered a rapid Ca²⁺ depression (Fig. 2A). The effectiveness of 4-Cl-cAMP was alsodose-dependent; at 2 mM, 4-Cl-cAMP caused a statistically significant(p < 0.0001, two-tailed t test) 81% Ca²⁺ depression (n = 29), whereas 200 µM 4-Cl-cAMP reduced the GABA-mediatedCa²⁺ rise by a statistically significant (p < 0.001, two-tailed ttest) 39% (n = 25). Figure 2B shows that the coadministrationof the potent PKA inhibitor Rp-3 $'$ ,5 $'$ -cyclic monophosphothioatetriethylamine (Rp-cAMPS) largely blocked the effects of 4-Cl-cAMP,suggesting that the actions of membrane-permeable cAMP analogsare the result of PKA activation. Application of 4-Cl-cAMP (1mM) triggered a 78% decrease in GABA-mediated Ca²⁺ levels, whereas 4-Cl-cAMP (1 mM) administration, in the presenceof Rp-cAMPS (200 µM), resulted in a 46% Ca²⁺ decrease (n = 42). As with low concentrations of 8-Br-cAMP, theadministration of relatively low levels of 4-Cl-cAMP triggeredCa²⁺ rises that were not observed at higher concentrations. Figure2C shows two neurons treated to both low (20 µM) and high (1 mM)concentrations of 4-Cl-cAMP. 4-Cl-cAMP at a concentration of 20µM triggered an enhancement in both the mean Ca²⁺ concentration (Ca²⁺ concentrations shown for each bracketed region ± SEM) and, insome neurons, the size of GABA-mediated Ca²⁺ transients. By comparing the mean Ca²⁺ rise during bracketed region B (after bicuculline withdrawal)with the mean Ca²⁺ rise during bracketed region C (during 20 µM 4-Cl-cAMP), we foundthat 4-Cl-cAMP triggered a >20% increase in GABA-mediated Ca²⁺ rises in 17 of 57 neurons. This effect is in striking contrastto the large Ca²⁺ decrease observed on administration of 1 mM 4-Cl-cAMP. Theseneurons were cultured on embryonic day 18 and maintained for 5d in vitro (DIV). Figures often show data records from two ormore neurons recorded simultaneously. This serves both to validatesubtle, but consistent, effects of pharmacological manipulationsand to show the heterogeneity of neural response characteristics.
Fig. 2. Modulation of GABA activity mediating Ca²⁺ rises. A, The membrane-permeable analog of cAMP, 4-Cl-cAMP (2 mM), elicited a rapidand reproducible Ca²⁺ depression. B, Coadministration of the protein kinase A inhibitorRp-cAMPS (200 µM) largely blocked the Ca²⁺ depression elicited by 4-Cl-cAMP (1 mM). C, Two representativeneurons show that administration of a low concentration of 4-Cl-cAMP(20 µM) triggered a Ca²⁺ increase, whereas a high concentration of 4-Cl-cAMP (1 mM) triggereda Ca²⁺ depression. Numbers under each bracket refer to the mean ± SEMCa²⁺ concentration for the period within the bracketed region. Twentytime points (3 sec interval) were used to determine each Ca²⁺ concentration, except for the beginning of the experiment [bicuculline(BIC) administration], at which 10 time points were used. Lettersunder brackets identify each bracketed region.
[View Larger Version of this Image (33K GIF file)]

To remove any complicating effects of synaptically released glutamate on Ca²⁺ rises, neurons were constantly perfused with the ionotropic glutamatereceptor antagonists AP5 (100 µM) and CNQX (10 µM). In the presenceof glutamate receptor blockers AP5 and CNQX, basal Ca²⁺ levels did not change when neurons were switched between perfusionsolutions containing bicuculline (20 µM) or the Na⁺ channel blocker TTX (1 µM), suggesting that in the absence ofglutamatergic neurotransmission, GABA was the sole transmitterresponsible for increasing neuronal Ca²⁺ levels (data not shown).

The Na⁺ channel blocker TTX (1 µM) inhibited Ca²⁺ transients mediated by the synaptic release of GABA (Fig. 1C). 8-Br-cAMP (1mM) had no independent effect on basal Ca²⁺ levels (Fig. 1C). As an additional control we added cAMP (1 mM)to the perfusion solution. Because cAMP is membrane-impermeable,it should not mimic the intracellular effects of 8-Br-cAMP or4-Cl-cAMP. Figure 1D shows that cAMP had very little effect onGABA-mediated Ca²⁺ rises, suggesting that 8-Br-cAMP and 4-Cl-cAMP were acting primarilythrough an intracellular mechanism to depress Ca²⁺ levels rather than at an extracellular receptor. The Ca²⁺ rise before the addition of cAMP was 101 ± 10 nM; during cAMPapplication, the Ca²⁺ rise decreased to 87 ± 10 nM, representing a statistically insignificant(p > 0.05, two-tailed t test) 14% cAMP-dependent decrease (n =38).

8-Br-cAMP inhibits GABA activity through presynaptic and postsynaptic mechanisms
To determine whether activation of the cAMP-dependent signal transduction cascade inhibits GABA-related Ca²⁺ rises through a presynaptic or postsynaptic mechanism, we comparedthe effects of 8-Br-cAMP on postsynaptic Ca²⁺ rises elicited by bath application of GABA with the effects of8-Br-cAMP on electrically stimulated Ca²⁺ rises dependent on presynaptic GABA release. Figure 3A showsCa²⁺ rises elicited by bath application of GABA (10 µM). Interestingly,Ca²⁺ rises were either inhibited (top trace) or potentiated (bottomtrace) by 8-Br-cAMP (1 mM). Relative to the control Ca²⁺ rise immediately preceding 8-Br-cAMP administration, 8-Br-cAMPdepressed the Ca²⁺ rise by >20% in 32 of 109 neurons and potentiated the GABA-evokedCa²⁺ rises in 19 of 109 neurons by >20%. In the absence of 8-Br-cAMP,repeated peak Ca²⁺ rises evoked by GABA did not vary by >20% in any of the 109 neuronsassayed. Figure 3C is a scatter plot analysis of the modulatoryeffects of 8-Br-cAMP administration on GABA-evoked Ca²⁺ rises. Each point (neuron) is a representation of the first Ca²⁺ rise in the presence of 8-Br-cAMP divided by the control Ca²⁺ rise immediately preceding 8-Br-cAMP administration for eachof the 109 neurons assayed. Data are displayed as percentages.Zero percent on the y-axis signifies that the peak rise in thepresence of 8-Br-cAMP was equivalent to the control peak Ca²⁺ rise (no modulation); values <0% represent depression, and values>0% represent response potentiation. Of note is the dual effects(both potentiation and depression) of 8-Br-cAMP on GABA-evokedCa²⁺ rises. To ensure that the GABA-evoked Ca²⁺ rise was purely postsynaptic in nature, the neurons were continuouslyperfused with TTX (1 µM) to block action potential-dependent synapticrelease of neurotransmitters.
Fig. 3. 8-Br-cAMP reduces presynaptic release of GABA. A, Brief (15 sec) repeated exogenous administrations of GABA (10 µM) (arrows)to the perfusion solution elicited rapid and reproducible postsynapticCa²⁺ rises. 8-Br-cAMP (1 mM) coadministration was capable of eitherenhancing or depressing the amplitude of GABA-evoked Ca²⁺ rises (see text). To ensure that GABA-evoked Ca²⁺ rises were exclusively postsynaptic in nature, the neurons werecontinuously perfused with TTX (1 µM) to block action potential-dependentpresynaptic transmitter release. B, Repeated electrical stimulation(E.S.) triggered reproducible Ca²⁺ rises triggered by presynaptic GABA release. Administration ofTTX (1 µM) or bicuculline (BIC, 20 µM) blocked the Ca²⁺ rise, suggesting that electrical stimulation triggered actionpotential-dependent synaptic release of GABA. Administration of8-Br-cAMP (1 mM) largely blocked the GABA activity. This experimentwas performed in the constant presence of AP5 (100 µM) and CNQX(10 µM) to block the Ca²⁺ rise elicited by glutamate receptor activation. C, D, Analysisof the modulatory effects of 8-Br-cAMP administration on GABA-evokedCa²⁺ rises (C) and on electrically evoked Ca²⁺ rises (D). Circles represent the first Ca²⁺ rise in the presence of 8-Br-cAMP divided by the control Ca²⁺ rise immediately preceding 8-Br-cAMP administration; each circlerepresents the response of a single neuron. Results are displayedas percentages of the control Ca²⁺ rise. The 0% point on the y-axis signifies that the rise in thepresence of 8-Br-cAMP was equivalent to the control Ca²⁺ rise. Values >0% represent response potentiation; values <0%represent depression. E, The effects of 8-Br-cAMP on bath applicationof GABA and electrically stimulated synaptic release of GABA onCa²⁺ rises were compared. Only neurons with control evoked Ca²⁺ rises (second Ca²⁺ rise, just before 8-Br-cAMP) from 120 to 140 nM were used toallow for an equitable comparison. See Results for details. Errorbars indicate SEM. The mean GABA-evoked Ca²⁺ rise was slightly depressed by the administration of 8-Br-cAMP(postsynaptic effect), whereas the electrically evoked rise wasdramatically depressed by 8-Br-cAMP administration (presynapticplus postsynaptic). The electrically evoked Ca²⁺ rise was virtually abolished by TTX or bicuculline. Electricalstimulation experiments were performed after 4 DIV, a period whensynaptic connections are found in most neurons.
[View Larger Version of this Image (27K GIF file)]

To determine that GABA was released by an action potential-dependent mechanism at this early stage of development, a seriesof experiments was performed on neurons at 4 DIV. Electrical stimulationcaused a large Ca²⁺ rise in both neural cell bodies and neurites. Neurites loadedwith fluo-3 (Fig. 4A) show a large electrically evoked Ca²⁺ rise localized to small regions, suggesting dendrite segmentspostsynaptic to axonal boutons (Fig. 4D). This Ca²⁺ rise was reduced by bath application of either TTX (Fig. 4B)or bicuculline (Fig. 4C). These results suggest that action potential-mediatedpresynaptic release of GABA was responsible for the Ca²⁺ rise. Ca²⁺ rises occurred in the presence of the glutamate receptor antagonistsAP5 (100 µM) and CNQX (10 µM), ruling out synaptic glutamate releaseas the cause of the Ca²⁺ rise. To demonstrate further that synapses were formed at thisdevelopmental stage, cells were immunostained with synapsin antiserum.Highly localized, punctate synapsin staining is shown in Figure4E. For control purposes, these cells were also immunostainedfor the structural protein $alpha$ -tubulin (Fig. 4F). In contrast tothe punctate synapsin staining, tubulin immunoreactivity was foundthroughout neurons and glia.
Fig. 4. Electrical stimulation triggers GABA-mediated Ca²⁺ rises in neurites. A, Fluo-3-loaded neurites are shown under control conditions(no electrical stimulation). B, In the presence of TTX (1 µM),electrical stimulation does not elicit a Ca²⁺ rise. C, Electrically induced Ca²⁺ rise is also largely inhibited by bath application of bicuculline(20 µM). D, In the absence of bicuculline and TTX, large and localized(red arrows) Ca²⁺ rises were triggered by electrical stimulation. These experimentswere performed in the presence of AP5 (100 µM) and CNQX (10 µM).A $'$ -D $'$ , High magnification of areas from A-D shown by the box inA. The color bar shows color codes of low and high Ca²⁺ levels. Scale bar, 2.5 µm. E, Neurons immunostained for synapsinI. Blue arrows indicate punctate staining, corresponding to synapselocation. F, Same region immunostained for $alpha$ tubulin. Yellow arrowsidentify the same neurite in both micrographs. Scale bar, 8 µm.
[View Larger Version of this Image (81K GIF file)]

Figure 3B shows that electrical stimulation triggered reproducible Ca²⁺ rises in the neural cell soma. The addition of either TTX (1µM) or bicuculline (20 µM) to the perfusion solution blocked therise. As in neurites, Ca²⁺ rises occurred in the presence of the glutamate receptor antagonistsAP5 (100 µM) and CNQX (10 µM). Under this condition, the additionof 8-Br-cAMP (1 mM) caused a large depression in the electricallyevoked Ca²⁺ rise. Relative to the control electrically stimulated Ca²⁺ rise immediately preceding 8-Br-cAMP administration, 8-Br-cAMPdepressed the Ca²⁺ rise by >20% in 40 of 49 neurons. No neurons exhibited a >20%potentiation of the peak evoked Ca²⁺ response. A scatter plot analysis of the effects of 8-Br-cAMPon electrically evoked Ca²⁺ rises in 49 neurons is shown in Figure 3D. Of note is the largelyinhibitory actions of 8-Br-cAMP on electrically evoked Ca²⁺ rises. This is in contrast with data for purely postsynapticallyevoked Ca²⁺ rises (Fig. 3C), suggesting that 8-Br-cAMP also affects GABAactivity mediating Ca²⁺ rises through presynaptic regulation of GABA release.

Figure 3E compares the modulatory effects of 8-Br-cAMP on Ca²⁺ rises elicited by bath-applied GABA with electrically evokedrelease of presynaptic GABA. For a comparison of effectivenessof 8-Br-cAMP on postsynaptic (GABA-evoked) and presynaptic pluspostsynaptic (electrically induced GABA release) responses, datafor Figure 3E were collected from neurons that exhibited a peakCa²⁺ rise from 120 to 140 nM during the second (control) GABA-evokedCa²⁺ rise. Ca²⁺ rises of approximately equivalent levels were used so that apresynaptic component of 8-Br-cAMP-mediated Ca²⁺ modulation could be fairly subtracted from the purely postsynapticmodulation of GABA-evoked Ca²⁺ rises. Of interest was the finding that the mean Ca²⁺ rise evoked by bath application of GABA was only slightly depressed(13%; statistically insignificant, P > 0.05, two-tailed t test)by 8-Br-cAMP, whereas electrically induced Ca²⁺ rises dependent on synaptic GABA release were highly significantly(p < 0.0001, two-tailed t test) reduced (61%). This differencein 8-Br-cAMP depression of electrically versus GABA-evoked Ca²⁺ rises (48%) was probably the result of inhibited GABA release.Unlike the other experiments, which used 5 DIV cultures, 4 DIVcultures were used for electrical stimulation experiments. Atthis time point during development, neurons were synapticallyconnected, yet the Ca²⁺-elevating action mediated by the spontaneous release of GABAwas relatively low. Taken together, these data suggest that cAMP-dependentprocesses regulate Ca²⁺ rises by decreasing the amount of presynaptic GABA release andto a lesser extent by altering postsynaptic Ca²⁺ responsiveness to GABA.

Modulation of adenylyl cyclase activity
To determine whether altering endogenous cAMP levels would modulate GABA synaptic activity mediating Ca²⁺ rises, neurons were treated either with forskolin (an adenylylcyclase activator) to increase cAMP levels or with SQ-22,536 (anadenylyl cyclase inhibitor) to decrease cAMP levels. Figure 5Ashows two representative neurons exhibiting four Ca²⁺ rises: two Ca²⁺ rises before and two Ca²⁺ rises after a 15 min application of forskolin (20 µM). The administrationof forskolin greatly depressed (>70%) the Ca²⁺ rises elicited by bicuculline withdrawal. The effects of forskolinon GABA-mediated Ca²⁺ rises are quantified in Figure 5B; 1st and 2nd refer to the twoCa²⁺ rises elicited by bicuculline withdrawal before forskolin administration,whereas 3rd and 4th refer to the Ca²⁺ rises after forskolin administration. A comparison of the firsttwo with the second two Ca²⁺ rises shows that the effects of forskolin were statisticallysignificant (p < 0.0001, two-tailed t test).
Fig. 5. Adenylyl cyclase modulation alters GABA Ca²⁺ rises. A, Before the addition of adenylyl cyclase modulators, withdrawal of bicuculline(BIC, 20 µM) elicited rapid, reproducible Ca²⁺ responses. A, After a 15 min administration of the adenylyl cyclaseactivator forskolin (20 µM), GABA-mediated Ca²⁺ rises elicited by the removal of bicuculline from the perfusionsolution were significantly depressed, relative to Ca²⁺ rises elicited before forskolin administration. B, Bar graphrepresentation of the mean Ca²⁺ rises triggered by the four bicuculline withdrawals; 1st and2nd refer the Ca²⁺ rises before forskolin administration, and 3rd and 4th referto the Ca²⁺ rises after forskolin administration. C, Relative to the initialtwo Ca²⁺ rises, the Ca²⁺ rises elicited after the administration of the adenylyl cyclaseinhibitor SQ-22,536 (100 µM) were significantly depressed. Thedashed line is meant to approximate the mean GABA-mediated Ca²⁺ rise before adenylyl cyclase modulators were added. D, Graphicalrepresentation of the mean Ca²⁺ rises triggered by the four bicuculline withdrawals; 1st and2nd refer to the two Ca²⁺ rises before SQ-22,536 administration, and 3rd and 4th referto the two Ca²⁺ rises after SQ-22,536 administration. Error bars indicate SEM.All experiments were performed in the presence of AP5 (100 µM)and CNQX (10 µM).
[View Larger Version of this Image (36K GIF file)]

Interestingly, SQ-22,536 (100 µM) also depressed the Ca²⁺ rise elicited by bicuculline withdrawal (Fig. 5C). As with forskolin,a 15 min pretreatment caused a statistically significant (p <0.05, two-tailed t test) decrease (>29%) in the mean Ca²⁺ rise initiated by bicuculline withdrawal (Fig. 5D). Together,these results indicate that both increasing and decreasing cAMPlevels through modulating adenylyl cyclase activity reduces GABA-mediatedCa²⁺ rises.

Protein kinase A inhibition
To determine whether a basal level of PKA-mediated phosphorylation plays a role in maintaining the level of GABA Ca²⁺ rises, we assessed the effect of the potent PKA inhibitors H89and Rp-cAMPS. Figure 6A shows that the administration of Rp-cAMPS(200 µM) to synaptically active neurons initiated a rapid Ca²⁺ depression. The removal of bicuculline caused a mean Ca²⁺ rise of 70 ± 6 nM. Addition of Rp-cAMPS decreased the Ca²⁺ rise to 18 ± 2 nM, representing a statistically significant (p< 0.0001, two-tailed t test) 74% decrease in Ca²⁺ activity (n = 45). Of interest was the finding that the Ca²⁺ depression triggered by Rp-cAMPS persisted for an extended periodeven after the Rp-cAMPS was washed out. Fifty-eight percent ofthe neurons assayed (26 of 45) did not recover >50% of their pre-Rp-cAMPSCa²⁺ level during any time after Rp-cAMPS withdrawal. In control experiments,none of 35 unstimulated neurons showed >50% reduction in GABACa²⁺ rises over an identical period.
Fig. 6. GABA Ca²⁺ levels are reduced by protein kinase A inhibitors. A, Administration of the protein kinase A inhibitor Rp-cAMPS (200µM) caused a rapid reduction in the Ca²⁺ level. In the top neuron, the Ca²⁺ level remained depressed for an extended period after the removalof Rp-cAMPS from the perfusion solution. B, Pretreating neuronswith Rp-cAMPS (200 µM) blocked GABA-mediated Ca²⁺ rise induction elicited by bicuculline (BIC, 20 µM) removal.C, Another protein kinase A inhibitor, H89 (15 µM), also rapidlydepressed GABA-mediated Ca²⁺ levels. As with Rp-cAMPS, the Ca²⁺ depression triggered by H89 persisted for an extended periodafter H89 withdrawal. D, The administration of H89 (15 µM) depressedCa²⁺ rises triggered by electrical stimulation (E.S., arrows) of GABArelease. Electrically induced Ca²⁺ rises could be blocked by tetrodotoxin or bicuculline (not shownhere). As with its effects on spontaneous GABA release, the effectsof H89 persisted even after it was withdrawn from the perfusionsolution.
[View Larger Version of this Image (39K GIF file)]

Rp-cAMPS also inhibited the induction of Ca²⁺ rises mediated by the synaptic release of GABA (Fig. 6B). The two representativeneurons in Figure 6B initially exhibited three robust Ca²⁺ rises, whereas after Rp-cAMPS pretreatment, bicuculline withdrawaldid not initiate a Ca²⁺ rise. As did Rp-cAMPS, a short, 2 min application of H89 (15µM) triggered a rapid Ca²⁺ depression (Fig. 6C). H89 reduced the GABA-mediated Ca²⁺ rise from 44 ± 5 to 12 ± 1 nM (n = 14). The level of H89-mediateddepression was statistically significant (p < 0.0001, two-tailedt test). As a measure of the long-term effectiveness of H89, only4 of the 14 neurons assayed recovered >50% of their pre-H89 Ca²⁺ level 30 min after H89 withdrawal.

H89 also depressed GABA activity triggered by electrical stimulation. Figure 6D shows that the brief administration of H89(15 µM) resulted in a statistically significant (p < 0.0001, two-tailedt test) depression in the Ca²⁺ rise. Electrical stimulation triggered a mean Ca²⁺ rise of 441 ± 26 nM. Addition of H89 reduced the Ca²⁺ rise to 170 ± 12 nM (n = 78). As in the endogenous activity assaysdescribed above, inhibition initiated by H89 persisted long afterit was washed from the perfusion chamber in some neurons. Theaddition of TTX or bicuculline largely blocked the electricallyevoked Ca²⁺ rise.

PKA and voltage-dependent Ca²⁺ channels
In these experiments, we addressed the mechanism of postsynaptic PKA actions. In the constant presence of TTX (1 µM), thebath application of GABA (10 µM) triggered a rapid Ca²⁺ rise that was depressed by the H89 (15 µM) administration (Fig.7A). After H89 withdrawal from the perfusion solution, neuronalCa²⁺ responsiveness to GABA slowly recovered toward pre-H89 levels.Because GABA elicits a Ca²⁺ rise through the activation of voltage-activated Ca²⁺ channels (VACCs), the direct effect of H89 on high K⁺ (15 mM)-induced Ca²⁺ rises triggered by VACC activation was assessed. Similar to itseffects on GABA, H89 administration rapidly depressed Ca²⁺ rises mediated by VACCs (Fig. 7B). After H89 withdrawal the recoveryof Ca²⁺ responsiveness had a general appearance that was very similarto the recovery of GABA responsiveness, suggesting that the H89-mediateddepression of GABA responses may result, in part, from VACC inhibition.Figure 7, C and D, shows scatter plot analyses of the effectsof H89 on GABA-evoked (n = 105) or high K⁺-evoked (n = 104) Ca²⁺ rises, respectively. Single-cell values were determined by dividingthe first evoked Ca²⁺ rise in the presence of H89 by the control-evoked Ca²⁺ rise immediately preceding H89 administration. Values are expressedas percentages of the control Ca²⁺ rise. A Ca²⁺ rise in the presence of H89 that was larger than control riseswas >0%, whereas a rise of smaller peak height than the controlrise was <0%; rises of equal peak height were 0%. Of note, theoverall level of Ca²⁺ depression elicited by H89 was greater for K⁺-evoked Ca²⁺ rises than for GABA-evoked Ca²⁺ rises. Figure 7E shows that high K⁺-induced Ca²⁺ rises were largely suppressed by the administration of the L-typeCa²⁺ channel blocker nimodipine (1 µM). A graphical representationof mean Ca²⁺ rises in response to GABA and high K⁺ before and during H89 or nimodipine application is shown in Figure7F. The mean Ca²⁺ depressions triggered by H89 and nimodipine were statisticallysignificant (p < 0.0001, two-tailed t test). These findings suggestthat tonic PKA-mediated Ca²⁺ channel phosphorylation is required for GABA to elicit a robustCa²⁺ rise.
Fig. 7. PKA inhibition reduces evoked Ca²⁺ responsiveness. A, GABA (10 µM) (arrows) elicited rapid Ca²⁺ rises that were depressed by the administration of the PKA inhibitorH89 (15 µM) in two neurons. B, H89 also depressed Ca²⁺ rises initiated by high K⁺ (15 mM) (arrows) administration. C, D, Analysis of the modulatoryeffects of H89 on GABA-evoked Ca²⁺ rises (C) or high K⁺-evoked Ca²⁺ rises (D). Circles are percentage representations of the firstCa²⁺ rise in the presence of H89 divided by the control Ca²⁺ rise immediately preceding H89 administration; each circle representsthe response of a single neuron. The 0% point on the y-axis signifiesthat the evoked rise in the presence of H89 was equivalent tothe evoked Ca²⁺ rise. Values >0% represent potentiation; values <0% representdepression. E, The L-type Ca²⁺ channel blocker nimodipine (1 µM) largely blocked Ca²⁺ rises elicited by high K⁺. Both GABA and high K⁺ were applied for 15 sec. F, Graphical representation of the meanCa²⁺ rises elicited either by GABA or high K⁺ before (white bars) or during the coadministration of H89 (blackbars) or nimodipine (striped bar). N, Total number of neuronsassayed. Error bars indicate SEM.
[View Larger Version of this Image (32K GIF file)]

Modulation of GABA Ca²⁺ rises in adenylyl cyclase-coupled neurotransmitter receptor systems
The experiments above used pharmacological tools to directly alter different stages of intracellular pathways that affectkinase-mediated phosphorylation. We include the experiments belowto demonstrate that activating neurotransmitter receptors thathave previously been shown to modulate cAMP levels (either increaseor decrease) exert actions parallel to those occurring when agentsthat act downstream of the receptor are activated (i.e., experimentsdescribed above).

We tested whether transmitter receptors shown to be either positively or negatively coupled to cAMP production alter GABACa²⁺ rises. Toward this end, we chose the well characterized dopamineD1 receptor. The D1 receptor has been shown to be coupled to anincrease in cAMP levels (Shultz et al., 1987; Steffey et al.,1991; Liu et al., 1992; Lovenberg et al., 1991). Administrationof the dopamine D1 receptor-specific agonist SKF-38393 (5 µM)triggered a rapid and reproducible depression in the GABA-mediatedCa²⁺ rise (Fig. 8A). The withdrawal of bicuculline from the perfusionsolution triggered a mean Ca²⁺ rise of 86 ± 4 nM from the basal Ca²⁺ level in the presence of bicuculline. Addition of SKF-38393 causedthe Ca²⁺ rise to decrease to 56 ± 3 nM, representing a statistically significant(p < 0.0001, two-tailed t test) 35% depression in the GABA-mediatedCa²⁺ rise (n = 79). Previously, we found that NPY (100 nM) causeda large (>70%) depression in the Ca²⁺ rise elicited by synaptically released GABA (Obrietan and vanden Pol, 1996b). An example of the Ca²⁺-depressing actions of NPY is shown in Figure 8B. Several studieshave shown that NPY receptor stimulation triggers inhibitory G-proteinactivation, leading to a decreased cAMP level (McAuley et al.,1991; Bleakman et al., 1992; Larhammar et al., 1992; Zhu et al.,1992). Additionally, administration of the muscarinic acetylcholinereceptor agonist McN-A-343 (100 µM) triggered a Ca²⁺ depression (Fig. 8C). The withdrawal of bicuculline from theperfusion solution elicited a mean Ca²⁺ rise of 96 ± 7 nM from the basal Ca²⁺ level. McN-A-343 administration caused the Ca²⁺ rise to decrease to 65 ± 5 nM, representing a statistically significant(p < 0.0001, two-tailed t test) 32% depression in the GABA-mediatedCa²⁺ rise (n = 52). A large number of studies have shown that themuscarinic acetylcholine receptors modulate cAMP levels (McKinneyet al., 1991; Schwarz et al., 1993; Burford et al., 1995; Migeonet al., 1995). Interestingly, in 13 of 58 neurons, a lower McN-A-343concentration (15 µM) increased GABA-mediated Ca²⁺ levels by >10%. In contrast, only 1 of 52 neurons treated withthe higher concentration of McN-A-343 (100 µM) showed a >10% increasein the GABA-mediated Ca²⁺ rise. These results support the hypothesis that receptor systemscoupled to either an increase or a decrease in cAMP productionmay alter GABA Ca²⁺ rises significantly.
Fig. 8. Ca²⁺ rises mediated by GABA activity are depressed by selective activation of neurotransmitter receptors coupled to adenylylcyclase regulation. The removal of bicuculline (BIC, 20 µM) fromthe perfusion solution triggered a rapid and sustained Ca²⁺ rise in the three representative neurons. A, Stimulation of theD1 receptor by the administration of SKF-38393 (5 µM) reducedthe amplitude of the spontaneous GABA-mediated Ca²⁺ rise. B, NPY (100 nM) triggered a rapid Ca²⁺ depression. Blockade of the GABA_A receptor with bicuculline atthe end of the experiment reduced Ca²⁺ to basal levels. C, Stimulation with the muscarinic acetylcholinereceptor agonist McN-A-343 (100 µM) also triggered Ca²⁺ depression. The ionotropic glutamate receptor antagonists AP5(100 µM) and CNQX (10 µM) were perfused throughout the experimentto block synaptically released glutamate from triggering a Ca²⁺ rise.
[View Larger Version of this Image (19K GIF file)]

DISCUSSION
Activation of the GABA_A receptor, either through exogenous agonist application or synaptic GABA release, elicits a Ca²⁺ rise in the majority of developing neurons from many brain regions(Obrietan and van den Pol, 1995). In the present study, we characterizedthe functional role of the cAMP signal transduction pathway interms of its ability to regulate GABA-related Ca²⁺ rises. Our data suggest that either activating or inhibitingthe cAMP signal transduction pathway significantly depressed theGABA activity detected with Ca²⁺ imaging. The results of affecting the cAMP signal transductionpathway were similar to the effects of stimulating transmitterreceptors thought to be coupled to either a decrease or an increasein cAMP levels.

PKA activation or inhibition, as described in this paper, may cause a variety of different mechanisms to work together orin opposition to one another, with the general effect being adecrease in the Ca²⁺ rise initiated by GABA-mediated neurotransmission. To our knowledge,ours is the first report characterizing the regulation of GABA-mediatedCa²⁺ rises by direct modulation of the cAMP signal transduction pathway.These effects were observed with agents that either activated(membrane-permeable cAMP analogs and forskolin) or inhibited (PKAinhibitors and SQ-22536) the cAMP signal transduction pathwayat several different points along the pathway.

Postsynaptic effects
Blocking PKA activity with H89 or Rp-cAMPS depressed peak Ca²⁺ rises elicited by the bath application of GABA. Because the presynapticrelease of GABA-containing vesicles was blocked with TTX, theobserved inhibitory effect of PKA was postsynaptic in nature.A number of possible mechanisms could account for the depressionof GABA-mediated Ca²⁺ levels observed when the cAMP signal transduction cascade wasaltered. A decrease in GABA_A receptor activity resulting froman inhibition of steady-state GABA_A receptor phosphorylation couldexplain the depression resulting from PKA inhibition. Along theselines, several studies have shown that GABA_A receptor-mediatedactivity is regulated by phosphorylation. GABA_A currents weredecreased by >90% if cells were ATP-depleted (Chen et al., 1990),suggesting that a basal level of phosphorylation was requiredfor maintenance of optimal GABA_A receptor channel function. Inaddition, GABA_A receptor conductance has been shown to be directlyaffected by PKA-mediated phosphorylation (Moss et al., 1992).In the hippocampus, the frequency of GABA-mediated giant depolarizingpotentials is modulated by 8-Br-cAMP or forskolin and inhibitedby Rp-cAMPS (Strata et al., 1995). Within this context, our resultssuggest that tonic postsynaptic PKA-mediated phosphorylation isrequired for optimal Ca²⁺ responsiveness.

Ca²⁺ responses triggered by the direct activation of VACCs (largely L-type) were also suppressed by H89. Because the abilityof GABA to elicit a Ca²⁺ rise in hypothalamic neurons is dependent on L-type Ca²⁺ channel activation (Obrietan and van den Pol, 1995), these resultssuggest that H89-mediated depression of GABA-evoked Ca²⁺ rises may result, in part, from the inhibition of L-type VACCactivity. A basal level of phosphorylation may be required foroptimal L-type Ca²⁺ channel activity; Ca²⁺ currents in HEK-293 cells transfected with the L-type Ca²⁺ channel gene were depressed by administration of PKA inhibitors(Perez-Reyes et al., 1994). Additionally, forskolin increasedthe L-type Ca²⁺ current in ferret ventricular myocytes, and this increase wasblocked by H89 (Yuan and Bers, 1995). Our results in neurons areconsistent with these findings. This does not rule out a possibleadditional effect of phosphorylation on K⁺ channels that could, in turn, influence VACCs.

Presynaptic effects
The cAMP signal transduction pathway appeared to act at both presynaptic and postsynaptic sites to affect GABA-related Ca²⁺ rises. Ca²⁺ rises triggered by electrical stimulation of presynaptic GABArelease were depressed to a much greater extent by 8-Br-cAMP thanpostsynaptic Ca²⁺ rises elicited by the bath application of GABA. Additionally,postsynaptic Ca²⁺ rises in a subpopulation of neurons were potentiated by 8-Br-cAMP,whereas potentiation was not observed when Ca²⁺ rises were elicited by electrically induced presynaptic GABArelease. These differential effects suggest that the cAMP signaltransduction pathway may inhibit presynaptic GABA release, aswell as modulate postsynaptic GABA responsiveness. This conclusionis consistent with the view that PKA has a spatially limited actionand may exert independent or opposing effects in presynaptic axonscompared with the postsynaptic somatodendritic complex.

PKA activators 8-Br-cAMP or 4-Cl-cAMP decreased GABA-related Ca²⁺ rises, although we also noted that low concentrations of 8-Br-cAMPor 4-Cl-cAMP increased Ca²⁺ levels in a subpopulation of neurons during endogenous activityassays. These Ca²⁺ modulatory effects of 8-Br-cAMP and 4-Cl-cAMP were largely througha presynaptic mechanism. For a presynaptic receptor coupled toadenylyl cyclase activation (which would result in increased PKAactivity), there have been a variety of reports describing eitherpotentiation or inhibition of transmitter release. For example,activation of the dopamine D1 receptor (coupled to cAMP production)facilitates neurotransmission in the hippocampus (Imperato etal., 1993) and in the ventral tegmetal area (Cameron and Williams,1993), whereas D1 receptor stimulation has been shown to decreaseneurotransmission in the basal forebrain (Momiyama et al., 1996)and in the shell region of the nucleus accumbens (Pennartz etal., 1992).

The exclusive effect of PKA inhibitors on Ca²⁺ rises elicited by presynaptic GABA release was inhibitory. Receptors coupledto adenylyl cyclase inhibition (which would result in decreasedPKA activity), including the GABA_B receptor (Dittman and Regehr,1996), the adenosine A1 receptor (Potier and Dutar, 1993), andthe NPY receptor (Bleakman et al., 1992), have been shown to decreasetransmitter release. These findings suggest that the effects ofPKA on transmitter release may depend on the presynaptic expressionof a variety of phosphorylation targets that may be differentiallyexpressed in different brain regions, developmental stages, orneural phenotypes. This is consistent with the presynaptic localizationof many hypothalamic neuromodulatory receptors that act throughG-proteins to regulate cAMP (Chen and van den Pol, 1996).

Long-term Ca²⁺ depression
In assays in which Ca²⁺ rises were elicited via synaptic GABA release, inhibition of PKA by H89 or Rp-cAMPS triggered a rapidand long-term Ca²⁺ depression (>30 min) in a large number of neurons (58%). Basedon the differential postsynaptic effects of PKA inhibitors, long-termCa²⁺ depression seems to be mediated through a largely presynapticmechanism. Interestingly, membrane-permeable cAMP analogs triggeredshort- but not long-term Ca²⁺ depression also through a largely presynaptic mechanism. Theseresults suggest that the cellular mechanisms that inhibit PKA-mediatedphosphorylation may be uniquely positioned to depress neural activityover extended periods.

NPY has both presynaptic and postsynaptic actions on GABA activity in developing hypothalamic neurons. Whereas NPY triggereda predominately brief postsynaptic depression of GABA-evoked Ca²⁺ rises (Obrietan and van den Pol, 1996b), presynaptic actionsof NPY on transmitter release were often long-term (Obrietan andvan den Pol, 1996b; van den Pol et al., 1996c). In addition, NPYreceptor stimulation depressed the Ca²⁺ rise in a similar percentage of neurons and for a similar durationas did direct PKA inhibition. NPY has been shown both to decreasecAMP levels in neurons (Harfstrand et al., 1987; McAuley et al.,1991) and to act through a G_i/G_o-protein-coupled mechanism toreduce Ca²⁺ rises elicited by synaptic GABA release (Bleakman et al., 1992;Obrietan and van den Pol, 1996b; van den Pol et al., 1996c). Activationof a G_i-protein-coupled mechanism could result in decreased adenylylcyclase activity and, in turn, decreased PKA activity, an effectsimilar to adding Rp-cAMPS or H89 to the perfusion solution. Theseresults indicate that the long-term effects of NPY receptor activationon GABA-mediated Ca²⁺ rises may be the result of decreased PKA activity. Other receptorsystems coupled to adenylyl cyclase regulation have been shownto trigger extended depression of neural activity, including theGABA_B receptor (Yang et al., 1994; Wagner and Alger, 1995) andmetabotropic glutamate receptor (Bolshakov and Siegelbaum, 1994;O'Mara et al., 1995). Immunohistochemical analysis has revealeda high level of adenylyl cyclase expression both in postsynapticdensities and in presynaptic axon terminals (Mons and Cooper,1995), suggesting that adenylyl cyclase may play an importantrole both as a regulator of postsynaptic membrane ion conductanceand presynaptic neurotransmitter release.

Biphasic effects of phosphorylation on GABA transmission
GABA-related Ca²⁺ rises were depressed by both strong activation and inhibition of the cAMP signal transduction system. Thisbiphasic response could be explained if the effects of PKA onGABA-mediated Ca²⁺ rises were characterized by an inverted U-shape function (Fig.9). During GABA neurotransmission, a basal level of tonic PKA-mediatedphosphorylation results in a near maximal Ca²⁺ level. This condition would put PKA activity near the top ofthe inverted U-shape function. When PKA activity is radicallyaltered, either through large increases (D1 receptor activation,forskolin, and cAMP analogs) or decreases (NPY receptor activation,SQ-22,536, Rp-cAMPS, and H89), PKA activity moves out of the regionof the inverted U-shape function that provides maximal GABA-mediatedCa²⁺ rises.
Fig. 9. Model of biphasic effect of PKA activity on GABA transmission. Proposed model describing how increases or decreases in PKAactivity result in a reduction in GABA-mediated Ca²⁺ rises. Arrows and dashed lines indicate the range of endogenousPKA activity required for maximal GABA-mediated Ca²⁺ rises. See Discussion for details.
[View Larger Version of this Image (20K GIF file)]

Low extracellular concentrations of 8-Br-cAMP (50-150 µM) or 4-Cl-cAMP (20 µM) increased GABA-mediated activity in some neurons,whereas high concentrations of 8-Br-cAMP ( $>=$ 500 µM) or 4-Cl-cAMP( $>=$ 200 µM) only decreased Ca²⁺ levels. This is consistent with the hypothesis that the basallevel of PKA activity in some neurons is just below that neededto provide a maximal level of GABA-mediated Ca²⁺ rises. As described by an inverted U-shape response, this effectwould result in a movement toward the apex of the inverted U.The data fitted to this model indicate that GABA-mediated Ca²⁺ rises depend on ongoing PKA activity, and that PKA activity mustbe maintained within a narrow zone for GABA to elicit a maximalCa²⁺ rise.

Functional role of GABA-mediated Ca²⁺ increases during early development
Changes in cytosolic Ca²⁺ levels affect a variety of developmentally regulated neural processes. Induction of Ca²⁺ influx was primarily thought to be through the activation ofclassic membrane-depolarizing transmitters such as glutamate.Recent data have shown that GABA can exert a similar depolarizingaction in developing neurons. This Ca²⁺-elevating action of GABA is not restricted to hypothalamic neuronsbut was found in the majority of developing neurons from eightbrain regions, including hippocampus, spinal cord, cortex, olfactorybulb, and striatum (Reichling et al., 1994; Obrietan and van denPol, 1995), and after severe neural injury (van den Pol et al.,1996b). The ability of GABA to increase Ca²⁺ levels suggests that it may have an important role during nervoussystem development. Along these lines, the GABA agonist muscimolcan upregulate BDNF mRNA expression in rat hippocampal neurons,and this effect is blocked by the L-type Ca²⁺ channel blocker nifedipine (Berninger et al., 1995). GABA secretiondecreased DNA synthesis in cortical progenitor cells (LoTurcoet al., 1995). GABA induces motility of embryonic cortical neuronsthrough an increase in intracellular Ca²⁺ (Behar et al., 1996). Other GABA-mediated actions during neuraldevelopment include altering neurite outgrowth (Barbin et al.,1993), triggering chemokinesis (Behar et al., 1994), inducingGABA receptor expression (Meier et al., 1984), and regulatingneural phenotype (Marty et al., 1996). We have recently reportedthat GABA triggers localized Ca²⁺ increases in developing neurites and growth cones (Obrietan andvan den Pol, 1996a), suggesting a possible Ca²⁺-dependent role for GABA in altering the directionality of growthcone motility and the rate of neurite outgrowth. Based on thesereports and the findings in our paper, during early developmentthe activation of neurotransmitter receptors (such as NPY, glutamate,dopamine, serotonin, melatonin, and acetylcholine) coupled tothe cAMP signal transduction pathway could substantially alterGABA-related Ca²⁺ rises. This, in turn, could affect the myriad of Ca²⁺-dependent developmental processes described above.

Depression of Ca²⁺ rises attributable to an inhibitory action of presynaptic neuromodulators on GABA release is only found duringearly development. Because GABA does not raise Ca²⁺ in older neurons, but may instead decrease it (Obrietan and vanden Pol, 1995), neuromodulatory inhibition of GABA release inmature neurons would be expected to exert the opposite effecton Ca²⁺. Thus, in developing neurons, modulatory inhibition of GABA releasereduces cytosolic Ca²⁺ but in mature neurons would raise Ca²⁺.

FOOTNOTES

Received Nov. 1, 1996; revised March 19, 1997; accepted April 3, 1997.

This work was supported by National Institutes of Health Grants NS10174 and NS34887, the National Science Foundation, andAir Force Office of Scientific Research.

Correspondence should be addressed to Anthony N. van den Pol, Department of Neurosurgery, Yale University, School of Medicine,333 Cedar Street, New Haven, CT 06520.

REFERENCES

Anholt RR (1994) Signal integration in the nervous system: adenylate cyclases as molecular coincidence detectors. Trends Neurosci 17:37-41[Web of Science][Medline].
Barbin G, Pollard H, Gaiarsa JL, Ben-Ari Y (1993) Involvement of GABA_A receptors in the outgrowth of cultured hippocampal neurons. Neurosci Lett 152:150-152[Web of Science][Medline].
Behar TN, Schaffner AE, Colton CA, Somogyi R, Olah Z, Lehel C, Barker JL (1994) GABA-induced chemokinesis and NGF-induced chemotaxis of embryonic spinal cord neurons. J Neurosci 14:29-38[Abstract].
Behar TN, Schaffner AE, Tran HT, Barker JL (1995) GABA-induced motility of spinal neuroblasts develops along a ventrodorsal gradient and can be mimicked by agonists of GABA-A and GABA-B receptors. J Neurosci Res 42:97-108[Web of Science][Medline].
Behar TN, Li Y-X, Tran HT, Ma W, Dunlap V, Scott C, Barker JL (1996) GABA stimulates chemotaxis and chemokinesis of embryonic cortical neurons via calcium-dependent mechanisms. J Neurosci 16:1808-1818[Abstract/Free Full Text].
Belin MF, Fevre-Montange M, Reboul A, Didier-Bazes M, Ehret M, Maitre M, Tardy M (1991) Primary dissociated cell culture of embryonic rat metencephalon: presence of GABA in serotonergic neurons. Neurosci Lett 125:101-106[Web of Science][Medline].
Ben-Ari Y, Cherubini E, Corradetti R, Gaiarsa JL (1989) Giant synaptic potentials in immature rat CA3 hippocampal neurones. J Physiol (Lond) 416:303-325[Abstract/Free Full Text].
Berninger B, Marty S, Zafra F, da Penha Berzaghi M, Thoenen H, Lindholm D (1995) GABAergic stimulation switches from enhancing to repressing BDNF expression in rat hippocampal neurons during maturation in vitro. Development (Camb) 121:2327-2335[Abstract].
Bleakman D, Harrison NL, Colmers WF, Miller RJ (1992) Investigation into neuropeptide Y-mediated presynaptic inhibition in cultured hippocampal neurones of the rat. Br J Pharmacol 107:334-340[Web of Science][Medline].
Bolshakov VY, Siegelbaum SA (1994) Postsynaptic induction and presynaptic expression of hippocampal long-term depression. Science 264:1148-1152[Abstract/Free Full Text].
Burford N, Tobin A, Nahorski S (1995) Differential coupling of m1, m2 and m3 muscarinic receptor subtypes to inositol 1,4,5-trisphosphate and adenosine 3 $'$ ,5 $'$ -cyclic monophosphate accumulation in Chinese hamster ovary cells. J Pharmacol Exp Ther 274:134-142[Abstract/Free Full Text].
Cameron DL, Williams JT (1993) Dopamine D1 receptors facilitate transmitter release. Nature 366:344-347[Medline].
Chen G, van den Pol AN (1996) NPY Y1- and Y2-like receptors coexist in pre- and postsynaptic sites: inhibition of GABA release in isolated self-innervating SCN neurons. J Neurosci 16:7711-7724[Abstract/Free Full Text].
Chen G, Trombley PQ, van den Pol AN (1996) Excitatory actions of GABA in rat developing hypothalamic neurones. J Physiol (Lond) 494:451-464[Abstract/Free Full Text].
Chen QX, Stelzer A, Kay AR, Wong RKS (1990) GABA_A receptor function is regulated by phosphorylation in acutely dissociated guinea-pig hippocampal neurons. J Physiol (Lond) 420:207-222[Abstract/Free Full Text].
Cherubini E, Gaiarsa JL, Ben-Ari Y (1991) GABA: an excitatory transmitter in early postnatal life. Trends Neurosci 14:515-519[Web of Science][Medline].
Cooper DM, Mons N, Fagan K (1994) Ca²⁺-sensitive adenylyl cyclases. Cell Signal 6:823-840[Web of Science][Medline].
Dittman JS, Regehr WG (1996) Contributions of calcium-dependent and calcium-independent mechanisms to presynaptic inhibition at a cerebellar synapse. J Neurosci 16:1623-1633[Abstract/Free Full Text].
Fukura H, Komiya Y, Igarashi M (1996) Signaling pathway downstream of GABA_A receptor in growth cone. J Neurochem 67:1426-1434[Web of Science][Medline].
Grieco D, Porcellini A, Avvedimento EV, Gottesman ME (1996) Requirement for cAMP-PKA pathway activation by M phase-promoting factor in the transition from mitosis to interphase. Science 271:1718-1723[Abstract].
Grynkiewicz G, Poenie M, Tsien RY (1985) A new generation of calcium indicators with greatly improved fluorescence properties. J Biol Chem 260:3440-3450[Abstract/Free Full Text].
Gu Q, Moss RL (1996) 17- $beta$ -Estradiol potentiates kainate-induced currents via activation of the cAMP cascade. J Neurosci 16:3620-3629[Abstract/Free Full Text].
Harfstrand A, Fredholm B, Fuxe K (1987) Inhibitory effects of neuropeptide Y on cyclic AMP accumulation in slices of the nucleus tractus solitarius region of the rat. Neurosci Lett 76:185-190[Web of Science][Medline].
Huang C-C, Hsu K-S, Gean P-W (1996) Isoproterenol potentiates synaptic transmission primarily by enhancing presynaptic calcium influx via P- and/or Q-type calcium channels in the rat amygdala. J Neurosci 16:1026-1033[Abstract/Free Full Text].
Imperato A, Obinu MC, Gessa GL (1993) Stimulation of both dopamine D1 and D2 receptors facilitates in vivo acetylcholine release in the hippocampus. Brain Res 618:341-345[Web of Science][Medline].
Impey S, Mark M, Villacres EC, Poser S, Chavkin C, Storm DR (1996) Induction of CRE-mediated gene expression by stimuli that generate long-lasting LTP in area CA1 of the hippocampus. Neuron 16:973-982[Web of Science][Medline].
Johnson BD, Scheuer T, Catterall WA (1994) Voltage-dependent potentiation of L-type Ca²⁺ channels in skeletal muscle cells requires anchored cAMP-dependent protein kinase. Proc Natl Acad Sci USA 24:11492-11496.
Larhammar D, Blomqvist A, Yee F, Jazin E, Yoo H, Wahlested C (1992) Cloning and functional expression of a human neuropeptide Y/peptide YY receptor of the Y1 type. J Biol Chem 267:10935-10938[Abstract/Free Full Text].
Lieb K, Andersen C, Lazarov N, Zienecker R, Urban I, Reisert I, Pilgrim C (1996) Pre- and postnatal development of dopaminergic neuron numbers in the male and female mouse midbrain. Dev Brain Res 94:37-43[Medline].
Liu YF, Civelli O, Zhou QY, Albert PR (1992) Cholera toxin-sensitive 3 $'$ ,5 $'$ -cyclic adenosine monophosphate and calcium signals of the human dopamine-D1 receptor: selective potentiation by protein kinase A. Mol Endocrinol 6:1815-1824[Abstract/Free Full Text].
LoTurco JJ, Owens DF, Heath MJS, Davis MBE, Kriegstein AR (1995) GABA and glutamate depolarize cortical progenitor cells and inhibit DNA synthesis. Neuron 15:1287-1298[Web of Science][Medline].
Lovenberg TW, Roth RH, Nichols DE, Mailman RB (1991) D1 dopamine receptors of NS20Y neuroblastoma cells are functionally similar to rat striatal D1 receptors. J Neurochem 57:1563-1569[Web of Science][Medline].
Marti E, Biffo S, Fasolo A (1992) Neuropeptide Y m-RNA and peptide are transiently expressed in the developing rat spinal cord. NeuroReport 3:401-404[Web of Science][Medline].
Marty S, Berninger B, Carroll P, Thoenen H (1996) GABAergic stimulation regulates the phenotype of hippocampal interneurons through the regulation of brain-derived neurotrophic factor. Neuron 16:565-570[Web of Science][Medline].
McAuley MA, Macrae IM, Farmer R, Reid JL (1991) Effects of neuropeptide Y on forskolin, $alpha$ 2- and $beta$ -adrenoceptor-regulated cAMP levels in the rat brain slice. Peptides 12:407-412[Web of Science][Medline].
McKinney M, Miller J, Gibson V, Nickelson L, Aksoy S (1991) Interactions of agonists with M2 and M4 muscarinic receptor subtypes mediating cyclic AMP inhibition. Mol Pharmacol 40:1014-1022[Abstract].
Meier E, Drejer J, Schousboe A (1984) GABA induces functionally active low-affinity GABA receptors on cultured cerebellar granule cells. J Neurochem 43:1737-1744[Web of Science][Medline].
Migeon J, Thomas S, Nathanson N (1995) Differential coupling of m2 and m4 muscarinic receptors to inhibition of adenylyl cyclase by Gi $alpha$ and G(o) $alpha$ subunits. J Biol Chem 270:16070-16074[Abstract/Free Full Text].
Momiyama T, Sim JA, Brown DA (1996) Dopamine D1-like receptor-mediated inhibition of excitatory transmission onto rat magnocellular basal forebrain neurones. J Physiol (Lond) 495:97-106[Abstract/Free Full Text].
Mons N, Cooper DMF (1995) Immunohistochemical localization of adenylyl cyclase in rat brain indicates a highly selective concentration at synapses. Proc Natl Acad Sci USA 92:8473-8477[Abstract/Free Full Text].
Moss SJ, Smart TG, Blackstone CD, Huganir RL (1992) Functional modulation of GABA_A receptors by cAMP-dependent protein phosphorylation. Science 257:661-665[Abstract/Free Full Text].
Nagel G, Hwang TC, Nastiuk KL, Nairn AC, Gadsby DC (1992) The protein kinase A-regulated cardiac Cl channel resembles the cystic fibrosis transmembrane conductance regulator. Nature 360:81-84[Medline].
O'Mara SM, Rowan MJ, Anwyl R (1995) Metabotropic glutamate receptor-induced homosynaptic long-term depression and depotentiation in the dentate gyrus of the rat hippocampus in vitro. Neuropharmacology 34:983-989[Web of Science][Medline].
Obrietan K, van den Pol AN (1995) GABA neurotransmission in the hypothalamus: developmental transition from Ca²⁺ excitatory to inhibitory. J Neurosci 15:5065-5077[Abstract].
Obrietan K, van den Pol AN (1996a) Growth cone calcium elevation by GABA. J Comp Neurol 372:167-175[Web of Science][Medline].
Obrietan K, van den Pol AN (1996b) Neuropeptide Y depresses GABA-mediated Ca²⁺ transients in developing suprachiasmatic nucleus neurons: a novel form of Ca²⁺ long-term depression. J Neurosci 16:3521-3533[Abstract/Free Full Text].
Pennartz CMA, Dolleman-Van Der Weel MJ, Kitai ST, Silva FHLD (1992) Presynaptic dopamine d1 receptors attenuate excitatory and inhibitory limbic inputs to the shell region of the rat nucleus accumbens studied in vitro. J Neurophysiol 67:1325-1334[Abstract/Free Full Text].
Perez-Reyes E, Yuan W, Wei X, Bers DM (1994) Regulation of the cloned L-type cardiac calcium channel by cyclic-AMP-dependent protein kinase. FEBS Lett 342:119-123[Web of Science][Medline].
Potier B, Dutar P (1993) Presynaptic inhibitory effect of baclofen on hippocampal inhibitory synaptic transmission involves a pertussis toxin-sensitive G-protein. Eur J Pharmacol 231:427-433[Web of Science][Medline].
Rajaofetra N (1989) Pre-natal and post-natal ontogeny of serotonergic projections to the rat spinal cord. J Neurosci Res 22:305-321[Web of Science][Medline].
Reichling DB, Kyrozis A, Wang J, MacDermott AB (1994) Mechanisms of GABA and glycine depolarization-induced calcium transients in rat dorsal horn neurons. J Physiol (Lond) 476:411-421[Abstract/Free Full Text].
Sciancalepore M, Cherubini E (1995) Protein kinase A-dependent increase in frequency of miniature GABAergic currents in rat CA3 hippocampal neurons. Neurosci Lett 187:91-95[Web of Science][Medline].
Schwarz R, Davis R, Jaen J, Spencer C, Tecle H, Thomas A (1993) Characterization of muscarinic agonists in recombinant cell lines. Life Sci 52:465-472[Web of Science][Medline].
Shultz PJ, Sedor JR, Abboud HE (1987) Dopaminergic stimulation of cAMP accumulation in cultured rat mesangial cells. Am J Physiol 253:H358-H364[Abstract/Free Full Text].
Smith RD, Goldin AL (1996) Phosphorylation of brain sodium channels in the I-II linker modulates channel function in Xenopus oocytes. J Neurosci 16:1965-1974[Abstract/Free Full Text].
Smith TW, Nikulasson S, De Girolami U, De Gennaro LJ (1994) Immunohistochemistry of synapsin I and synaptophysin in human nervous system and neuroendocrine tumors: applications in diagnostic neuro-oncology. Clin Neuropathol 12:335-342.[Web of Science]
Steffey ME, Snyder GL, Barrett RW, Fink JS, Ackerman M, Adams P, Bhatt R, Gomez E, MacKenzie RG (1991) Dopamine D1 receptor stimulation of cyclic AMP accumulation in COS-1 cells. Eur J Pharmacol 207:311-317[Web of Science][Medline].
Strata F, Sciancalepore M, Cherubini E (1995) Cyclic AMP-dependent modulation of giant depolarizing potentials by metabotropic glutamate receptors in the rat hippocampus. J Physiol (Lond) 489:115-125[Abstract/Free Full Text].
Surmeier DJ, Bargas J, Hemmings HCJ, Nairn AC, Greengard P (1995) Modulation of calcium currents by a D1 dopaminergic protein kinase/phosphatase cascade in rat neostriatal neurons. Neuron 14:385-397[Web of Science][Medline].
van den Pol AN, Obrietan K, Cao V, Trombley PQ (1995) Embryonic hypothalamic expression of functional glutamate receptors. Neuroscience 67:419-439[Web of Science][Medline].
van den Pol AN, Cao V, Belousov AB (1996a) Dopamine enhancement and depression of glutamate-regulated calcium and electrical activity in hypothalamic neurons. J Neurophysiol 46:3934-3948.
van den Pol AN, Obrietan K, Chen G (1996b) Excitatory actions of GABA after neuronal trauma. J Neurosci 16:4283-4292[Abstract/Free Full Text].
van den Pol AN, Obrietan K, Chen G, Belousov AB (1996c) Neuropeptide Y-mediated long-term depression of excitatory activity in suprachiasmatic nucleus neurons. J Neurosci 16:5883-5895[Abstract/Free Full Text].
Wagner JJ, Alger BE (1995) GABAergic and developmental influences on homosynaptic LTD and depotentiation in rat hippocampus. J Neurosci 15:1577-1586[Abstract].
Yamashita M, Fukuda Y (1993) Calcium channels and GABA receptors in the early embryonic chick retina. J Neurobiol 24:1600-1614[Web of Science][Medline].
Yang XD, Connor JA, Faber DS (1994) Weak excitation and simultaneous inhibition induce long-term depression in hippocampal CA1 neurons. J Neurophysiol 71:1586-1590[Abstract/Free Full Text].
Yuan W, Bers DM (1995) Protein kinase inhibitor H-89 reverses forskolin stimulation of cardiac L-type calcium current. Am J Physiol 268:C651-C659[Abstract/Free Full Text].
Yuste R, Katz LC (1991) Control of postsynaptic Ca²⁺ influx in developing neocortex by excitatory and inhibitory neurotransmitters. Neuron 6:333-344[Web of Science][Medline].
Zhang H, Li Y-C, Young AP (1993) Protein kinase A activation of glucocorticoid-mediated signaling in the developing retina. Proc Natl Acad Sci USA 90:3880-3884[Abstract/Free Full Text].
Zhu J, Li W, Toews ML, Hexum TD (1992) Neuropeptide Y inhibits forskolin-stimulated adenylate cyclase in bovine adrenal chromaffin cells via a pertussis toxin-sensitive process. J Pharmacol Exp Ther 263:1479-1486[Abstract/Free Full Text].

Copyright ©1997 Society for Neuroscience   0270-6474/1997/174785-15$05.00/0

This article has been cited by other articles:

S. Sivakumaran, M. H. Mohajerani, and E. Cherubini
At Immature Mossy-Fiber-CA3 Synapses, Correlated Presynaptic and Postsynaptic Activity Persistently Enhances GABA Release and Network Excitability via BDNF and cAMP-Dependent PKA
J. Neurosci., February 25, 2009; 29(8): 2637 - 2647.
[Abstract] [Full Text] [PDF]

H. J. Choi, C. J. Lee, A. Schroeder, Y. S. Kim, S. H. Jung, J. S. Kim, D. Y. Kim, E. J. Son, H. C. Han, S. K. Hong, et al.
Excitatory Actions of GABA in the Suprachiasmatic Nucleus
J. Neurosci., May 21, 2008; 28(21): 5450 - 5459.
[Abstract] [Full Text] [PDF]

J. Fernandez-Solari, C. Scorticati, C. Mohn, A. De Laurentiis, S. Billi, A. Franchi, S. M. McCann, and V. Rettori
Alcohol inhibits luteinizing hormone-releasing hormone release by activating the endocannabinoid system
PNAS, March 2, 2004; 101(9): 3264 - 3268.
[Abstract] [Full Text] [PDF]

H. Dziema and K. Obrietan
PACAP Potentiates L-Type Calcium Channel Conductance in Suprachiasmatic Nucleus Neurons by Activating the MAPK Pathway
J Neurophysiol, September 1, 2002; 88(3): 1374 - 1386.
[Abstract] [Full Text] [PDF]

K. Obrietan, X.-B. Gao, and A. N. van den Pol
Excitatory Actions of GABA Increase BDNF Expression via a MAPK-CREB-Dependent Mechanism---A Positive Feedback Circuit in Developing Neurons
J Neurophysiol, August 1, 2002; 88(2): 1005 - 1015.
[Abstract] [Full Text] [PDF]

T. S. Perrot-Sinal, A. M. Davis, K. A. Gregerson, J. P. Y. Kao, and M. M. McCarthy
Estradiol Enhances Excitatory Gammabutyric Acid-Mediated Calcium Signaling in Neonatal Hypothalamic Neurons
Endocrinology, June 1, 2001; 142(6): 2238 - 2243.
[Abstract] [Full Text] [PDF]

K. Strange, T. D. Singer, R. Morrison, and E. Delpire
Dependence of KCC2 K-Cl cotransporter activity on a conserved carboxy terminus tyrosine residue
Am J Physiol Cell Physiol, September 1, 2000; 279(3): C860 - C867.
[Abstract] [Full Text] [PDF]

Q.-S. Liu, P. R. Patrylo, X.-B. Gao, and A. N. van den Pol
Kainate Acts at Presynaptic Receptors to Increase GABA Release From Hypothalamic Neurons
J Neurophysiol, August 1, 1999; 82(2): 1059 - 1062.
[Abstract] [Full Text] [PDF]

Y. Kakazu, N. Akaike, S. Komiyama, and J. Nabekura
Regulation of Intracellular Chloride by Cotransporters in Developing Lateral Superior Olive Neurons
J. Neurosci., April 15, 1999; 19(8): 2843 - 2851.
[Abstract] [Full Text] [PDF]

A. N. van den Pol, X.-B. Gao, P. R. Patrylo, P. K. Ghosh, and K. Obrietan
Glutamate Inhibits GABA Excitatory Activity in Developing Neurons
J. Neurosci., December 15, 1998; 18(24): 10749 - 10761.
[Abstract] [Full Text] [PDF]

D. W Ali, S. Catarsi, and P. Drapeau
Ionotropic and metabotropic activation of a neuronal chloride channel by serotonin and dopamine in the leech Hirudo medicinalis
J. Physiol., May 15, 1998; 509(1): 211 - 219.
[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 (31)

Citing Articles via Google Scholar

Google Scholar

Articles by Obrietan, K.

Articles by van den Pol, A. N.

Search for Related Content

PubMed

PubMed Citation

Articles by Obrietan, K.

Articles by van den Pol, A. N.