Adenosine Induces Inositol 1,4,5-Trisphosphate Receptor-Mediated Mobilization of Intracellular Calcium Stores in Basal Forebrain Cholinergic Neurons

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The Journal of Neuroscience, September 1, 2002, 22(17):7680-7686

Adenosine Induces Inositol 1,4,5-Trisphosphate Receptor-Mediated Mobilization of Intracellular Calcium Stores in Basal Forebrain Cholinergic Neurons
Radhika Basheer¹, Elda Arrigoni², Hemant S. Thatte³, Robert W. Greene⁴, Indu S. Ambudkar⁵, and Robert W. McCarley¹
Departments of ¹ Psychiatry, ² Neurology, and ³ Surgery, Harvard Medical School, Veterans Affairs Medical Center, West Roxbury, Massachusetts 02132, ⁴ Department of Psychiatry, University of Texas Southwestern Medical Center and Dallas Veterans Affairs Medical Center, Dallas, Texas 75390, and ⁵ Secretory Physiology Section, Gene Therapy and Therapeutics Branch, National Institute of Dental and Craniofacial Research, National Institutes of Health, Bethesda, Maryland 20892

  ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In the cholinergic basal forebrain, we found previously that the extracellular adenosine concentration increase that accompaniessleep deprivation, acting via the A₁ receptor, led to activationof the transcription factor nuclear factor- $kappa$ B and to the upregulationof A₁ adenosine receptor mRNA. We thus began to examine intracellularsignaling mechanisms. We report here that adenosine, acting ina dose-dependent manner and predominantly via A₁ receptors, stimulatedIP₃ receptor-regulated calcium release from intracellular stores.To the best of our knowledge, this calcium signaling pathway effectis a novel action of the G_i-coupled A₁ adenosine receptor in neurons.Moreover, this calcium mobilization was not seen at all in noncholinergicneurons but was present in a large proportion of cholinergic neurons.These data suggest a potential role for a calcium-signaling pathwayin adenosine-induced long-term effects of sleep deprivation anda key role for cholinergic neurons in thisprocess.

Key words: adenosine; cholinergic basal forebrain; A₁ adenosine receptor; intracellular calcium mobilization; inositol 1,4,5-trisphosphate receptor activation; sleep deprivation

  INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

There is now considerable evidence that adenosine, acting in the basal forebrain (BF), is a homeostatic sleep factor regulatingthe increased propensity to sleep after an increased durationof wakefulness (Porkka-Heiskanen et al., 1997; Basheer et al.,1999, 2000). There is also a considerable body of evidence aboutthe immediate effects of adenosine on postsynaptic membrane ionicmechanisms. Adenosine, via the A₁ receptor, activates an inwardlyrectifying potassium current and blocks the hyperpolarizing current,thereby causing hyperpolarization of neurons (Rainnie et al.,1994; for review, see Haas and Selbach, 2000).

In contrast, very little is known in the brain, and nothing in the BF, about the long-term effects of adenosine that may bemediated by prolonged receptor activation and second messenger-mediatedintracellular mechanisms. This may be important not only fromthe standpoint of the intrinsic value of increased cellular andbiological knowledge but also for the possible behavioral consequencesof such actions. For example, sleep restriction over several daysproduces progressive, additive effects such as decreased neurobehavioralalertness, decreased verbal learning, and changes in metabolic,endocrine, and immune functions, often referred to as "sleep debt"(Dinges et al., 1995, 1997; Spiegel et al., 1999; Drummond etal., 2000). Such effects might stem from adenosine receptor-mediatedactivation of second-messenger pathways that ultimately lead toaltered transcription of genes coding for proteins that are importantin the long-term effects of sleepdeprivation.

The BF cholinergic zone has cells with several neurotransmitter phenotypes, including cholinergic, GABAergic, glutamatergic,and peptidergic (Gritti et al., 1993; Zaborszky et al., 1999;Semba, 2000). It has not been clear whether one or more of thesecell types is associated with a distinctive second-messenger profileand hence might be associated with a distinctive functional role.The A₁ receptor-mediated immediate ionic effects do not appearto discriminate between cell types, because they occur in cholinergicand noncholinergic neurons, at least in the laterodorsal tegmentalnucleus (Rainnie et al., 1994).

Our previous identification of increased nuclear factor (NF)- $kappa$ B DNA binding as a consequence of sleep deprivation and an effectmediated by the A₁ receptor (Basheer et al., 2001a) suggestedthat we should first look at the possible signaling pathways couplingthe A₁ receptor to activation of this transcription factor. SeveralG_i/o-coupled receptors have been shown to be capable of "dualsignaling" [i.e., inhibition of adenylate cyclase and stimulationof phospholipase C (PLC)] (Gudermann et al., 1996, 1997). In smoothmuscle cells and astrocytes, the A₁ adenosine receptor has beenshown to be capable of dual signaling (Gerwins and Fredholm, 1992;Biber et al., 1997). Activation of the PLC pathway is capableof activating protein kinase C (PKC) by IP₃-mediated mobilizationof internal calcium (Nishizuka, 1992; Berridge, 1998). Finally,PKC-mediated phosphorylation of the inhibitor I- $kappa$ B and subsequentrelease and nuclear translocation of NF- $kappa$ B are very well characterizedin T lymphocytes (McKinsey et al., 1997). However, A₁ adenosinereceptor-mediated activation of the PLC pathway and mobilizationof intracellular calcium have not been reported in neurons, althoughthere are reports of transient changes in intracellular calciumthat can act as a part of a signal cascade coupling receptor activationto the nuclear events regulating transcription (Hardingham andBading, 1999).

We thus chose to examine the intracellular signal transduction cascade activated by adenosine. More specifically, we investigatedthe following possible cascade components: whether adenosine wascapable of inducing an increase in cytosolic calcium; the intracellularor extracellular source of this calcium; the involvement of theendoplasmic reticulum (ER) IP₃ receptor (IP₃R) versus the ryanodinereceptor (RyR); and the adenosine receptor type(s) mediating theseeffects.

We report here that in the BF, adenosine acts to mobilize cytosolic calcium in a dose-dependent manner, that this mobilizationis mediated by the ER IP₃R, and that these actions occur primarilythrough the A₁ adenosine receptor. Moreover, these events occuronly in cholinergicneurons.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Experimental animals. Male Long-Evans rats (350-300 gm) were housed in a 12 hr light/dark cycle (lights on 7:00 A.M. to 7:00P.M.) at a constant temperature (23°C) with access to food andwater ad libitum.

Acute brain slice preparation and loading of calcium orange dye. The animals were decapitated after isoflurane-induced anesthesia,and their brains were rapidly removed. Coronal sections (200 µmthick) were cut with a vibratome (TPI series 3000; St. Louis,MO) at 4°C in artificial CSF (aCSF; in mM: 124 NaCl, 2 KCl, 3KH₂PO₄, 1.3 MgCl₂, 2.5 CaCl₂, 26 NaCO₃, and 10 glucose, pH 7.35;315-320 mOsm when gassed with 95% O₂ and 5% CO₂). Three slicesper animal [bregma coordinates from 0 to 0.6 (Paxinos and Watson,1998), including the horizontal and diagonal band (HDB)-substantiainnominata (SI)-magnocellular preoptic area (MCPO) region of theBF] were collected. The slices were hemisected and mounted onParafilm. Calcium orange dye in aCSF (1 ml; 10 µM final concentration)was layered over the brain slice and incubated for 1 hr at 21°C;slices were washed and used for drug treatment and imaging incarboxygenated buffer. Uniform loading of the dye was evidentbecause of the visible levels of basal fluorescence of calciumorange in resting (unstimulated) neurons. Tetrodotoxin (1 µM)in the buffer was used for all of the experiments to ensure thepostsynaptic nature of the effects. The real-time change in intracellularcalcium fluorescence was measured every 1.37 sec to determinethe time needed for maximumeffect.

To test the effect of fixing the slices in neutralized formalin on the intensity of calcium orange, we performed a time-courseexperiment in which calcium orange-loaded slices (four slicesper time point from four rats) were treated with 100 µM adenosinefor 0, 10, 20, 30, 40, 60, and 100 sec and fixed in formalin atthe end of each time point before the fluorescence intensity wasmeasured. The process of fixing did not have any effect on theincrease in fluorescence intensity in response to adenosine. Thetime course of fluorescence intensity increase in fixed slicesfollowed the same pattern that was observed in real-time measurements(Fig. 1A,B).

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Figure 1. Effect of adenosine on the intracellular calcium of BF neurons. A, Typical time course of calcium increase, measured as increase in calcium orange fluorescence in a live neuron in an acute slice after treatment with 100 µM adenosine (two photon microscope measurements every 1.37 sec). Insets, Photomicrographs of a cell at the indicated time points. Note that the maximal fluorescence is achieved by 45-60 sec, and note the size of the neuron. Scale bar, 25 µm. B, Time course of fluorescence of neurons in slices fixed at various times after adenosine treatment (100 µM). Insets, Photomicrographs of neurons in slices fixed at the indicated time points. Note the close correspondence to the time course of fluorescence in an unfixed neuron (A) and the sizes of the neurons. Scale bar, 50 µm. C, Adenosine concentration-response curve: adenosine concentrations and mean ± SEM fluorescence are shown (n = 11 neurons per point). Note that the maximum response is achieved at 100 µM adenosine, the concentration chosen for other experiments.

Drugs. The sources of the drugs used were as follows: adenosine, the RyR blocker 1,1'-diheptyl-4-4'-bipyridinium (DHBP), theIP₃R blocker xestospongin C, and 2-aminoethoxydiphenylborane (2APB)were obtained from Calbiochem (La Jolla, CA). The A₁ agonist N⁶-cyclo-hexyl-adenosine (CHA), A₁ antagonist 8-cyclopentyl-1,3-dimethylxanthine(CPT), A₂ agonist N⁶-[2-(3,5-dimethoxyphenyl)-2-(methylphenyl)-ethyl]adenosine (DPMA),A₃ agonist N⁶-(4-aminobenzyl)-9-[5-(methylcarbonyl)- $beta$ -D-ribofuranosyl]adenine(AB-MECA), and A₃ antagonist 3-ethyl-5-benzyl-2-methyl-4-phenylethynyl-dihydropyridine-dicarboxylate(MRS1191) were obtained from Sigma-RBI (St. Louis,MO).

Immunofluorescence labeling.Coronal sections that were used for calcium imaging were fixed in buffered formalin,pH 7.2, permeabilizedwith 0.5% TritonX-100in PBS under constant shaking for 2 hr, andsubsequently treated with specific ChAT antibody (AB 144; goatantibody; Chemicon, Temecula, CA) used at a dilution of 1:4000.FITC-conjugated secondary antibody (anti-goat antibody; 1:100dilution; Chemicon) was used to visualize ChAT-positive neurons.Samples were imaged by multiphotonmicroscopy.

Multiphoton microscopy for intracellular calcium imaging.A Bio-Rad (Hercules, CA) MRC 1024ES Multiphoton Imaging system coupledwith a mode-locked Spectra-Physics (Fremont, CA) tunable Tsunami-sapphirelaser system (pulse duration,<80 fsec;repetition rate,82 MHz)and a Zeiss (Oberkochen, Germany) Axiovert S100 inverted microscopeequipped with a high-quality water immersion objective (40×; 1.2numerical aperture) was used for quantitative fluorescence imagingof samples in epifluorescence mode. Multiphoton excitation wasbased on the principle that a fluorophore can absorb two or morephotons essentially simultaneously and thereby undergo a transitionto an excited state (Denk et al., 1995). Labeled neurons in thebrain sections were identified by XYZ scanning, generally at depthsof 30-170 µm. The 512 × 512 pixel images were collected in a directdetection configuration at a pixel resolution of 0.484 µm witha Kalman 3 collection filter. Multiple labeled images were acquiredin separate channels using narrow bandpass filters to restrictthe emission wavelength and thus avoid bleed-through of aberrantfluorescence. Images were reconstructed and processed using Bio-RadLaserSharp and Metamorph (Universal Imaging, West Chester, PA)software. The data are presented as the average of at least threeblinded experiments performed on differentdays.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Adenosine mediates cytosolic calcium increase in a time- and concentration-dependent manner

To investigate the effect of adenosine on the intracellular calcium response, brain slices were loaded with calcium orange,a calcium-sensitive fluorescent dye used previously in slices(Duffy and MacVicar, 1996). The temporal kinetics of the adenosine-mediatedcalcium response was examined in 18 individual neurons (n = 3rats; three slices per rat) in real time (Fig. 1A). The temporalprofile of adenosine-mediated calcium mobilization after 0, 10,20, 30, 40, 60, and 100 sec of adenosine treatment (11-15 neuronsper time point) was examined by measuring the fluorescence intensityafter fixing the slices (four slices per time point from fourrats) at the end of each time point (see Materials and Methods)(Fig. 1B). Although fixing with neutralized formalin increasedthe overall intensity of the fluorescence in slices, the net change(cytosolic minus background fluorescence) was found to be comparablewith that observed in living neurons in real time. Similar resultswere obtained in calcium orange-loaded, cultured human embryonickidney (HEK) 293 cells, in which cytosolic calcium fluorescenceintensity remained stable without any leak into the medium afterfixation with formalin (data not shown). In both cases (i.e.,with or without fixing), the maximal (fourfold to sixfold) increasein calcium orange fluorescence was attained by 45-60 sec afteradenosine treatment (Fig. 1A,B). Consequently, this time periodwas chosen for adenosine treatment in the rest of our experiments.As shown in Figure 1C, the intracellular calcium increased ina dose-dependent manner with increasing concentrations of adenosine,reaching a maximal effect at 100 µM. Consequently, all of theexperiments described below were performed using 100 µM adenosinefor 60sec.

Adenosine-mediated cytosolic calcium increase was selective to cholinergic neurons

Interestingly, the calcium mobilization induced by adenosine in brain slices was limited to a selective subpopulation of neuronsthat were ~25-35 µm in size and located in the cholinergic portionof the BF region, which includes the HDB, the SI, and the MCPO.The observation that only a limited population of cells showedcalcium mobilization with adenosine treatment was intriguing.To rule out potential artifacts caused by differential loadingof the dye calcium orange in a specific cell type, we examinedmobilization of intracellular calcium with thapsigargin (50 µMfor 60 sec), an intracellular calcium pump inhibitor that is knownto release calcium from internal stores in all cell types. Subsequentimmunolabeling for ChAT showed that the thapsigargin-mediatedincrease in calcium orange fluorescence was seen in both cholinergicand noncholinergic cells (Fig. 2, right). In contrast, only thoseneurons with an increase in calcium orange fluorescence in responseto adenosine were ChAT-positive (Fig. 2, left). In this analysis,a total of 129 ChAT-positive neurons (average size, 31.7 ± 2.9µm) in the HDB-SI-MCPO area of the BF were examined (seven slices).Of these, 83 neurons (64.3%) showed an adenosine-mediated increasein fluorescence, whereas the remaining 46 (35.7%) did not showan increase in fluorescence in response to adenosine. The latterappeared similar in fluorescence to ChAT-positive neurons fromcontrol slices that were loaded with the fluorescent dye but nottreated with adenosine.

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Figure 2. Adenosine-induced cytosolic calcium increase was seen only in cholinergic neurons of the BF. Left column, Effect of adenosine (60 sec) treatment. Right column, Effects of thapsigargin (60 sec) treatment. Top, The calcium orange fluorescence retained in the neurons after immunolabeling for ChAT. Middle, Immunolabeling of the same neurons for ChAT, detected using FITC-conjugated secondary antibody. Bottom, Overlay showing double fluorescence. Note the presence of calcium fluorescence primarily in cholinergic neurons with adenosine (yellow arrowhead). One cholinergic neuron in A (white arrowhead) does not show calcium orange fluorescence. Calcium orange fluorescence is increased in thapsigargin-treated slices (B) in both cholinergic (yellow arrowhead) and noncholinergic (white arrowhead) cells. Images were acquired separately in each channel (dual-scan mode) to eliminate the possibility of signal bleed-over from one channel to another.

An A₁-selective agonist largely mimicked the pattern of adenosine response

The increase in intracellular calcium in response to adenosine (100 µM; n = 51) was measured in individual neurons in slices,as were the responses to the A₁ receptor-selective agonist CHA(100 nM; n = 22), the A₂-selective agonist DPMA (100 nM; n = 11),and the A₃-selective agonist AB-MECA (10 nM; n = 33) (Fig. 3A).At these concentrations, these agonists have been shown to haverelatively high selectivity for their respective receptor subtypes(Klotz, 2000). A Kruskal-Wallis one-way ANOVA showed significantdifferences among the treatment groups (H = 115.054; df = 4; p< 0.001). Post hoc analysis (Dunn's method) showed a significantincrease (p < 0.05) in cytosolic calcium with adenosine, CHA,or AB-MECA treatment compared with controls (nonstimulated basal-levelfluorescence; n = 45). The observed fivefold increase in fluorescencewith adenosine treatment was closely matched by application ofthe A₁-selective agonist CHA. The A₃-selective agonist inducedonly a twofold increase in fluorescence compared with controls.The fluorescence in the cells treated with the A₂-selective agonistDPMA was not significantly different from controls.

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Figure 3. Cytosolic calcium increase in response to different adenosine (AD) receptor agonists: A, A significant increase in cytosolic calcium fluorescence was observed in response to adenosine. A similar response was obtained by treatment with the A₁ agonist CHA compared with controls (p < 0.01). There was a twofold increase in cytosolic calcium fluorescence with treatment with the A₃ agonist AB-MECA versus controls (p < 0.05), whereas the A₂ agonist DPMA had no significant effect. B, The effect of adenosine was significantly but partially blocked by pretreatment of slices with the A₁-selective antagonist CPT (significantly lower than adenosine treatments but higher than controls; p < 0.05). However, combined use of CPT and the A₃-selective antagonist MRS1191 rendered the adenosine response not significantly different from controls. The asterisks describe a significant difference when compared with controls.

Figure 3B shows that although the effect of adenosine was not blocked completely, it was primarily blocked by pretreatmentof the slices with the A₁-selective antagonist CPT (1 µM; n =58). The effect was blocked completely when both CPT (1 µM) andthe A₃-selective antagonist MRS1191 (100 nM; n = 58) were used(differences between the treatment groups were statistically significantas determined by Kruskal-Wallis nonparametric ANOVA; H = 97.252;df = 3; p < 0.001).

Adenosine-mediated cytosolic calcium increase is caused by release from an intracellular thapsigargin-sensitive calcium store

Increases in cytoplasmic calcium can be a result of influx of external calcium or release from intracellular stores. To determinewhether the increase in cytosolic calcium was a result of influxfrom the external medium, the calcium orange-loaded slices weretreated with adenosine in calcium-free buffer. The increases incytosolic calcium in response to adenosine, CHA, and AB-MECA incells stimulated in calcium-free medium were not significantlydifferent from that seen in the presence of calcium in the externalmedium (illustrated in Fig. 4A; a Kruskal-Wallis one-way ANOVAconfirmed the visual impression by a statistically significantdifference between the calcium and the no-calcium treatment groups:H = 173.777; df = 9; p < 0.001). This suggested that the sourceof calcium was from internal stores.

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Figure 4. The adenosine (AD)-induced cytosolic increase in calcium is independent of calcium in the external medium. A, The changes in cytosolic fluorescence intensity were compared for slices in the presence and absence of calcium in the external medium for each treatment group. Filledbars denote the values observed in the presence of calcium, and open bars represent the values obtained in calcium-free medium. Kruskal-Wallis one-way ANOVA showed statistically significant differences between the groups (H = 173.77; df = 9; p < 0.001; post hoc analysis by Dunn's method was done for comparison of different treatment groups vs controls). Note that treatment with the adenosine A₁ agonist CHA as well as treatment with the A₃ agonist AB-MECA resulted in increased mobilization of cytosolic calcium regardless of the presence of calcium in the external medium. B, Pretreatment of slices with 50 µM thapsigargin to deplete internal stores of calcium abolished the response to adenosine (p < 0.01). The asterisks describe a significant difference when compared with controls.

In a separate experiment, depletion of the internal stores by pretreatment of slices with thapsigargin failed to show a calciumresponse measured after 60 sec of adenosine treatment (H = 45.987;df = 2; p < 0.001) (Fig. 4B). This also confirmed that the adenosine-mediatedincrease in cytosolic calcium was a result of mobilization froman internalsource.

Adenosine-mediated calcium release from IP₃R but not RyR regulated intracellular stores

In neurons, a major source of internal calcium is the stores present in the elaborately distributed network of the ER. BothIP₃Rs and RyRs distributed throughout the ER are responsible forreleasing calcium from this internal source (Kostyuk and Verkhratsky,1994; Simpson et al., 1995). To determine whether both or eitherone of these was responsible for the release of internal calcium,we examined the effect of blocking each of those receptors oncytosolic calcium increase in response to adenosine. Three slicesper pharmacological agent were pretreated with DHBP (30 µg/ml),a potent antagonist of RyRs (Kang et al., 1994); xestosponginC (20 µM), a potent cell-permeable blocker of IP₃R (Gafni et al.,1997); and 2APB (50 µM), a functional and membrane-permeable IP₃Rantagonist (Hamada et al., 1999) for 10 min. The drug treatmentalone did not produce any increase in the fluorescence. Blockingof RyR with DHBP (n = 15) did not prevent an adenosine-mediatedincrease in fluorescence, whereas treatment of the slice witheither of the IP₃R blockers (xestospongin C, n = 26; 2APB, n =18) significantly reduced the increase in fluorescence seen withadenosine (H = 55.864; df = 4; p < 0.001) (Fig. 5). These resultssuggested that adenosine mobilizes intracellular calcium primarilyvia IP₃Rs and not via RyRs.

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Figure 5. Inhibition of IP₃R but not RyR blocks the effect of adenosine (AD) on intracellular calcium. A significant increase in intracellular calcium by adenosine (p < 0.01) was unaffected when RyR activity was blocked by DHBP. Conversely, blocking the IP₃R with xestospongin C (XeC) or 2APB led to no response to adenosine treatment. The difference between the groups was significant by Kruskal-Wallis one-way ANOVA (H = 55.864; df = 4; p < 0.001; Dunn's post hoc analysis was done for multiple comparisons vs controls). The asterisks describe a significant difference when compared with controls.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The present study demonstrated that adenosine stimulated cytosolic calcium increases in a subpopulation of cholinergic neuronsin the BF of rats. This intracellular calcium increase was a resultof internal release, primarily via IP₃Rs, in the absence of calciuminflux. The response to adenosine was mediated predominantly byA₁ receptors, with a smaller but significant contribution by A₃adenosine receptors. Both A₁ and A₃ receptors are coupled to inhibitoryG-proteins. Although there is evidence in the literature for A₃receptor-mediated activation of IP₃ production and calcium mobilizationin neurons (Abbracchio et al., 1995) and for A₁ receptor-mediatedcalcium signaling in smooth muscle cells and astrocytes (Gerwinsand Fredholm, 1992; Biber et al., 1997), this report is the first,to the best of our knowledge, to show A₁ receptor-mediated mobilizationof IP₃-regulated intracellular calcium in a subpopulation of cholinergicneurons in theBF.

Our data demonstrated that adenosine induced a relatively slow release of intracellular calcium from internal calcium storesand that it occurred at higher concentrations of adenosine. Thetime course of calcium increase was similar to that in other reportson PLC-linked G-protein-coupled receptors, such as metabotropicglutamate receptor 5 and the angiotensin II receptor (Ceolottoet al., 2001; Nash et al., 2001). The fact that IP₃-dependentmobilization of intracellular calcium is dependent on a high concentrationof adenosine, similar to what has been described in astrocytesby Biber et al. (1997), supports the notion that increased agonist,and a consequently higher number of stimulated receptors, wouldrelease a larger number of G-protein $beta$ $gamma$ subunits and thus potentiatethe activation of PLC (Camps et al., 1992). Recently, G-protein $beta$ $gamma$ subunit-mediated activation of PLC and a subsequent increasein cytosolic calcium caused by release from internal stores hasbeen reported for G₁-coupled dopamine D₂ receptors in the striatum(Hernández-López et al., 2000). In neurons, the ER contributessignificantly to the dynamics of calcium signaling by acting aseither a source or a sink of calcium (Simpson et al., 1995; Berridge,1998, 2000). Both IP₃Rs and RyRs are widely distributed in brainER and can influence the release of internal calcium (McPhersonet al., 1991; Seymour-Laurent and Barish, 1995). Our results stronglysuggest that adenosine-dependent calcium increase in cholinergicneurons is mediated via IP₃Rs.

Calcium mobilization in cholinergic neurons of the BF

The selectivity of adenosine-induced calcium mobilization in cholinergic neurons is of interest in disambiguating the rolesof different neurotransmitter phenotypes in the BF. That the increasein intracellular calcium fluorescence was always in cholinergicneurons suggested a selective functional recruitment of a subpopulationof cholinergic neurons in the BF. Recently, selective actionsof galanin on cholinergic versus noncholinergic neurons in theHDB of the BF have been noted (Jhamandas et al., 2002). The cholinergicneurons examined in this study belong to part of the HDB, SI,and MCPO. These cholinergic neurons target both the neocortexand amygdala and regulate aspects of arousal, cognition, attention,and emotion (Szymusiak, 1995; Semba, 2000). Several approachestoward disentangling the anatomy of the cholinergic subpopulationshave been adopted; for example, neurochemical distinctions maybe based on the immunohistochemical studies for the coexpressionof several neuropeptides (for review, see Semba, 2000). Recently,a functional correlation based on the firing pattern of cholinergicneurons was used to determine the projections to the retrosplenialor prefrontal cortex in separate sets of cholinergic neurons inthe BF (Manns et al., 2000). Our data point to a large population(65%) of cholinergic neurons with a unique biochemical responseto adenosine of calcium mobilization from internalstores.

An interesting question is the possible mechanism(s) by which the adenosine receptor, particularly the A₁ receptor, knownfor its wide presence on all types of cells, exhibits a selectivebiochemical response in cholinergic neurons. Site- and context-specificdifferential activation of G-protein-coupled receptors has beenposited to occur as a result of different molecular interactions,either by homodimerization-heterodimerization or interactionswith accessory proteins to influence the activity of the receptor(for review, see Bouvier, 2001). In particular, A₁ adenosine receptorfunction can be influenced by a homodimer (Ciruela et al., 1995),by a heterodimer (Gines et al., 2000; Ciruela et al., 2001), andby interaction with ectoadenosine deaminase (Franco et al., 1997).

We suggest that it is unlikely that the selectivity to cholinergic neurons is artifactual. The fact that thapsigargin treatmentcould elicit similar responses in all types of cells stronglysupports our suggestion. Notably, our data also show that thedye calcium orange might be particularly useful for subsequentimmunochemistry to identify the responding cholinergic neurons.This feature of calcium orange most likely relates to its highphotostability and membrane impermeability after de-esterificationin cytoplasm (Eberhard and Erne, 1991; Thomas et al., 2000). Ourresults suggested that calcium orange retains its place withinthe neuron even after fixation with formalin as a fixative. Weobserved that calcium orange-loaded neurons could be fixed withoutapparent leak of fluorescence outside the cells, because therewas no "aura" around neurons and no increase in background after1 and 24 hr of formalin treatment. Similar observations have beenreported for another fluorescent dye, Lucifer yellow (Stewart,1978). Moreover, fixation of the slices also did not alter thefluorescence inside the cells, because the adenosine-induced increasein fluorescence after fixation was the same as that observed inreal time. Similar results were obtained in calcium orange-loadedcultured HEK 293 cells, in which cytosolic calcium fluorescenceintensity remained stable, without any leak into the medium, afterfixation with formalin (data notshown).

Calcium signaling and transcription

Calcium signals induce gene expression that may be important for long-lasting adaptations (Bading, 2000; Mattson et al., 2000;Mellström and Naranjo, 2001). Such a role for calcium is welldescribed in the nervous system, in which transient changes inintracellular calcium can produce distinct transcriptional responses(Bading et al., 1993; Ghosh and Greenberg, 1995). Calcium changesalso regulate the transcription factor NF- $kappa$ B (Dolmetsch et al.,1998). We have reported previously that adenosine treatment ofbrain slices resulted in nuclear translocation of NF- $kappa$ B in theBF, a phenomenon also observed after 3 hr of sleep deprivation(Basheer et al., 2001a). Together, these observations supportthe idea that increased levels of extracellular adenosine (aspresent with sleep deprivation) may preferentially activate thePLC pathway to mobilize internal calcium, then activate PKC, whichis shown to induce nuclear translocation of NF- $kappa$ B in lymphocytes(Nishizuka, 1992; Finco and Baldwin, 1995).

A link between sleep deprivation-induced adenosine increase and NF- $kappa$ B activation

The behavioral significance of these results may be best understood in the context of sleep deprivation and its long-termeffects. Our previous reports showed a unique pattern of sleepdeprivation-induced increases in extracellular adenosine as wellas its effect on A₁ adenosine receptor activation of transcriptionfactor NF- $kappa$ B in the BF (Porkka-Heiskanen et al., 1997, 2000; Basheeret al., 2000, 2001a). One of the questions generated from thosestudies was the identity of the signal transduction pathway linkingthe increased levels of extracellular adenosine with the PKC-dependentinduction of NF- $kappa$ B (Finco and Baldwin, 1995). Our results haveprovided evidence that adenosine can mobilize IP₃-regulated intracellularcalcium, which may help the activation of NF- $kappa$ B. NF- $kappa$ B, in turn,may be involved in the expression of genes, including that ofthe A₁ receptor, which is upregulated with sleep deprivation (Basheeret al., 2001b) and which may play a role in mediating the longer-termeffects of sleepdeprivation.

Finally, we believe that these observations help in understanding the complex organization of the BF by providing a biochemicaldistinction for a major subgroup of cholinergic neurons; theseneurons may play a specific role in mediating some of the longer-termeffects of sleep deprivation-induced adenosine in theBF.

  FOOTNOTES

Received March 25, 2002; revised May 30, 2002; accepted June 3, 2002.

This work was supported by National Institute of Mental Health Grant MH 39683 and awards from the Veterans Administrationto R.W.M. and from the Sleep Medicine Education Research Foundationto R.B. We thank Dr. Aldebaran M. Hofer for providing HEK 293cells and helpful suggestions and Dr. Matthew Palmer for designingthe slicechamber.

Correspondence should be addressed to Dr. Robert W. McCarley, Harvard Medical School and Boston Veterans Affairs HealthCareSystem, Psychiatry, 116A, 940 Belmont Street, Brockton, MA 02301.E-mail: Robert_mccarley{at}hms.harvard.edu.

  REFERENCES

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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