Adenosine A1 Receptors Reduce Release from Excitatory But Not Inhibitory Synaptic Inputs onto Lateral Horn Neurons

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The Journal of Neuroscience, August 15, 2001, 21(16):6308-6320

Adenosine A1 Receptors Reduce Release from Excitatory But Not Inhibitory Synaptic Inputs onto Lateral Horn Neurons
Susan A. Deuchars, Ruth E. Brooke, and Jim Deuchars
School of Biomedical Sciences, University of Leeds, Leeds, LS2 9NQ, United Kingdom

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Although adenosine is an important neuromodulator in the CNS, its role in modulating sympathetic outflow at the level of thespinal cord has not been studied. Because very little is knownabout adenosine A1 receptors (A1Rs) in the spinal cord, we determinedtheir location and role with particular reference to the controlof sympathetic preganglionic activity and interneuronal activityin the rat. High levels of immunoreactivity for A1Rs were observedthroughout the spinal cord. Immunostaining was dense in the intermediolateralcell column (IML) and intercalated nucleus, regions containingretrogradely labeled sympathetic preganglionic neurons (SPNs).Electron microscopy revealed A1R immunoreactivity (A1R-IR) withinpresynaptic terminals and (to a lesser extent) postsynaptic structuresin the IML, as well as the luminal membrane of endothelial cellslining capillaries. Using double-labeling techniques, some presynapticterminals were observed to synapse onto SPNs. To investigate theeffects of activating these A1Rs, visualized whole-cell patch-clamprecordings were made from electrophysiologically and morphologicallyidentified SPNs and interneurons. Applications of the A1R agonistcyclopentyladenosine (CPA) reduced the amplitude of EPSPs elicitedby stimulation of the lateral funiculus, an effect blocked bythe A1R antagonist 8-cyclopentyl-1,3-dipropylxanthine. These effectswere attributable to adenosine acting at a presynaptic site becauseCPA application increased the paired-pulse ratio. CPA did notaffect evoked IPSPs. These data show that activating A1Rs reducesfast excitatory, but not inhibitory, transmission onto SPNs andinterneurons in the IML and that A1Rs may play a protective roleon neurons involved in the control of sympatheticoutflow.

Key words: sympathetic; adenosine A1 receptors; blood vessel; excitatory amino acid transmission; spinal cord; electron microscopy

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Adenosine, generated partly by the extracellular catabolism of ATP through the ectonucleotidase cascade (Lee et al., 1981;Cunha et al., 1992), is an important neuromodulator in the CNS,acting on G-protein-linked cell surface receptors classified asA1, A2, and A3. A major role for adenosine acting at A1 receptors(A1Rs) may be neuroprotective because release of adenosine duringhypoxic or ischemic episodes inhibits neurotransmission to counteractpossible excitotoxicity (Fowler, 1989; Rudolphi et al., 1992;Katchman and Hershkowitz, 1993). On A1Rs, adenosine exerts itsaction presynaptically and postsynaptically to elicit mainly inhibitoryeffects. Presynaptic A1Rs reduce neurotransmitter release viaactivation of G-proteins that inhibit adenylate cyclase activity(Stiles, 1992). A1R-mediated reductions in release of both glutamateand GABA have been reported in the hypothalamus, substantia nigrareticulata, and the periaqueductal gray regions (Shen and Johnson,1997; Bagley et al., 1999; Oliet and Poulain, 1999). However,in the hippocampus, although depression of EPSCs during hypoxiawas elicited by A1R activation, depression of IPSCs was attributableto another mechanism (Katchman and Hershkowitz, 1993). PostsynapticA1Rs seem to be pharmacologically identical to those located presynaptically(Thompson et al., 1992), and activation causes hyperpolarizationparticularly through opening of potassium channels (Trussell andJackson, 1987; Gerber et al., 1989).

Because adenosine acting on A1Rs may play a crucial role in neuroprotection during stressful events, it seems important toknow its exact role in areas of the CNS involved in autonomicfunctions. Studies indicate roles for the A1Rs in synaptic transmissionin the brainstem (Thomas and Spyer, 1999), but little is knownof the spinal cord. Ligand binding studies using radioactive A1-selectiveagonists pinpointed intense binding in the dorsal and ventralhorn of the lumbar spinal cord (Goodman and Synder, 1982; Geigeret al., 1984; Choca et al., 1987). Moreover, hybridization studieslocalizing mRNA for the A1Rs showed concentrated labeling in ventralhorn neurons and moderate hybridization throughout the spinalgray matter, although the white matter was unlabeled (Reppertet al., 1991). However, little mention is made of regions involvedin sympathetic control, such as the intermediolateral cell column(IML).

Despite a lack of evidence for A1R localization in the IML, there is a sign that A1Rs play a role in determining sympatheticoutflow. Intrathecal injections of an A1R agonist decreased bloodpressure and heart rate, although it was not determined whetherthis was a result of sympathoinhibition (Koh et al., 1996). Furthermore,such intrathecal applications cannot pinpoint sites of actionof drugs that may include receptors on blood vessels, as wellas those located presynaptically and postsynaptically onneurons.

We therefore studied the localization of the A1Rs at the light and electron microscopic level using immunohistochemistry,concentrating on thoracic spinal cord, which contains neuronsinvolved in cardiovascular control. When these studies revealeda striking density of A1Rs in the IML and extensive vascular andneuronal localization in the spinal cord, electrophysiologicalexperiments were performed to examine the role of A1Rs in modulatingthe activity of neurons contributing to sympatheticoutflow.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Immunohistochemistry. Male rats (150-200 gm; n = 10) were deeply anesthetized by intraperitoneal Sagatal (60 mg/kg) and transcardiallyperfused with fixative containing 4% paraformaldehyde and 0.1-0.5%glutaraldehyde in 0.1 M phosphate buffer (PB), pH 7.4. All experimentswere performed under a UK Home Office License and in accordancewith the regulations of the UK Animals (Scientific Procedures)Act of 1986. Efforts were made to minimize animal suffering andto use only the minimum number of animals required. Spinal cordswere removed at the thoracic level and post-fixed in perfusingfixative for 4 hr. The tissue was then cut into ~1 cm sections,embedded in gelatin (10%), fixed (0.5% glutaraldehyde), sectionedat 50 µm on a vibrating microtome (Leica, Nussloch, Germany),and collected into PBS, pH 7.2. For electron microscopy, sectionswere cryoprotected by incubation in 10% sucrose in 0.1 M PB for10 min, followed by 20% sucrose in 0.1 M PB for 20 min and thenfreeze-thawed twice in liquid nitrogen to permeabilize the membranes.For light microscopy, the tissue was permeabilized using 0.1%Triton X-100 included with the primary antibodysolution.

Sections were immersed in primary antibody in PBS for 12-48 hr at 4°C.We used various primary antisera directed against differentparts of the A1Rs so that similar patterns of labeling would indicatespecific localization of the receptor. The antiserum used forthe majority of the labeling in this study was raised in rabbitagainst a unique intracellular sequence of the rat A1R, residues310-323, and was diluted 1:200-1:400. This antibody has been shownpreviously to specifically recognize the adenosine A1 receptorin Xenopus oocytes expressing the A1 receptor but not in untransfectedcells, as well as in rat CNS by Western blotting (Smith et al.,2001). Another antibody raised in rabbit against a similar sequence(amino acids 304-326; 1:100; Sigma, Poole, UK) has been reportedpreviously to specifically recognize the A1 receptor by Westernblotting in human brain and in Chinese hamster ovary cells stablyexpressing the A1 receptor but not in untransfected cells (Schindleret al., 2001). A primary antibody raised in goat against a peptidemapping near the C terminus of the adenosine A1 receptor was dilutedat 1:200-1:800 (Santa Cruz Biotechnology, Santa Cruz, CA). Finally,another antibody raised in rabbit and generated against an extracellularsequence of the A1R (amino acids 163-176; Affinity BioReagents,Exeter, UK) was used at a dilution of 1:200. The specificity ofthis antibody to the A1 receptor has been shown by Western blottingin the CNS, as well as in A1 receptor-transfected Xenopus oocytes(Smith et al., 2001). For additional controls, sections were incubatedwith PBS in place of primary antiserum or with the goat primaryantiserum that had been preabsorbed with the peptide antigen for1 hr before use (1 µg of peptide for 1 µg ofantibody).

For light and electron microscopy, sections were washed three times for 10 min each in PBS, placed into biotinylated secondaryantibodies to rabbit IgG or goat IgG as appropriate, diluted 1:200in PBS (Vector Laboratories, Peterborough, UK) for 5 hr at 4°C,washed three times for 10 min each in PBS, and then put into VectastainElite ABC reagent (Vector Laboratories) for 18-20 hr at 4°C. Thesesections were then washed in Tris HCl buffer, pH7.4, and incubatedin diaminobenzidine (DAB) solution (5 mg in 10 ml of Tris bufferwith 0.01% H₂O₂) for 10 min. Some sections were put on subbedslides for light microscopy only. Other sections were washed in0.1 M PB for 10 min and post-fixed in 0.5% osmium tetroxide (in0.1 M PB) for 45 min. After washing in 0.1 M PB, the sectionswere then dehydrated through a series of ethanols, followed bytwo 10 min washes in propylene oxide (Fisher Scientific, Loughborough,UK). The sections were then immersed in Durcupan ACM resin (Fluka,Neu-Ulm, Germany) for 12-20 hr, mounted on glass slides, and placedin an oven at 60°C for 48 hr to polymerize the resin. Slides weresubsequently examined at the light microscope level, and imageswere obtained via an integrating analog CCD camera (JVC KYF 55B)attached to an Acquis image capture system (Synoptics, Cambridge,UK) and adjusted for brightness-contrast-intensity and color balanceusing Corel PhotoPaint 9 beforeprinting.

When areas with suitable staining for electron microscopy were selected, the coverslip was removed, and the relevant areawas cut out and glued to the flat surface of a resin block. Aftertrimming of the block, serial ultrathin sections (70 nm) werecut using a Leica Ultra Cut S ultramicrotome and collected onFormvar-coated 1 mm slot grids. The sections were then stainedwith lead citrate before viewing on a Phillips CM10 transmissionelectron microscope. Negatives were digitized using an Umax Astra2200 scanner and manipulated in Corel Draw9.

For fluorescence light microscopy, sections incubated in rabbit primary antibody were detected by incubation for 4 hr in Cy3-conjugateddonkey anti-rabbit IgG (1:1000; Stratech, Luton, UK). Goat primaryantibodies were detected by biotinylated anti-goat (1:200; VectorLaboratories), followed by streptavidin-Alexa⁴⁸⁸ (1:1000; Molecular Probes, Rijnsburger-Weg, The Netherlands).Sections were dried onto gelatinized slides at 4°C, covered withVectamount (Vector Laboratories), and stored at 4°C. Cy3 was visualizedwith a custom Cy3 filter set and Alexa⁴⁸⁸ with a standard FITC filter set, and digital images were acquiredasabove.

Retrograde labeling of sympathetic preganglionic neurons and immunohistochemistry. To retrogradely label the complete populationof sympathetic preganglionic neurons (SPNs), male rats (150 gm;n = 3) were injected intraperitoneally with 0.1 ml of 1% Fluorogold(Fluorochrome Inc., Englewood, NJ) 7 d before immunohistochemistry.The rats were then deeply anesthetized with pentobarbitone sodium(60 mg/kg, i.p.) and perfused transcardially with 0.9% NaCl, followedby fixative containing 4% paraformaldehyde. Sections were washedin PBS, and the A1R immunostaining was performed for fluorescencedetection as described above. Fluorogold was visualized with UVillumination and immunostaining with either Cy3 or FITC filtersasappropriate.

SPNs with defined ganglionic projections were retrogradely labeled from the superior cervical ganglion (n = 5) or the adrenalgland (n = 3) in 150-200 gm rats under halothane anesthesia (5%in O₂) by the injection of 5-10 µl of 1% cholera toxin B chain(CTB) (List Biologic, Campbell, CA) in saline. After 3-7 d ofrecovery, the rats were anesthetized with intraperitoneal Sagatal(60 mg/kg) and perfused transcardially with 4% paraformaldehydeand 0.025-0.1% glutaraldehyde as described above. Sections werecut on the vibrating microtome at 50 µm and freeze-thawed in liquidnitrogen as described above. Retrogradely transported CTB wasdetected before the A1R immunohistochemistry in two ways, bothrequiring incubation in goat anti-CTB (1:10,000; List Biologic)for 12-24 hr at 4°C. One approach was a preembedding gold procedureperformed on tissue that had been perfused with low glutaraldehydeto facilitate penetration of gold particles into the tissue. Sectionswere transferred from primary antibody into secondary antibodiesrecognizing goat IgG conjugated to 1 nm gold particles (AmershamPharmacia Biotech, Little Chalfont, UK) diluted 1:200 in pH 7.6Tris-HCl buffer containing 1% fish gelatin and 1% goat serum for18-20 hr at 4°C. After thoroughly rinsing the sections (four timesfor 10 min each) in PBS, fixing in 2% glutaraldehyde in 0.1 MPB for 2 min, and washing in distilled deionized water (four timesfor 10 min each), the gold particles were silver enhanced for5-10 min using an IntenSE silver enhancement kit (Amersham PharmaciaBiotech). The other method used biotinylated anti-goat IgG afterprimary antibody incubations, detected with Vector ABC kit (VectorLaboratories), and visualized with the tetramethylbenzidine (TMB),pH6.0, method (Marfurt et al., 1988) to provide a crystallinereaction product. In both cases, sections were then incubatedin a rabbit primary antibody against the A1R, which was visualizedusing the DAB method described above. Sections were then osmicatedand processed for light and electron microscopy as describedabove.

Electrophysiology. Rats aged 10-15 d were anesthetized with urethane (2 gm/kg, i.p.). The thoracic spinal cord was exposed,and the dorsal and ventral roots were cut to isolate the cord.The upper and middle thoracic spinal cord was removed and submergedin ice-cold sucrose artificial CSF (aCSF) containing (in mM):217 sucrose, 26 NaHCO₃, 3 KCl, 2 MgSO₄, 2.5 NaH₂PO₄, 1 CaCl₂,and 10 glucose (equilibrated with 95%O₂-5%CO₂). The dorsal andventral roots were cut, and the dura mater was removed. The piamater was carefully teased away from the spinal cord, and theclean spinal cord was immersed in warm agar that was placed onice for rapid setting. Slices (250 µm thick) of the embedded spinalcord were cut on a Vibroslice and placed into the recording chamberor a holding chamber for later use. The sections were submergedin aCSF (in mM: 124 NaCl, 26 NaHCO₃, 3 KCl, 2 MgSO₄, 2.5 NaH₂PO₄,2 CaCl₂, and 10 glucose) and superfused at a rate of 3-5 ml/min.All experiments were performed at room temperature. A visualizedpatch-clamp recording set-up was used with an upright microscope(BX50WI; Olympus Optical, Tokyo, Japan). The IML was located at10× magnification, and the cells were visualized at 60× magnificationfor recording. Both SPNs and interneurons within and around theIML were targeted for these experiments, identified both electrophysiologicallyand anatomically (at the end ofrecording).

Whole-cell patch-clamp recordings were obtained from neurons after achieving tight (>5 G $Omega$ ) resistance seals. Recordings weremade in current-clamp mode using an Axopatch 1D (Axon Instruments,Foster City, CA). Patch electrodes (tip diameter of 3 µm; resistanceof 4-6 M $Omega$ ) were filled with (in mM): 130 K-gluconate, 10 KCl,11 EGTA, 2 MgCl₂, 1 CaCl₂, 10 HEPES, 5 Na₂ATP, and 0.3 Na₂GTP,pH 7.2 (295 mOsm). Neurobiotin (0.5%) was included in the patchsolution and diffused into the neuron during recording. For someexperiments, the filling solution was composed of (in mM): 110Cs₂SO₄, 0.5 CaCl₂, 2 MgCl₂, 5 EGTA, 5 HEPES, 5 tetraethylammonium(TEA), and 5 Na₂ATP.

Neurons were first characterized by applying hyperpolarizing and depolarizing current pulses (1 sec duration). Hyperpolarizingcurrent pulses ( $-$ 10 to $-$ 150 pA) produced voltage responses thatwere characteristically different for the two types of neuronstudied. The input resistance of the neuron could also be calculatedfrom the response to a hyperpolarizing current pulse. Depolarizingcurrent pulses brought the neurons to threshold for firing, andthe shapes of the action potentials were examined to further differentiatetheneurons.

The lateral funiculus (lf), which contains the descending fibers originating in the areas of the brainstem involved in sympatheticcontrol, was stimulated using a bipolar stimulating electrodeplaced just below the surface of the slice. The lf was stimulatedat two times the threshold for response using an isolated stimulator(model DS2A; Digitimer, Hertfordshire, UK). Single-pulse stimulationwas used except for the series of experiments looking at paired-pulseratios when a second stimulus was applied 100-300 msec after thefirst. The response in control solution was always an EPSP, buton blocking this EPSP with selective antagonists, an IPSP couldalso be obtained at more depolarized potentials using the samestimulation parameters. The input resistance of the neuron wasalso tested just before, during, and after application ofdrugs.

Drugs were applied in the superfusing solution at a rate of 3-5 ml/min, and the concentration given is the final concentrationin the bath. Drugs used were the A1R agonist cyclopentyladenosine(CPA) and the A1R antagonists 8-cyclopentyl-1,3-dipropylxanthine(DPCPX) (dissolved in dimethylsulfoxide) and 8-cyclopentyl-1,3-dimethylxanthine(CPT) (dissolved in 0.1N NaOH). To block the EPSPs, the excitatoryamino acid antagonists 6,7-dinitroquinoxaline-2,3(1H,4H)-dione(DNQX) (dissolved in 0.1N NaOH) or 1,2,3,4-tetrahydro-6-nitro-2,3-dioxobenzo[f]quinoxaline-7-sulfonamidedisodium (NBQX), and D( $-$ )-2-amino-5-phosphopentanoic acid (AP-5)were applied. To block synaptic activity, tetrodotoxin (TTX),DNQX, AP-5, strychnine, and bicuculline were applied. All drugswere obtained from Sigma/RBI (Poole, UK) and dissolved in waterunless otherwisestated.

Data analysis. The voltage responses to current pulses were plotted to reveal the presence of any currents specific to eithertype of neuron. The action potential duration, amplitude, andafterhyperpolarization (AHP) were measured for each neuron becauseinterneurons display action potentials of significantly shorterdurations and smaller AHPs (S. Deuchars et al., 2000).

The EPSP (and IPSP) amplitude was measured as the peak change from the holding potential and averaged over 10-20 consecutivesweeps for control and drug responses. Plotting the drug responseas a mean percentage of the control response in each case showedthe effects of the drugs on the EPSP. The effects of the drugswere tested statistically using the paired Student's t test, anddifferences were considered significant when p < 0.05. Any effectsof the drugs on resting potential and input resistance were alsonoted. The responses of a neuron to paired-pulse stimulation ofthe lf were given as the ratio of the second response to the firstresponse. Paired-pulse ratios were then calculated in controlmedium and in CPA and compared to determine whether there wasa significantchange.

Histology. After recordings of up to 4 hr, electrodes were very slowly removed from neurons, and the slice was immersed infixative containing 0.5% glutaraldehyde-4% paraformaldehyde forup to 18 hr. Slices were embedded in gelatin and immersed in thesame fixative. Sections (50 µm thick) were cut on a vibratingmicrotome, freeze-thawed twice by immersing in liquid nitrogen,and incubated in extravidin-peroxidase (1:250; Sigma) for 24-48hr, which was then visualized with DAB (Sigma). Sections werethen processed for light microscopy or for light and electronmicroscopy as described previously (Deuchars and Thomson, 1995)and reconstructed using a drawing tube attached to a light microscope.This allowed anatomical confirmation of the type of neuronrecorded.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Immunohistochemistry

Specificity of antibodies
The specificity of many of the antibodies has been reported previously (see Materials and Methods) (Schindler et al., 2001;Smith et al., 2001). In addition, no staining was observed incontrol sections that had no primary antibody present or in whichthe primary antibody was preadsorbed against the control peptide(only available with the goat antibody from Santa Cruz Biotechnology),indicating that the antibodies recognized the appropriate sequencein the tissue. Furthermore, the pattern of immunostaining wasidentical with all antibodies tested (Figs. 1, 2) and was alsoconsistent with previous reports of A1 receptor localization usingin situ hybridization (Reppert et al., 1991) or autoradiography(Goodman and Synder, 1982; Geiger et al., 1984; Choca et al.,1987), and so we are confident that our procedures specificallylocalized the adenosine A1 receptor.

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Figure 1. Adenosine A1 receptor immunoreactivity in the thoracic spinal cord. A, Low magnification of staining obtained with the A1 receptor antibody raised in rabbit (gift from Dr. Mike Yates, Leeds University) in the thoracic spinal cord. Immunoreactivity was visualized with diaminobenzidine. Labeling was observed throughout the spinal cord. Even at low magnification, the IML is clearly seen as heavily stained. Staining is also dense around the central canal (CC), the dorsal horn (DH), and the ventral horn (VH). B, Low magnification of staining obtained with the A1 receptor antibody raised in goat (Santa Cruz Biotechnology), prepared identically to the material in A, except for the primary antibody. Note that the pattern of staining is almost identical, with the IML and ventral horn being particularly prominent. C, High magnification of the IML. Staining was a compact collection of punctate structures covering the IML adjacent to the white matter (WM). The arrow indicates one such punctate structure. D, In the vicinity of the central canal, labeling could be observed in the somata and dendrites of neurons (arrows), as well as presumptive fibers. E, In the dorsal horn, staining of fibers was dense in lamina II, and labeled neuronal somata could also be observed in laminas II and III (arrows). F, In the ventral horn, labeled fibers, somata, and dendrites of large neurons (arrow) were observed.

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Figure 2. Fluorescence images indicating that adenosine A1 receptor immunoreactivity in the IML is dense in the region of retrogradely labeled SPNs. A, Low magnification of adenosine A1R-IR detected with the antibody raised in goat and visualized with Alexa⁴⁸⁸ viewed through a FITC filter set. The IML contains dense labeling and so stands out from surrounding structures. The boxed area surrounding the IML is shown at higher magnification in B. B, Higher magnification of the boxed area in A. At this magnification, it is clear that the staining in the IML has a punctate appearance. C, SPNs retrogradely labeled in the IML by an intraperitoneal injection of Fluorogold and visualized by UV illumination in a coronal section. SPNs appear blue-white under these conditions and contain Fluorogold in cell bodies and dendrites. The same section is shown in D. D, A1R-IR in the same section as C, detected with Cy3-conjugated secondary antibodies and viewed through a Cy3 filter set so that immunoreactivity for the adenosine A1R appears red. The A1R-IR makes the IML stand out as brighter red than the surrounding neuropil, and this bright staining persists into the lateral funiculus. E, SPNs retrogradely labeled in the IML by an intraperitoneal injection of Fluorogold and visualized by UV illumination in a longitudinal section. The same section is shown in F. F, A1R-IR in the same area of the section as E but viewed through a Cy3 filter set so that immunoreactivity for the adenosine A1 receptor appears red. The A1 immunoreactivity runs in fibers along the IML (arrows).

Light microscopy
Adenosine A1 receptor immunostaining was observed throughout the spinal cord (Fig. 1). In the ventral horn, strong stainingwas apparent in somata of presumptive motor neurons, as well asfibers (Fig. 1A,B,F). In the dorsal horn, staining was strongestin lamina II in both fibers and cell bodies (Fig. 1A,B,E). Labeledneurons and fibers were also apparent in the vicinity of the centralcanal (Figs. 1A,B,D). The IML was evident even at low magnificationsas a region of dense staining (Figs. 1A,B, 2A). The predominantstaining was punctate in nature (Figs. 1C, 2B). When SPNs wereretrogradely labeled by intraperitoneal injections of Fluorogold,then this dense region of A1R-IR precisely overlaid the retrogradelylabeled SPNs (Fig. 2C-F). In longitudinal sections, the labeledfibers appeared to run in a ladder-like pattern similar to thatdescribed for the distribution of SPNs (Petras and Cummings, 1972)and to follow the spread of SPNs at the rungs of theladder.

Electron microscopy
Ultrastructural examination of the IML always revealed A1R-IR highly targeted to the luminal membrane of endothelial cellsof blood vessels (Fig. 3A), in myelinated fibers in the lateralfuniculus (n = 30) (Fig. 3C) and in presynaptic terminals (n =100) onto dendritic shafts (n = 85) (Fig. 3B,E,F), spines (n =1), and somata (n = 2) (Fig. 4E). In accordance with the receptorsbeing incorporated into the membrane, reaction product was oftenobserved adjacent to the membrane (Figs. 3B,D, 4A-C,E,F). In addition,some cytoplasmic reaction product was observed (Fig. 4D), presumablyreflecting A1Rs that are being trafficked to the membrane or havebeen internalized during agonist induced desensitization (Sauraet al., 1998). Some postsynaptic targets of A1R-IR terminals wereidentified as SPNs by the presence of crystalline reaction productwhen retrogradely transported CTB was visualized with TMB (n =30) (Fig. 3E,F). In other cases, SPNs were identified by the presenceof silver intensified gold particles when CTB was localized withthe preembedding immunogold approach (n = 30) (Fig. 4A-F). Inthese cases, the labeled structures were followed in serial sectionsto verify the presence of several gold particles and so confirmthat labeling was specific (Fig. 4A,B). Where A1R-immunoreactiveterminals synapsed onto unlabeled postsynaptic structures, itwas impossible to say whether the postsynaptic cell is an interneuronor part of an SPN in which there is no reaction product; however,the electrophysiological experiments do suggest that interneuronsare also likely targets of these A1R-immunoreactive terminals(see below). A1R-IR was also detected in the soma of retrogradelylabeled SPNs in which it was associated with endoplasmic reticulumbut not with the synaptic specialization (Fig. 4E).

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Figure 3. Electron microscopic localization of the adenosine A1R-IR in the IML. A, A capillary in which A1R-IR is highly targeted to the luminal membrane of endothelial cells of blood vessels (arrows). B, A presynaptic terminal in the IML containing immunoreactivity for the A1R adjacent to the membrane (broken arrow indicates immunoreaction product). This terminal forms an asymmetric-type synaptic contact (arrow) with a dendritic structure. C, A1R-IR (broken arrows) was detected in numerous myelinated fibers in the lateral funiculus. D, A presynaptic terminal in the IML containing A1R-IR adjacent to the membrane (broken arrow indicates immunoreaction product). This terminal forms an asymmetric-type synaptic contact (arrows) with a dendritic structure (den). E, F, A1R-IR terminals formed synaptic contacts (arrows) with structures identified as SPN dendrites (SPN den) by the presence of crystalline reaction product (arrows) as a result of retrograde labeling with cholera toxin B chain, which was visualized with the TMB method. Note that the A1R-IR (broken arrows) is adjacent to the plasma membrane but some distance from the synaptic face. UT, unlabeled terminal.

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Figure 4. Adenosine A1R-IR terminals form synaptic contacts with structures identified as SPNs by retrograde labeling. A, An A1R-IR terminal (broken arrow) forms an asymmetric-type synaptic contact (arrow) with a dendritic structure that contains silver-intensified gold particles (open arrows), indicating that it is a retrogradely labeled structure. The same terminal is shown in B. Note that the reaction product is adjacent to the membrane of the terminal but some distance from the active zone. B, The same terminal shown in A but serially several sections on, confirming that the dendrite is retrogradely labeled. The section has been tilted slightly with the goniometer to visualize the synaptic specialization. The silver grains in this section (open arrows) are spatially separate to those in A, indicating that these are different particles and not the result of intensification of the initial gold particles throughout the dendrite. C, D, F, Synaptic terminals (A1R-IR) containing A1 receptor immunoreactivity form synaptic contacts (arrows) with dendrites identified as retrogradely labeled SPNs by the silver-intensified gold particles (open arrows). Immunoreactivity is both adjacent to the membrane of labeled terminals (C, F) and within the cytoplasm (D). E, An A1R-IR terminal forms a synaptic contact (arrow) with the soma of an SPN. The soma contains not only silver-intensified gold particles (open arrows) but also A1R-IR associated with the endoplasmic reticulum (broken arrow).

Electrophysiology

These studies were performed on both SPNs and interneurons within the IML of the thoracic spinal cord because it is likelythat both of these neurons could be targeted by synapses containingadenosine A1 receptors. The two groups of neurons were distinguishedby their very different electrophysiological and morphologicalcharacteristics. From the voltage responses to hyperpolarizingcurrent pulses, it was noted that SPNs showed a delayed returnto the holding potential at the end of a current pulse, indicativeof activation of an I_A (Fig. 5A). In contrast, interneurons withinthe IML are characterized by a sag in the voltage response toa hyperpolarizing current pulse, suggesting activation of an I_H(Fig. 5B). The interneuronal action potentials are significantlyshorter in duration than those of SPNs (Fig. 5C) and have a complexbut smaller afterhyperpolarization. Neurons were filled with Neurobiotinduring the recording procedure, and 10 interneurons and nine SPNscould be recovered and reconstructed at the end of the experiment.SPNs had axons that coursed ventrally straight out of the IMLto the ventral horn in which they exited. Interneuronal axonalarborization, in contrast, was extensive, and the axons coursedboth dorsally and ventrally and showed varicosities within theIML, which could be attributable to sites of synaptic contact.Because identification of the SPNs and interneurons was easilydetermined from electrophysiology and could be confirmed withanatomy, the responses of both types of neurons to applicationsof A1R agonists and antagonists therefore could be compared.

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Figure 5. CPA reduces the amplitude of EPSPs elicited in both SPNs and interneurons. A, On the left are the voltage responses of an SPN to hyperpolarizing (averages of 3 sweeps) and depolarizing (single sweep) current pulses. The traces show a delayed return to resting potential at the end of the hyperpolarizing current pulses, indicative of activation of an I_A (arrow). The action potential duration was 7.2 msec, and the afterhyperpolarization was quite simple with two components. On the right are average traces (of 10 sweeps) of the EPSP elicited by lf stimulation in control solution, CPA (100 nM), and then after switching back to standard aCSF. The EPSP amplitude was decreased by CPA application. B, The left shows the voltage responses of an interneuron to the same hyperpolarizing (averages of 3 sweeps) and depolarizing (single sweep) current pulses. At hyperpolarized potentials, a sag in the voltage response was observed, suggesting that an I_H was activated. The action potential duration was 3.2 msec, and the AHP shows a distinct fast and slower phase. On the right are average traces (of 10 sweeps) of the EPSP elicited in the interneuron by lf stimulation. The EPSP amplitudes in control aCSF are not significantly different from those elicited in the SPN. In addition, the effects of CPA on the interneuronal EPSP are similar to those observed in the SPN. C, Comparisons of the duration of the interneuronal and SPN action potentials. D, Pooled data showing that the effects of CPA on the EPSPs elicited in SPNs are not significantly different from those in interneurons.

The A1R agonist CPA decreased the EPSPs elicited by lateral funiculus stimulation in both SPNs and interneurons
We chose to stimulate the lateral funiculus because this contains descending axons from areas of the brainstem that make monosynapticconnections onto SPNs, whereas dorsal horn input onto SPNs ispolysynaptic and thus more difficult to analyze (Dembowsky etal., 1985). Lateral funiculus stimulation elicited responses inall SPNs and interneurons tested. These consisted of a fast EPSPin control solution, which occurred at a constant latency andcould follow high-frequency stimulation (up to 50 Hz). These EPSPswere therefore considered to be of a monosynaptic nature and werenot significantly different in amplitude or latency for the twogroups of neurons. These EPSPs could be abolished by applicationsof the excitatory amino acid receptor antagonists CNQX (20 µM)or NBQX (20 µM) and AP-5 (50 µM), showing that these responsesare elicited by release of glutamate (n = 6) (Fig. 6C). This wasexpected because, in previous work, stimulation of the rostralventrolateral medulla (RVLM) elicited monosynaptic EPSPs in SPNsthat were mediated by activation of the excitatory amino acidreceptors, indicating that glutamate is the major neurotransmitterin this pathway (Deuchars et al., 1995). The effects of bath applicationsof 100 nM CPA, which is selective for A1Rs, were determined onboth SPNs and interneurons. CPA decreased the amplitude of theEPSP elicited in all SPNs tested from 10.5 ± 1.2 (mean ± SEM)to 5.6 ± 0.7 mV, a decrease of 44.5 ± 5% (n = 13; measured at $-$ 70 mV) (Fig. 5A,D). The effect of this drug on the EPSPs elicitedin interneurons was almost identical with CPA decreasing the amplitudeof these EPSPs from 9.0 ± 0.9 to 5.3 ± 0.8 mV, a decrease of 44.1± 4.5% (n = 11) (Fig. 5B,D). Not surprisingly, these decreasesin amplitude were not significantly different for the two groupsof neurons, and so all neurons were considered together for therest of the analysis. When CPA application ceased, the drug washedoff slowly, and the EPSP amplitude returned to near control values(Fig. 6).

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Figure 6. Time course of action of CPA and pharmacology of the EPSP. A, Graph of the amplitude of the EPSP elicited by lf stimulation in an SPN over time with sample EPSPs shown at the top for each of the conditions (average of 10 consecutive sweeps). It can be clearly seen that CPA application caused a decrease in EPSP amplitude that slowly recovered as the CPA was washed off. B, Pooled data from 26 neurons showing the effect of CPA on EPSP amplitude and input resistance. CPA caused a significant decrease in EPSP amplitude but had no significant effect on input resistance. C, In another SPN, the EPSP was abolished by application of the excitatory amino acid receptor antagonists CNQX (20 µM) and AP-5 (50 µM), indicating that the EPSP is mediated by activation of these receptors postsynaptically.

The effects of CPA could be antagonized by the A1R antagonist DPCPX
The A1R antagonist DPCPX (200-500 nM) was applied to neurons to selectively block the reduction observed with CPA. DPCPX wasfirst applied during application of CPA in which the EPSPs hadbeen reduced from 9.1 ± 1.3 to 5.8 ± 1.1 mV, a decrease of 39.4± 6.0% (n = 9). DPCPX antagonized the effects of CPA, and theEPSP amplitude returned to 8.8 ± 1.0 mV without effect on holdingpotential or input resistance (Fig. 7).

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Figure 7. DPCPX antagonized the effects of CPA. A, Graph of the EPSP amplitude elicited by lf stimulation against time in an interneuron with traces of the EPSP above (averages of 10 sweeps). CPA (100 nM) decreased the EPSP amplitude, an effect that was antagonized by application of DPCPX (300 nM), the A1R antagonist, together with CPA. B, Pooled data showing the effect of CPA on the EPSP and the antagonism by DPCPX, which restored the EPSP to the control amplitude. Both DPCPX and CPT (10 µM), another A1R antagonist, had no effect on EPSP amplitude when applied alone.

DPCPX (500 nM) and another A1R antagonist, CPT (10 µM), were applied alone to determine whether there was an ongoing releaseof adenosine, which tonically reduced the EPSP amplitude. Neitherdrug had an effect on holding potential or the evoked EPSP inwhich the amplitude was unchanged in DPCPX [10.6 ± 1.4 to 10.5± 1.7 mV (n = 5)] and CPT [8.9 ± 0.9 to 8.6 ± 0.8 mV (n = 8)](Fig. 7B). Thus, in our recording conditions, there is no tonicallyactiveadenosine.

The effects observed with CPA are attributable to a presynaptic action
To determine the sites of the A1R mediating the effects of CPA, the relative amplitude of the synaptic response to two stimuliapplied to the lf at short intervals was determined in controlaCSF and in CPA. If a change in paired-pulse ratio is observedwith CPA, this is probably attributable to activation of A1R presynaptically,which then decreases the probability of neurotransmitterrelease.
In control solution, the paired-pulse ratio was 0.88 ± 0.11 (n = 8). Because this ratio is <1, the control response is a paired-pulsedepression in the control solution likely attributable to a highprobability of neurotransmitter release with the first stimulus,causing depletion of synaptic vesicles so that there is a smallerresponse to the second stimulus. When CPA was applied, the paired-pulseratio increased to 1.26 ± 0.15, a significant change from thecontrol ratio of 0.88 ± 0.11. Thus, there was a switch from paired-pulsedepression to paired-pulse facilitation observed with CPA (n =8) (Fig. 8A). This is because, in the presence of CPA, the firstEPSP is much smaller, as discussed above. This means that thereare more synaptic vesicles remaining in the presynaptic cleftthat can be released with the second stimulus, so paired-pulsedepression does not occur. In addition, because fewer vesicleswere released with the first stimulus, there was an elevated levelof intracellular calcium; thus, the second stimulus can releasemore vesicles and the EPSP is larger. So now we see paired-pulsefacilitation, and these data indicate a presynaptic site of actionof adenosine.

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Figure 8. Effects of CPA are attributable to a presynaptic action. A, Responses of an SPN to twin pulse stimulation of the lf (200 msec apart) in control solution showed paired-pulse depression (i.e., the response to the second pulse was smaller than the first). In CPA, the second response is the same size as the first reduced response, with the ratio now being 1:1. On the right are the pooled data showing the paired-pulse ratio increases in the presence of CPA, indicative of a presynaptic site of action for adenosine. B, Effects of applications of CPA and DPCPX plus CPA in a neuron recorded using a patch solution in which cesium sulfate is the main component. CPA decreased the EPSP amplitude without effect on the membrane potential. This reduction was antagonized by DPCPX. C, In synaptic block medium containing TTX, DNQX, AP-5, strychnine, and bicuculline, action potentials and the response to lf stimulation were blocked. Hyperpolarizing current pulses were then applied to check input resistance, and CPA was applied. There was no change in membrane potential or input resistance with application of CPA in this recording medium.

In addition, experiments were performed using a patch pipette solution with the main component being cesium sulfate. TEA,the potassium channel blocker, was also included in the solution.Inclusion of these two nonselective potassium channel-blockingagents in the patch solution has been shown to dramatically reducepostsynaptic effects of adenosine attributable to opening of potassiumchannels (Li and Perl, 1994). Under these recording conditions,the effects of CPA on the EPSP amplitude were identical to thoseobserved previously, i.e., a decrease in amplitude of the evokedEPSP from 8.9 ± 1.5 to 4.8 ± 1.0 mV, a decrease of 42.9 ± 12%(n = 5) (Fig. 8B). In addition, DPCPX also antagonized these effectsof CPA (n = 3) (Fig. 8B). This suggests that the effects observedwere not attributable to a change in postsynaptic potassiumcurrents.
CPA had no significant effect on the input resistance of the neurons, measured as the change in voltage to a hyperpolarizingcurrent pulse at a holding potential of $-$ 70 mV (Fig. 6B). Furthermore,in these recording conditions (whole-cell current clamp), CPAdid not cause the SPNs or interneurons to hyperpolarize. To furthertest for postsynaptic sites of action, the effects of CPA on theholding potential and input resistance were also tested in synapticblock medium containing TTX (0.6 µM), DNQX (20 µM), AP-5 (50 µM),bicuculline (5 µM), and strychnine (2 µM) immediately after establishingwhole-cell configuration. In this medium, CPA had no effect onthe membrane potential or input resistance of the neurons tested(n = 6) (Fig. 8C). These data therefore indicate that, in youngrats, the major site of action of the A1Rs is presynaptic, inaccordance with the immunohistochemical localization of the A1Rsin adult tissue describedabove.

Fast IPSPs elicited by lf stimulation are not affected by applications of CPA
Stimulating the lateral funiculus activates both excitatory and inhibitory pathways that descend from the RVLM (Deuchars etal., 1997); thus, we were interested to see whether activationof A1Rs also affects inhibitory inputs onto these neurons. Incontrol conditions, the response observed with lf stimulationwas an EPSP that was always reduced in amplitude with CPA. Todetermine whether IPSPs were underlying these EPSPs, the excitatoryamino acid receptor antagonists DNQX or NBQX and AP-5 were appliedto eight neurons. In five of these neurons, an IPSP was revealed,whereas in the other three neurons, no additional postsynapticpotential was elicited. These fast IPSPs had a very short constantlatency and could follow high-frequency stimulation. In addition,the IPSP was still robust in the presence of the excitatory aminoacid antagonists that have been shown previously to block polysynapticIPSPs elicited by RVLM stimulation (Deuchars et al., 1997). Thesedata indicate that the IPSP was elicited at least in part by activationof a monosynaptic pathway. In the presence of these excitatoryamino acid antagonists, CPA had no effect on the IPSP amplitudebecause, in control conditions, the amplitude was $-$ 4.9 ± 0.7 mVand, in CPA, the amplitude was $-$ 4.9 ± 0.8 mV (Fig. 9). Thus, therewas no significant difference in the amplitudes of this fast IPSPin control and CPA solutions. On two occasions, after washoutof CPA, the GABA_A receptor antagonist bicuculline was superfusedonto the slice, which blocked the IPSP completely, whereas strychninehad no effect (data not shown). This indicates that the fast IPSPselicited by lf stimulation are attributable to activation of GABA_Areceptors. Thus, the A1 receptors are located presynapticallyon excitatory and not inhibitory fibers in the lf and have a selectiveeffect on excitatory transmission.

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Figure 9. Fast IPSPs elicited by lf stimulation are not affected by CPA. A, Reponses of an interneuron to lf stimulation in control and CPA-containing aCSF. CPA significantly reduced the EPSP amplitude. The EPSP was then antagonized by application of CNQX and AP-5 to reveal an underlying IPSP (seen here at $-$ 40 mV), which increased in amplitude as the membrane was depolarized. This IPSP was not affected by CPA application at the same concentration (100 nM) as that which reduced the EPSP. B, Pooled data from five neurons in which an IPSP was revealed. In all five cases, the IPSP was not affected by CPA, suggesting a selective site of action of the adenosine.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

These studies indicate that the A1R is located on excitatory terminals in the intermediolateral cell column that innervatesboth SPNs and interneurons. These interneurons may play a rolein sympathetic control because all interneurons in this regionhave activity correlated to sympathetic activity (Chau et al.,2000). Activation of these presynaptic A1Rs reduces release ofan excitatory amino acid (probably glutamate) from these excitatoryterminals but not of GABA from inhibitory terminals. Previousstudies on the distribution of A1Rs in the spinal cord failedto report any degree of binding in regions involved in sympatheticcontrol. Thus, our studies are extremely pertinent because thedegree of immunoreactivity observed here and the effects of theA1R agonists indicate a crucial role for adenosine in the controlof sympatheticactivity.

Another interesting observation was an abundance of A1R immunoreactivity in the luminal membrane of endothelial cells in thespinal cord. We believe that this is the first localization inboth the peripheral and central vasculature. This is also relevantto our studies because Koh et al. (1996, 1998) used an intrathecalmethod to determine the effects of A1R activation on cardiovascularvariables. Therefore, their observations may be attributable toactivation of receptors located on the blood vessels that maycause nitric oxide-dependant relaxation (Marshall, 2000), possiblyinfluencing neuronal activity. This necessitates the in vitroapproach to determine the exact role of adenosine in modulatingsynaptic transmission in the spinal cord, and our studies showclearly that activation of A1Rs reduces excitatory neurotransmitterrelease from presynaptic terminals onto SPNs andinterneurons.

Sources of adenosine

It is well established that adenosine plays an important role in modulating synaptic transmission throughout the CNS, butwhere does this adenosine come from? Adenosine may be releasedfrom vesicles within the presynaptic terminal itself or may bea result of the breakdown of ATP released from the presynapticneurons (Cunha, 2001). An additional alternative could be thatadenosine is formed from the breakdown of ATP intracellularlyduring periods of hypoxia or ischemia. In other autonomic regions,a major source of adenosine may be attributable to the extracellularmetabolism of ATP. For example, St. Lambert et al. (1997) showedin the brainstem that at least some effects of adenosine wereattributable to breakdown of ATP extracellularly but also thatthere was release of adenosine itself. Because there is very littleendogenous activation of A1Rs during our experiments, it wouldbe difficult to try and dissect out the sources of adenosine underthese recording conditions. However, because SPNs are excitedby activation of the P2X₇ receptor, whose endogenous ligand isATP (J. Deuchars et al., 2000), it is likely, in accordance withother CNS regions, that a probable source of the adenosine isfrom extracellular catabolism ofATP.

Is there a tonic effect of adenosine?

Because applications of DPCPX and CPT had no effect on EPSPs elicited by lf stimulation or resting membrane potential, basallevels of adenosine are not sufficient to activate A1Rs underour experimental conditions. Oliet and Poulain (1999) also sawno effect of CPT on EPSPs evoked with single stimuli; however,stimulating the hypothalamus with a train of stimuli caused adepression in the response over time that was CPT sensitive. Westimulated the lf with similar trains of stimuli at a rate of1 Hz (which is slow enough to prevent paired-pulse depressionoccurring); however, no reduction in EPSP amplitude was observed(S. Deuchars, unpublished observations). One possibility is thattonically released adenosine is broken down or taken up by terminalsor glial cells too fast for effects to be observed in conditionsof the experiments. This may therefore merit further investigationusing either inhibitors of adenosine metabolism or uptake, suchas in the dorsal horn (Ackley et al., 2000) in which adenosineantagonists alone also have littleeffect.

Is there a postsynaptic effect of adenosine?

At the electron microscopic level, both presynaptic and, to a lesser degree, postsynaptic A1Rs were located in the IML. However,electrophysiological data did not reveal postsynaptic A1Rs. Themajority of A1R-mediated postsynaptic effects are attributableto potassium channels opening, which causes hyperpolarization(Trussell and Jackson, 1987; Gerber et al., 1989). The potassiumreversal potential in our experiments was $-$ 96.8 mV, far removedfrom the membrane potential at which the effects of CPA were studied( $-$ 40 to $-$ 70 mV). A1R opening of potassium channels involves activationof G-proteins; thus, the whole-cell patch-clamp technique maywash out vital second messengers for observation of this postsynapticresponse. However, other reports observed postsynaptic hyperpolarizationusing similar whole-cell patch-clamp techniques (Li and Perl,1994; Herlenius and Lagercrantz, 1999). Interestingly, at theelectron microscopic level, A1Rs were associated with the endoplasmicreticulum rather than the somatic membrane, suggesting that A1Rsare synthesized in the postsynaptic neuron and then transportedto the terminals. In support of this, studies report adenosine-mediateddecreases in synaptic transmission in sympathetic ganglia (Alkadhiet al., 1984; Hogan et al., 1998). Therefore, combining our anatomicaland physiological data, it seems likely that the major effectof the A1Rs in the IML ispresynaptic.

Source of the presynaptic terminals

The location of A1Rs in myelinated axons in the lf and the fact that stimulating the lf elicited EPSPs that were reduced inamplitude by CPA suggests that the A1Rs may be located on presynapticterminals of descending fibers from higher centers. SPNs and interneuronsare innervated by direct inputs from supraspinal regions, includingthe RVLM, the A5 region of the pons, raphe nuclei, paraventricularnucleus, and lateral hypothalamus (Strack et al., 1989). In situhybridization reveals strong neuronal expression of the A1R inthe RVLM (Reppert et al., 1991), suggesting that these neuronsproduce the A1R and may transport it to their terminals in theIML.

Inhibitory transmission was not affected by activation of A1Rs

Interestingly, CPA affected EPSPs but not IPSPs, suggesting that there are no A1Rs in inhibitory terminals onto SPNs and interneurons.There is a monosynaptic inhibitory pathway from the RVLM regionof the brainstem onto SPNs (Deuchars et al., 1997) distinct fromthe excitatory bulbospinal pathway originating in that region.Thus, it is feasible that A1Rs are located exclusively on excitatoryterminals within the IML. There is evidence that A1R agonistsreduce release of inhibitory and excitatory transmitters in thehypothalamus, substantia nigra reticulata, and the periaqueductalgray regions (Shen and Johnson, 1997; Bagley et al., 1999; Olietand Poulain, 1999). However, in CA1 neurons, DPCPX failed to blockdepression of IPSCs induced by hypoxia (Katchman and Hershkowitz,1993), showing a selective site of action of adenosine similarto that observedhere.

What is the role of adenosine in the control of sympathetic outflow?

As described above, adenosine may play an important role in modulating synaptic transmission. Furthermore, adenosine actingat A1Rs has a neuroprotective role in the CNS because ischemicepisodes or hypoxia results in adenosine production, which inhibitsthe release of excitatory amino acids to prevent excitotoxicity(Fowler, 1989; Simpson et al., 1992; Katchman and Hershkowitz,1993; Sweeney, 1997).

In the autonomic nervous system, adenosine has long been known to have profound effects at the level of the end organ andwill cause vasodilatation in skeletal and cardiac muscle to increaseoxygen supply during hypoxic episodes (Marshall, 2000). In addition,there is a role for adenosine in the control of neuronal activityin areas of the brainstem crucial for cardiovascular regulation(Thomas and Spyer, 1999). However, at the level of the spinalcord, little was known about the role that it plays in the controlof neurons involved in sympathetic control. Although intrathecalstudies suggest that adenosine in the spinal cord modulates bloodpressure and heart rate (Koh et al., 1996), these may be attributableto effects at the blood vessels rather than on neuronal activity.This study therefore is the first to show the role for adenosinein the control of neurons influencing sympathetic outflow fromthe spinalcord.

In accordance with the many previous studies in the brain (see above), this study shows that activation of A1Rs reduces releaseof glutamate from presynaptic terminals in the IML without effecton inhibitory transmission. Because excessive release of glutamateis an important mechanism underlying the excitotoxic effects ofhypoxia and ischemia (Hara et al., 1993; Schroder et al., 1999)and adenosine is produced under such conditions (Rudolphi et al.,1992), our data are consistent with a neuroprotective role foradenosine in the IML. This is important because sympathetic outflowat the level of our recordings in the thoracic spinal cord ismainly to the heart and blood vessels in which abnormal activitycould lead to circulatoryproblems.

We have established that adenosine A1 receptors are located on excitatory presynaptic terminals innervating neurons in theIML involved in controlling sympathetic outflow. Activation ofthese receptors reduces the release of transmitter from theseexcitatory terminals. We therefore conclude that adenosine actingon A1 receptors can play an important role in determining thelevel of activity of the sympathetic nervous system at the levelof the spinalcord.

  FOOTNOTES

Received Feb. 1, 2001; revised May 17, 2001; accepted May 21, 2001.

We thank the British Heart Foundation and Wellcome Trust for their generous support, Brenda Frater for recovery of filledneurons, and Dr. Ida Llewellyn-Smith for help with recovery offilled neurons
Correspondence should be addressed to Dr. Susan A. Deuchars, School of Biomedical Sciences, Worsley Building, University ofLeeds, Leeds, LS2 9NQ, UK. E-mail: S.A.Deuchars{at}leeds.ac.uk.

  REFERENCES

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ABSTRACT
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MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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