Identification of the Dopamine D3 Receptor in Oligodendrocyte Precursors: Potential Role in Regulating Differentiation and Myelin Formation

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The Journal of Neuroscience, July 15, 1998, 18(14):5344-5353

Identification of the Dopamine D3 Receptor in Oligodendrocyte Precursors: Potential Role in Regulating Differentiation and Myelin Formation
Ernesto R. Bongarzone¹, Sherrel G. Howard¹^,², Vilma Schonmann¹, and Anthony T. Campagnoni¹
¹ Mental Retardation Research Center and Brain Research Institute and ² Molecular and Medical Pharmacology, School of Medicine, University of California at Los Angeles, Los Angeles, California 90024

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Expression of the dopamine D3 receptor (D3r) was found in primary mixed glial cultures from newborn brain and in the corpuscallosum in vivo during the peak of myelination. Expression ofthe D3r mRNA, but not D2r mRNA, was detected as early as 5 d invitro (DIV) by RT-PCR. Immunoblot studies revealed D3r proteinwas also expressed in the cultures. Double immunofluorescenceanalysis for the D3r and for surface markers of specific stagesof oligodendrocyte development indicated that D3r expression occurredin precursors and in immature oligodendrocytes but not in matureoligodendrocytes (i.e., A2B5⁺ 007 01 and A2B5⁺ 007⁺ 01 cells but not A2B5 007⁺ 01⁺ cells). Confocal microscopic analysis indicated that D3r wasassociated with cell bodies and cell membranes but not with theprocesses emanating from cell somas. Immunohistochemistry of brainsections revealed the presence of D3r in some oligodendrocyteslocated mainly within the genu and radiato of the corpus callosumduring the active period of myelination.
Treatment of cultures with 20 µM quinpirole led to decreased numbers of O1⁺ oligodendrocytes possessing myelin-like membranes as well asan increase in the number of precursors in 14 DIV cultures. Thiseffect was prevented by the dopamine antagonist haloperidol. Theseresults show that the D3r expression is not restricted to neuronsbut it is also expressed in differentiating oligodendrocytes beforeterminal maturation. It also suggests that dopamine or some otherD3r ligand may play a role in oligodendrocyte differentiationand/or the formation of myelin by mature oligodendrocytes.

Key words: myelination; dopamine receptors; brain development; cell lineage; oligodendroglia; neurotransmitters

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The D2 subfamily of dopamine receptors (D2r, D3r, and D4r) contains seven transmembrane regions (Bunzow et al., 1988; Sokoloffet al., 1990; Van Tol et al., 1991), a feature commonly associatedwith the members of the superfamily of G-protein-coupled receptors(Sibley et al., 1992). Although the activation of D2r and D4rinvolves the inhibition of adenyl cyclase (Sibley et al., 1992),the second messenger system associated with D3r has remained elusive(Sokoloff et al., 1992). The D3r gene encodes a 446 amino acidprotein with an overall homology of 52% with D2r, which increasesto 75% in the transmembrane domains (Sokoloff et al., 1990). Recently,a shorter isoform of D3r (425 amino acids) has been describedin the mouse, which appears to be pharmacologically active (Fishburnet al., 1993). The significance of these long and short activeisoforms of D3r is still unknown, but their presence might berelated to differential modulation of the dopaminergic system.

Like other neurotransmitter receptors, dopamine receptors are found within specific synaptic circuits in the CNS. The D3 receptorsubtype is expressed earlier than other dopamine receptor subtypes.Fishburn et al. (1996) were able to demonstrate the presence ofD3 receptor mRNA expression in mice as early as day 9.5 postconception(pc), whereas the D2 receptor subtype was not detectable beforeday 13.5 pc. The distribution and expression of D3r in the brainsof many species have been reported, including mouse (Demotes-Mainardet al., 1996), rat (Levesque et al., 1992; Landwehrmeyer et al.,1993a; Larson and Ariano, 1995), and human (Landwehrmeyer et al.,1993b), and they vary greatly depending on the area in the brain(Richtland et al., 1995). As the brain matures, the regional distributionof D3r becomes more defined, overlapping little with the D2r,(Gehlert et al., 1992; Diaz et al., 1995). During postnatal development,D3r mRNA concentrates in the mesocorticolimbic complex, with thehighest levels occurring in the nucleus accumbens, the Islandsof Calleja, and the olfactory tubercle (Levesque et al., 1992;Landwehrmeyer et al., 1993a; Ariano and Sibley, 1994).

The finding that some neurotransmitter receptors are actively expressed before the development and establishment of corticaland subcortical synapses during early embryonic development hasraised the possibility of alternative biological functions forthese receptors, in addition to their well described participationin synaptic transmission (Mattson, 1988). We have recently reportedthe expression of the D2r in oligodendrocytes (Howard et al.,1998), suggesting a possible nonsynaptic function for dopaminein these myelin-forming cells.

The purpose of this study was to examine the expression of the D2 receptor subfamily in oligodendrocytes in vitro and in vivo.Primary glial cultures have been well characterized and have provento be excellent models for examining the developmental expressionof genes important for oligodendrocyte survival and differentiation(Temple and Raff, 1985; Gard and Pfeiffer, 1990; Cameron and Rakik,1991; Barres et al., 1993). A large array of stage-specific markersis available with which to correlate gene expression and differentiationstate. Mature oligodendrocytes within these cultures elaboratemyelin-like membrane sheets providing a good in vitro model forexamining one of the major functions of this cell type. In thiscommunication, we describe the identification of D3r in immatureoligodendrocytes in vitro and in oligodendrocytes in vivo duringthe period of major myelin deposition, and we provide evidencethat D3r may modulate the timing of oligodendrocyte maturationand subsequent elaboration of myelin sheaths.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Tissue collection and cell culture. Brain cortices and olfactory tubercle and Island of Calleja areas collected from postnatalday 7 (P7) mouse brains were immediately frozen at $-$ 80°C. Theprocedure for culture of glial cells has been described in detailelsewhere (Bongarzone et al., 1996). Briefly, newborn (0- to 3-d-old)mouse cerebral hemispheres were dissociated through a nylon mesh,and cells were collected in 50 ml of 10% fetal calf serum DMEM.The cell suspension was poured through two collector tissue sieves(230 and 140 µm pore size) and centrifuged for 5 min at 100 ×g. The cells, 15 × 10⁶, were resuspended in 10 ml of medium and plated on 75 cm² culture flasks previously coated with poly-L-lysine and incubatedat 37°C 5% CO₂, with changes of medium every 4 d. Pellets of glialcells were prepared after 5, 7, 9, 11, 14, and 18 d in vitro (DIV)and immediately frozen in liquid nitrogen. Primary cultures werealso grown on poly-L-lysine-coated glass coverslips and fixedat the time points mentioned by incubation with 4% paraformaldehydein 1× PBS for 20 min at room temperature. Six-day-old primarycultures were treated with quinpirole, haloperidol, or the combinationof both drugs, with changes of drug-containing medium every 2d. Cells were collected for RNA isolation after 8 d of treatment(14 DIV after cell plating). In some cases, glial cells were grownon glass coverslips and then were fixed and processed for immunocytochemistryas described below. In other experiments, treatment was canceled6 DIV after initiation, and cells were maintained in drug-freemedium for another 4 DIV before being fixed and processed forimmunocytochemistry.

Extraction of RNA, cDNA synthesis, and RT-PCR reactions. Brain tissue or cell pellets were homogenized in an appropriate volume(100 mg of tissue/ml) of Trizol reagent (Life Technologies, Gaithersburg,MD) at 20,000 rpm for 30 sec (Polytron). Samples were incubatedfor 30 min at room temperature before extraction with chloroformfor 5 min. After centrifugation at 7000 rpm at 4°C, the aqueousphase was transferred to a new tube, and total RNA was precipitatedwith isopropanol at $-$ 20°C for a minimum of 1 hr. RNA was washedin 75% ethanol, redissolved in DEPC-treated water at a final concentrationof 5 mg RNA/ml, and stored at $-$ 80°C.

First-strand cDNA was synthesized by priming 20 µg of total RNA with an oligo-dT₁₅ and extension with Superscript reversetranscriptase (Life Technologies) at 42°C for 60 min. Two microlitersof the first-strand cDNA preparation were used as template inPCR reactions with the following specific sense and antisenseoligonucleotide primers: (1) D35, 5'-CCCTGTCCTACTGTGCACTCATC;and D33, 5'-ATAGAATCTTGAGGAAGGCTTTG; these primers direct theamplification from nucleotide 97 to 1333 for the mouse D3r cDNA(Fishburn et al., 1993); and (2) D25, 5'-GGCGCCCTATGGCTTGAAGAG;and D23, 5'-CCTAGGCAGGGAGGCGGCAAG; these primers direct the amplificationfrom nucleotide 78 to 1512 for the mouse D2r cDNA (Montmayeuret al., 1991). PCR conditions were 35 cycles, denaturation at94°C for 1.5 min, annealing at 63°C (D3r) or 64°C (D2r) for 1.5min, and extension at 72°C 1.5 min. PCR products were analyzedin a 1.5% agarose gel.

Cloning and sequencing. PCR fragments were cloned into the pCR 2.1 sequencing vector (Invitrogen, San Diego, CA). Sequenceanalysis was performed on cloned DNA strands by the Sanger dideoxychain termination method (Sambrook et al., 1989) with [ $alpha$ -³⁵S]dATP (DuPont NEN, Boston, MA) using one unit of Sequenase version2.0 (United States Biochemicals, Cleveland, OH) per reaction.

Southern blot. Ten microliters of D3 RT-PCR-amplified products were separated by electrophoresis in a 1.5% agarose gel andtransferred to a nylon membrane as described by Sambrook et al.(1989). After baking the membrane at 80°C for 2 hr, DNA was cross-linkedby UV irradiation. The blot was prehybridized with hybridizationsolution [2× SSC (1 ×SSC = 150 mM NaCl and 15 mM sodium citrate,pH 7.2), 1× Denhardt's solution, 0.1 mg/ml sheared salmon spermDNA (SS-DNA), 100 mM Tris-HCl, pH 7.6, and 1% SDS] without theprobe at 55°C for 2 hr. A specific oligonucleotide primer (5'-ATTTCAGCCGCATTTGCTGTG),whose sequence corresponds to nucleotides 289-310 from the D3rcDNA, was end-labeled with [ $gamma$ -³²P]dATP in the presence of T4 nucleotide kinase for 30 min at 37°C.The probe was further purified from nonincorporated radioactivityby ethanol precipitation. Hybridization (3 × 10⁶ cpm/ml) was performed at 55°C for 18 hr. Blot was washed (1×SSC and 1% SDS at 37°C) and exposed for 30 min at room temperature.

In situ hybridization. Sense and antisense oligonucleotide primers (same used for RT-PCR) specific for D3r sequence were end-labeledwith digoxigenin (DIG)-UTP as recommended by the manufacturer(Boehringer Mannheim, Indianapolis, IN). Fixed cultures were treatedfor 10 min with PBS containing 0.3% Triton X-100. Samples werewashed twice (5 min each) with PBS and then incubated for 10 minat 37°C with 100 mM Tris-HCl and 50 mM EDTA, pH 8.0, containing10 µg of RNase-free proteinase K/ml. Samples were rinsed twicein 2 mg/ml glycine in PBS and post-fixed for 10 min in 0.1% glutaraldehydeand 2% paraformaldehyde in PBS. Samples were then prehybridizedfor 2 hr at 42°C with hybridization buffer (50% deionized formamide,1× Denhardt's solution, 4× SSC, 1% SDS, 0.1 mg/ml yeast tRNA,and 0.1 mg/ml SS-DNA) before hybridization for 18 hr at 42°C inthis solution containing 100 ng/ml DIG-labeled primer. Sampleswere washed at 40°C in 50% formamide and 1× SSC and at room temperaturein 1× SSC and then blocked with 5% normal goat serum in Tris-bufferedsaline (TBS). Bound DIG probe was detected with anti-DIG antibodies(1:500). Preparations were washed in TBS and then incubated withnitroblue tetrazolium and X-phosphate as recommended by the manufacturer(Boehringer Mannheim). Color reaction was developed overnightin the darkness and stopped by rinsing the samples in 10 mM Tris-HCl,1 mM EDTA, and distilled water. Slides were mounted in Aquamount(Pittsburgh, PA).

Immunoblot. Membrane associated proteins were extracted with 0.1% Triton X-100 in the presence of a mixture of protease inhibitors,and 100 µg was electrophoresed in a 12% acrylamide-SDS gel (Laemmli,1970). Proteins were electrotransferred onto nitrocellulose membranes(Towbin et al., 1979), and blots were incubated with 5% nonfatmilk (Carnation) in TBS for 1 hr at room temperature. Polyclonalantibodies that recognize the C terminus of the D3r were diluted1:1000 in 0.5% blocking solution and incubated with the blotsfor 3 hr at room temperature. After washing the membranes withfresh 0.01% Tween 20 in TBS, goat anti-rabbit IgG antibodies labeledwith horseradish peroxidase were diluted 1:1500 and incubatedwith the blots for 1 hr at room temperature. Immunocomplexes werevisualized by enhanced chemiluminescence (Pierce, Rockford, IL).

Immunocytochemistry. Fixed cells were permeabilized by incubation with 0.01% Triton X-100 in PBS for 1.5 min at room temperature.Coverslips were blocked with 5% normal sheep serum (NSS) in PBSat room temperature for 2 hr. Samples were then incubated withthe following primary specific antibodies diluted in 0.5% NSSand 0.01% Tween 20 in PBS: goat polyclonal D3r anti-C terminus,1:800 (Santa Cruz Biotechnology, Santa Cruz, CA); mouse monoclonalanti-A2B5, 1:50 (American Type Culture Collection, Manassas, VA);mouse monoclonal anti-galactocerebroside (O1), 1:100 (Dr. A. Gard,Department of Structural Biology, University of South Alabama);mouse monoclonal anti-OO7, 1:100; monoclonal mouse anti-neurofilament,68 kDa, 1:100 (Chemicon, Temecula, CA); and rabbit polyclonalanti-neuron-specific enolase, 1:2000 (Chemicon). The first incubationwas performed at 4°C for 18 hr. Samples were rinsed thoroughlywith PBS and incubated with a 1:800 dilution of the appropriatesecondary antibodies labeled with fluorescein or rhodamine (BoehringerMannheim) for 2 hr at room temperature. Samples were then rinsedin PBS and then mounted on glass slides with Aquamount. Preparationswere observed by epifluorescence with a Leica DMR microscope andby confocal microscopy using a Zeiss LSM confocal microscope.

Immunohistochemistry. BALB/c mice at P3, P9, P14, and P25 and adult animals were profoundly anesthetized using halothane,perfused using a chilled sterile solution of PBS, and then fixedwith 2% paraformaldehyde in PBS. Brains were dissected out andpost-fixed overnight in 4% paraformaldehyde in PBS. Tissue wascryoprotected with OCT, frozen, and then used to cut coronallyoriented sections. Sections were processed for immunohistochemistryusing the free-floating technique. Endogenous peroxidase activitywas quenched by incubating the sections in 0.1% H₂O₂ in PBS for15 min. Tissue was then blocked in 10% normal rabbit serum (NRS)in PBS for 2 hr at room temperature. Sections were incubated withgoat anti-D3r antiserum (Santa Cruz), diluted 1:600 in 1% NRSand 0.02% Tween-20 for 72 hr at 4°C. Bound primary antibody wasdetected using the avidin-biotin-peroxidase system as recommendedby the manufacturer (Vector Laboratories, Burlingame, CA). Afterdevelopment with diaminobenzidine, nickel ions, and H₂O₂, sectionswere mounted on gold-plus slides (Fisher Scientific), air-dried,dehydrated with serial graded ethanol, clarified in xylenes, andcoverslipped with Permount.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Glial cells express the D3r in 14 DIV primary cultures

We analyzed whether cultured oligodendrocytes might express the principal members of the D2 subfamily of dopamine receptorsduring their in vitro differentiation. Glial cell cultures wereestablished from newborn mice (P0-P3) and maintained for 2-3 weeks.Under the experimental conditions described in this study, anycontaminating neurons, a potential source of dopamine receptors,did not survive. This was confirmed by the absence of immunoreactivityto the neuronal 68 kDa neurofilament and neuron-specific enolase(data not shown).

Glial cells were harvested at 7, 14, and 18 DIV, and their mRNAs were reverse-transcribed and used in PCR experiments designedto specifically detect the presence of either the D3r or the D2rmRNA. Primers D35 and D33 were chosen for the amplification ofthe long (1236 bp) and the short (1183 bp) isoforms of D3r (Fig.1A), and primers D25 and D23 were selected to amplify the long(1404 bp) and the short (1346 bp) isoforms of the D2r (Fig. 1A).Both isoforms of the D2r were easily detected in the P7 mousebrain sample (Fig. 1B). In contrast, neither D2r isoform was detectedin 7 or 14 DIV primary glial cultures (Fig. 1B) or in 18 DIV preparations(data not shown). The long isoform of the D3r, but not the shortisoform, was amplified from P7 mouse brain (Fig. 1B). Interestingly,an intense band corresponding to the long D3r mRNA was detectedin both 7 and 14 DIV primary cultures of mouse glia (Fig. 1B).The same result was obtained with a sample from 18 DIV primarycultures.

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Figure 1. Primary cultures of glia express the D3r but not the D2r mRNA. The message for both dopamine receptors was detected by RT-PCR analysis. A, The scheme illustrates the structural organization of the D2r and D3r genes and their mRNAs. Two sets of specific oligonucleotide primers (open arrows, sense primers; filled arrows, antisense primers) were designed to amplify the cDNAs containing the open reading frame sequence for these receptors. B, Ethidium bromide staining of RT-PCR fragments. The mRNAs for both isoforms of the D2r were detected in a P7 brain sample, although no expression of this receptor was evidenced by RT-PCR in the glial samples at 7 or 14 DIV. The 1236 bp cDNA for the long D3r was readily amplified from the P7 brain sample. A single band with the same relative size was also detected in RNA samples from 7 and 14 DIV primary cultures of glia.

To confirm the identity of the putative long D3r detected in the glial cultures, PCR fragments were subcloned and sequenced,and the products were found to be 100% homologous with the mouselong D3r (Fishburn et al., 1993).

Process-bearing cells express the D3r mRNA

Our primary cultures of glia are composed of a mixture of astrocytes (~70%), oligodendrocytes (~20%) and microglia (~10%).Thus, the mRNA encoding the long D3r might have arisen from anyof these cell types. To determine the cellular origin of the D3rexpression, an in situ hybridization analysis was performed withspecific D3r sense and antisense oligonucleotides labeled withdigoxigenin. Figure 2 shows the results of such an experimentperformed with a D3r antisense (Fig. 2B) and a control sense probe(Fig. 2A). With the antisense probe a strong, specific signalcould be detected primarily within process-bearing cells of thesize and morphology of cells in the oligodendroglial lineage.No labeling of astrocytes was evident.

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Figure 2. D3r mRNA is produced in oligodendroglial-like cells in culture. D3r message was detected in 14 DIV primary cultures of mouse glia by in situ hybridization using an antisense oligonucleotide labeled with digoxigenin specific for the 3' end of exon 6 of D3r (B). Note that only cells with the morphology described for oligodendrocytes were detected. The staining is restricted to only the oligodendroglial cell bodies, and no message was evidenced within the cellular processes. The astrocytic layer (lining underneath the oligodendrocytes) was barely stained, and it is comparable to the nonspecific staining using a sense oligonucleotide (A). Scale bar, 20 µm.

Developmental expression of the D3r begins around 5 DIV in primary cultures of glia

We analyzed changes in the expression of the D3r mRNA with time in culture. The D3r mRNA was reverse transcribed and amplifiedby PCR at different stages over a period of 2 weeks after plating.The PCR fragments were identified by Southern blot using a D3r-specificradiolabeled oligonucleotide. A single band with the predictedsize of ~1.2 kb, corresponding to the long isoform of the D3r,was detected in the control RNA sample isolated from P7 mousebrain (Fig. 3A). A similar band was also identified in all theRNA samples isolated from primary glial cultures, ranging from5 to 14 DIV (Fig. 3A). Although not a quantitative analysis, theexperimental conditions for the RT-PCR were strictly maintainedfor all the samples, and there were no evident changes in theintensity of the bands, suggesting that the expression of theD3r mRNA is maintained at similar levels over the first 2 weeksof culture.

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Figure 3. The in vitro expression of D3r seems to follow a developmentally regulated pattern. A, By Southern blot analysis using a specific radiolabeled internal oligonucleotide, D3r message was identified in RT-PCR samples generated from P7 brain and glial primary cultures at 5, 9, 11, and 14 DIV. B, By immunoblot detection, D3r proteins were detected in the membrane extracts from the olfactory tubercle isolated from P7 brain as a 49 kDa product (possibly the nonglycosylated form of the receptor) and a 70 kDa product (possibly the glycosylated form of the receptor). D3r proteins were also immunodetected in membrane proteins extracted from primary cultures at 5, 9, 11, and 14 DIV.

We investigated whether the D3r mRNA was translated into protein by Western blot analysis. Using an antibody specific to theC terminus of the D3r protein, we were able to detect the immature,presumably nonglycosylated, state of the D3r with the predictedrelative molecular weight of 49 kDa in a control membrane extractfrom the olfactory tubercle area of P7 mouse brain (Fig. 3B).A high molecular weight band (~70 kDa), presumably the fully glycosylatedversion of the receptor, was also immunodetected by the antibodies.The same basic pattern of the 49 and 70 kDa proteins was identifiedin membrane protein extracts isolated from primary cultures (Fig.3B). Interestingly, the level of D3r protein produced in glialcultures seemed to increase as the cultures aged, appearing toreach a peak of expression between 9 and 11 DIV and then decreasingslightly at 14 DIV (Fig. 3B). The bands on the Western blots between49 and 70 kDa presumably represent D3r products with varying levelsof glycosylation.

D3r is expressed primarily in immature oligodendrocytes and is localized in the plasma membrane and cell bodies but not in the cell processes

Oligodendrocyte differentiation in vitro has been examined extensively with the use of stage-specific markers. Through theuse of double immunocytochemistry, we were able to study the coexpressionof D3r with early and late markers of oligodendrocyte differentiation.At 7 DIV, oligodendrocyte precursors could be identified withmarkers such as A2B5 and GD3. At 7 DIV, oligodendrocyte precursorswere stained with the monoclonal antibody A2B5 (Fig. 4B, red fluorescence).All the A2B5⁺ oligodendrocyte precursor cells were found to express D3r (Fig.4B, arrows, green fluorescence). In these cells, the D3r immunoreactivitywas found associated with cell bodies, and little immunoreactivitywas detected in processes. At later stages (14 DIV) some oligodendrocytesthat had reached the stage of myelin membrane formation were easilyobserved by staining with the mature oligodendrocyte marker O1.As seen in Figure 4D these O1⁺ cells (red fluorescence) elaborated flattened, myelin-like sheets.The somas of these O1⁺ cells stained only very weakly, if at all, with the anti-D3rantibody (Fig. 4D, green fluorescence). At this stage there weremany O1 D3r⁺ cells with the morphological characteristics of immature oligodendrocytes(Fig. 4D, arrows).

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Figure 4. D3r colocalizes with A2B5⁺ but only occasionally with O1⁺ cells. Primary cultures were fixed at 7 DIV (A, B) and 14 DIV (C, D) and were analyzed by double immunofluorescence to detect D3r (green) with A2B5 (B) and O1 (D) (red). A, C, Phase-contrast micrographs corresponding to B and D, respectively. D3r colocalized with the early oligodendroglial marker A2B5 in all progenitor cells (B, arrows). At later stages in differentiation, oligodendrocytes that have started the synthesis of myelin membranes (evidenced with the monoclonal antibody O1; D) were faintly stained in their soma with the antibody against D3r (D). However, many D3r⁺ O1 cells without visible processes were also observed (D, arrows). Scale bars: B, 15 µm; D, 20 µm.

In these immunocytochemical studies, D3r was consistently observed to be associated with the cell bodies of the oligodendrocyteprecursors, and very little signal was observed within their processes.To illustrate this differential localization more clearly, Figure5 shows the subcellular distribution of D3r (red fluorescence)in 9 DIV primary cultures of glia doubly stained with 007 antibodies(green fluorescence) analyzed by confocal microscopy. The 007is a surface marker that stains cells that are more differentiatedthan oligodendrocyte precursors, including immature and matureoligodendrocytes. As Figure 5 shows, D3r was observed in associationwith the cell bodies and cell membrane of the 007⁺ cells but the processes of these cells (stained in green with007) did not stain for D3r protein. Taken together, the doubleimmunocytochemical studies indicate that D3r is expressed primarilyin oligodendrocyte precursors and immature oligodendrocytes butnot in mature oligodendrocytes. Furthermore, D3r does not appearto localize in the cell processes of these cells.

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Figure 5. D3r was detected in association with the plasma membrane but not with the cellular processes in differentiating oligodendrocytes. The subcellular localization of the D3r was studied in double immunofluorescence (D3r, red; OO7, green) staining of 9 DIV primary cultures by confocal microscopy. D3r was detected in association with the plasma membrane of oligodendrocytes, which could be clearly evidenced with the OO7 antibody. D3r immunoreaction was also observed within the cytoplasm of these cells. A network of cellular processes was easily visualized with OO7; however, no D3r immunoreaction was detected in association with them. Scale bar, 20 µm.

D3r is transiently expressed in oligodendrocytes located within the corpus callosum during the period of myelination

We wanted to determine whether oligodendrocytes in vivo expressed the D3r. To do this we performed immunohistochemical studieswith a D3r-specific antibody during the early postnatal periodof brain development, just before maximal myelination in the brain.A number of brain structures showed immunodetectable levels ofthe receptor. During the developmental period examined, D3r expressionwas noted in large neurons located in the mesocorticolimbic area.Highest expression was observed in the Island of Calleja and olfactorytubercle. These areas showed the earliest expression of D3r (P3)that was maintained throughout the developmental period examined.Figure 6B shows a representative field of a coronal section atthe level of Island of Calleja of a P14 mouse brain in which D3rwas localized in large clustered neurons of ~20 µm in diameter.D3r was also found expressed in pyramidal cells within layers3 and 5 of the prefrontal cortex and in a lower level in the nucleusaccumbens (data not shown).

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Figure 6. D3r was detected in differentiating oligodendrocytes in the corpus callosum. The anatomical distribution of D3r was examined by immunohistochemistry in brain sections during the first 4 postnatal weeks and in the adult brain. A, Nonspecific staining of P14 corpus callosum using nonimmune serum. B, Mesocorticolimbic large-sized neurons from Islands of Calleja were heavily immunostained with the anti-D3r antibody. C-E, Micrographs showing a portion of the genu corpus callosum immunostained with the anti-D3r antibody at P3 (C), P14 (D), and P25 (E). Cells with small somal diameters (~7 µm) arranged in "strings" (arrowheads) or scattered individually throughout the white matter (arrows) were evident at P14 and to a lesser extent at P25. Scale bars: B, 20 mm; C-E, 10 mm.

To determine whether cells in the oligodendrocyte lineage expressed D3r, we focused our analysis on white matter areas, particularlyin the corpus callosum in which >90% of the cells are oligodendrocytes.Cells with small cell bodies stained with the anti-D3r antibodyin fiber tracts located adjacent to the neocortex. These cellshad small somal diameters (~7 µm) with the "string of pearls"orientation characteristic of interfascicular oligodendrocytes(Peters et al., 1991). In addition to these, cells of similarmorphology and size were scattered individually throughout thewhite matter tracts (Fig. 6). At P3 very little immunostainingcould be observed in these cells (Fig. 6C). However, at laterstages of neural development (beginning at P9; data not shown),D3r was evident within these oligodendroglial cells, with a peakof expression observed at P14, approximately 1 week before maximalmyelination in this area (Fig. 6D). In the adult brain, whitematter was barely immunoreactive, showing very few D3r⁺ cells in a scattered distribution throughout the fiber tracts(data not shown). These cells were of the size and morphologyof small neurons. During development, D3r⁺ oligodendroglia was located almost exclusively in the genu ofthe corpus callosum, and some D3r⁺ cells were observed entering the radiato of the corpus callosum.No staining was evident in the external capsule or the anteriorcommissure. It is important to note that in all the cells analyzed,D3r was always associated with the cell bodies, and there wasno immunostaining of the processes. Satellite and perivascularoligodendrocytes and astroglia did not show expression of thereceptor at any stage of development.

Treatment of glial cultures with the dopamine agonist quinpirole altered the normal pattern of oligodendrocyte differentiation

It was of interest to determine whether the presence of the D3r had any functional significance for the oligodendrocyte. Accordingly,we examined whether quinpirole, a dopamine D2r/D3r agonist, hadany effect on oligodendrocyte differentiation and/or myelin formationin the glial cultures. In vitro differentiation of quinpirole-treatedprimary cultures was evaluated by counting the number of A2B5⁺ cells, O1⁺ cells, and O1⁺ cells bearing myelin-like sheets in 14 DIV primary cultures.A2B5 was used as a marker for oligodendrocyte precursor cells,and O1 was used as a marker for mature oligodendrocytes. As shownin Figure 7A, there is normally a drop in the number of A2B5⁺ cells as the cultures mature. In this case the number of A2B5⁺ cells decreased from 21 cells per field at 7 DIV to 9 cells perfield at 14 DIV. Treatment of the primary cultures with the agonistquinpirole resulted in an increase in the number of A2B5⁺ cells in the 14 DIV cultures from 9 to 14 cells per field. Tobe certain that the effect of quinpirole was mediated throughD3r, parallel primary cultures were treated with quinpirole andthe dopamine antagonist haloperidol. Under these conditions, theantagonist blocked the effect of the agonist, with the numberof A2B5⁺ cells reaching levels similar to the untreated control at 14DIV (Fig. 7A). Treatment with quinpirole had little effect onthe number of oligodendrocytes at 14 DIV (Fig. 7A).

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Figure 7. Stimulation of D3r by quinpirole decreased the in vitro differentiation of oligodendrocytes. A, The in vitro differentiation of oligodendrocytes was analyzed by counting the number of immature A2B5⁺ cells remaining in 14 DIV cultures and compared with the respective number in cultures at 7 DIV. The activation of D3r by quinpirole induced an increase of the number of A2B5⁺ cells in 14 DIV primary cultures with respect to the untreated control. This effect was blocked by coincubation with the antagonist haloperidol. Data are presented as the number of A2B5⁺ cells counted per field (0.1 mm²). At least 10 fields were observed from three separated experiments. Results were analyzed by the one-way ANOVA test (p < 0.05). The number of oligodendrocytes present at 14 DIV (analyzed by the presence of the marker O1) was also counted and analyzed as described previously. B, In vitro differentiation of oligodendrocytes was also evaluated by counting the number of O1⁺ cells connected to myelin-like membranes in 14 DIV (condition 1) and 16 DIV (condition 2) primary cultures. In condition 1, quinpirole or haloperidol treatments were begun at 6 DIV and continued until 14 DIV, and cultures were analyzed. Under this condition quinpirole induced a marked decrease (46%) of O1⁺ cells bearing myelin sheets compared with the untreated or haloperidol controls. In condition 2, quinpirole or haloperidol treatments were begun at 6 DIV, the drugs were removed at 12 DIV, and the cultures were analyzed at 16 DIV. Quinpirole treatment for day 6 appeared to be sufficient to reduce the numbers of sheet-bearing cells at 16 DIV with no apparent recovery after removal of the drug. Data represent the average of three separated experiments in triplicate and were analyzed by the one-way ANOVA test (p < 0.05). C, D, Immunofluorescence analysis of O1⁺ cells associated to myelin-like membranes in 14 DIV control (C) and quinpirole-treated (D) primary cultures. Observe the lesser extension of myelin-like membranes in the treated samples (D). Scale bar, 25 µm.

Interestingly, agonist stimulation of D3r led to a 46% decrease in the number of O1⁺ oligodendrocytes bearing myelin sheets compared with untreatedcontrols (Fig. 7B). Furthermore, the presence of haloperidol antagonizedthe effect of quinpirole, increasing the number of oligodendrocytesbearing sheets to 92% of the untreated control. To investigatewhether the effect of D3r on the formation of myelin membraneswas irreversible, primary cultures were treated for 6 DIV andthen switched to a drug-free medium for another 4 DIV before O1⁺ cells bearing myelin-like membranes were counted. Interestingly,the number of quinpirole-treated oligodendrocytes associated withmyelin sheets (51%) did not return to normal levels 4 DIV afterwithdrawal of the drug (Fig. 7B). However, the antagonizing effectof haloperidol increased the number of cells associated with myelinsheets to 92% of the untreated control (Fig. 7B). The dose ofdrugs used in these studies (20 µM) did not produce any degenerationof the cultures and was substantially lower than that needed tocause a lethal effect on glial cells (data not shown). Figure7, C and D, illustrates the differences in membrane sheet formationbetween oligodendrocytes in the quinpirole-treated cultures (Fig.7D) and untreated cultures (Fig. 7C). Larger numbers of oligodendrocytesin the control cultures elaborated more extensive areas of myelinsheets at 14 DIV than in the quinpirole-treated cultures.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Our results show the expression of the D3r in immature oligodendrocytes in mouse primary glial cultures. We saw little orno expression of the D3r in mature oligodendrocytes. Interestingly,we were able to detect the D3r mRNA easily at 5 DIV, a time whenimmunoreactive protein on Western blots was detected at very lowlevels. Expression of the D3r in cells in the oligodendrocytelineage was confirmed in vivo, particularly in cells within thecorpus callosum before the period of maximal myelination in themouse brain.

Our finding that the D3r is expressed in immature oligodendrocytes represents the third neurotransmitter receptor system tobe identified in oligodendrocytes and their precursors. Galloet al. (1989, 1996) have described the properties of the glutamatereceptors in oligodendrocytes, and expression of the GABA_A receptorhas been reported in oligodendrocytes (Kettenmann, 1989; Von Blankenfeldet al., 1991). These results indicate that these neurotransmitterreceptors are involved in processes other than nerve conductionin oligodendrocytes, and they raise the interesting question ofwhat their functions might be in these glial cells. The conceptthat classical neurotransmitters may have additional, perhapstrophic, functions in glial and neuronal differentiation has beenunder consideration for some time and for which there is substantialprecedent in the literature (for review, see Lauder, 1993).

Gallo et al. (1996) have presented evidence that glutamate receptors might be involved in oligodendrocyte progenitor cellproliferation. In this study, we found that quinpirole (a D2/D3dopamine agonist) caused an increase of ~50% in the numbers ofoligodendrocyte precursors present in 14 DIV cultures. Furthermore,treatment with quinpirole significantly reduced the numbers ofoligodendrocytes elaborating membranous sheets, generally takento represent oligodendrocytes at their most differentiated state.These results suggest that dopamine or some other endogenous D3rligand, acting through this receptor, could prevent the oligodendrocytefrom myelinating prematurely by delaying subsequent myelin sheathelaboration. The effect of the agonist seems to be irreversible,because relatively brief exposure to the drug is sufficient todecrease sheet-bearing cells in vitro. The extent to which dopamineor some other D3r ligand might influence myelination in vivo remainsto be determined.

Expression of the D3r in cells in the oligodendrocyte lineage was noted only in the corpus callosum during a developmentalstage at which oligodendrocytes are beginning to elaborate processesand ensheathing axons. As brain maturation occurred, the expressionof D3r in these cells was found to decrease. In the adult nervoussystem, only scattered cells were labeled in the corpus callosum,which correlates well with the observed absence of D3r expressionin fully mature oligodendrocytes in vitro.

Although innervation by the dopamine system is somewhat restricted, anatomically there are three well defined dopamine systemsin the adult brain. The most studied has been the nigrostriatalsystem. Dopaminergic cell bodies, located in the zona compactaof the substantia nigra, project primarily to the neostriatumand the amygdala. In the second system cell bodies of the mesolimbicdopamine system are located in the ventral tegmental area andinnervate the nucleous accumbens and the olfactory tubercles.In the third system, cell bodies primarily from the hypothalamusinnervate the external layer of the median eminence. Thus, areasof the brain such as the corpus callosum, in which D3r expressionin oligodendrocytes was demonstrated, are surrounded by areasrich in dopamine. Certainly, at the time when oligodendrocyteprecursors are dividing and migrating within the brain, i.e.,shortly after birth in the mouse, the extracellular concentrationof dopamine (which has diffused out of, or is released from thenerve terminal) is relatively high compared with adult levels(Howard et al., 1997), although the reuptake mechanism for thecatecholamines is not yet fully developed (Nomura et al., 1976).The high water content of the brain could result in widespreaddiffusion of dopamine, such that dopamine could act on cells suchas oligodendrocyte precursors. As oligodendrocytes reach theirfully differentiated state in culture, D3r expression appearsto disappear, which would make the fully mature oligodendrocytesrefractory to the actions of dopamine or some other D3r ligand,at least through this receptor.

There is accumulating evidence that some neurotransmitters may participate in the modeling of neuronal shape and the outgrowthof their neurites (for review, see Mattson, 1988). Todd (1992)has shown that activation of D2r with quinpirole induced an increasein the neurite length of primary cultures of cortical neurons.More recently, Swarzenski et al. (1994) demonstrated that notonly D2r, but also D3r and D4r, may regulate the outgrowth ofneuronal processes. Indeed, the modulation of a number of neurotransmitterreceptors during early brain development can dramatically influencethe cytoarchitecture of different populations of neurons (Chubakovet al., 1986; Hauser et al., 1987; Mattson et al., 1989; Blantonet al., 1990; Lo Turco et al., 1991). It is not unreasonable,then, that in a cell whose primary function is to elaborate myelinmembrane, at least the dopamine system, might modulate the cytoarchitectureof the oligodendrocyte in terms of the amounts and timing of myelinformation.

Recently, we reported the presence of the D2r in a subset of mature interfascicular oligodendrocytes in the rat corpus callosum(Howard et al., 1998). This and the present study have shown thatcells in the oligodendrocyte lineage are capable of expressingmembers of the D2 subfamily of receptors. Although this remainsto be investigated further, we suggest that the D3 and D2 receptorsare expressed at different stages in oligodendrocyte developmentand that this expression may be involved in regulating myelinformation in the lineage. We propose that the immature oligodendrocytesexpress D3r, and this may serve to regulate myelin formation bysome, as yet unknown, mechanism. This expression normally disappearsin mature myelinating oligodendrocytes, rendering the cells unableto respond to dopamine or a related endogenous ligand and thereforeenabling the cells to complete their differentiation. In our previousstudy D2r was not detected in oligodendroglial cells at earlystages of brain development associated with oligodendroglial progenitorappearance and proliferation. This suggests that the expressionof D3r in cells of the oligodendrocyte lineage occurs after D3rexpression.

In summary, we have presented evidence that the D3r is present in cells within the oligodendrocyte lineage and that it mayplay a role in either the differentiation of oligodendrocytesand/or subsequent membrane formation by these cells. This addsanother important function for dopamine in the developing brainbeyond its well known role as a neurotransmitter.

  FOOTNOTES

Received Jan. 27, 1998; revised April 16, 1998; accepted May 1, 1998.

This work was supported by Grant NS23022 from the National Institutes of Health and Grants RG2693 (A.T.C.) and PP0573 (S.G.H.)from the National Multiple Sclerosis Society.
Correspondence should be addressed to Anthony T. Campagnoni, Mental Retardation Research Center and Brain Research Institute,School of Medicine, University of California at Los Angeles, 760Westwood Plaza, Los Angeles, CA 90024.

  REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Ariano MA, Sibley DR (1994) Dopamine receptor distribution in the rat CNS: elucidation using anti-peptide antisera directed against D1A and D3 subtypes. Brain Res 649:95-110[ISI][Medline].
Barres BA, Schmid R, Sendtner M, Raff MC (1993) Multiple extracellular signals are required for long-term oligodendrocyte survival. Development 118:283-295[Abstract].
Blanton MG, Lo Turco JJ, Kriegstein AR (1990) Endogenous neurotransmitter activates N-methyl-D-aspartate receptors on differentiating neurons in embryonic cortex. Proc Natl Acad Sci USA 87:8027-8030[Abstract/Free Full Text].
Bongarzone ER, Foster LM, Byravan S, Verity AN, Landry CF, Schonmann V, Amur-Umarjee S, Campagnoni AT (1996) Conditionally immortalized neural cell lines: potential models for the study of neural cell function. In: Methods, a companion to methods in enzymology (Murphy S, ed), pp 489-500. San Diego: Academic.
Bunzow JR, Van Tol HH, Grandy DK, Albert P, Salon J, Christie M, Machida CA, Neve KA, Civelli O (1988) Cloning and expression of a rat D2 dopamine receptor cDNA. Nature 336:783-787[Medline].
Cameron RS, Rakik P (1991) Glial cell lineage in the cerebral cortex: a review and synthesis. Glia 4:124-137[ISI][Medline].
Chubakov AR, Gromova EA, Konovalov GV, Sarkisova EF, Chumasov EI (1986) The effects of serotonin on the morphofunctional development of rat cerebral neocortex in tissue culture. Brain Res 369:285-297[ISI][Medline].
Demotes-Mainard J, Henry C, Jeantet Y, Arsaut J, Arnauld E (1996) Postnatal ontogeny of dopamine D3 receptors in the mouse brain: autoradiographic evidence for a transient cortical expression. Brain Res Dev Brain Res 94:166-174[Medline].
Diaz J, Levesque D, Lammers CH, Griffon N, Martres MP, Schwartz JC, Sokoloff P (1995) Phenotypical characterization of neurons expressing the dopamine D3 receptor in the rat brain. Neuroscience 65:731-745[ISI][Medline].
Fishburn CS, Belleli D, David C, Carmon S, Fuchs S (1993) A novel short isoform of the D3 dopamine receptor generated by alternative splicing in the third cytoplasmic loop. J Biol Chem 268:5872-5878[Abstract/Free Full Text].
Fishburn CS, Bedford M, Lonai P, Fuchs S (1996) Early expression of D3 dopamine receptors in murine embryonic development. FEBS Lett 381:257-261[ISI][Medline].
Gallo V, Suergiu R, Giovannini C, Levi G (1989) Expression of excitatory amino acid receptors by cerebellar cells of the type-2 astrocyte cell lineage. J Neurochem 52:1-9[ISI][Medline].
Gallo V, Zhou JM, McBain J, Wright P, Knutson PL, Armstrong RC (1996) Oligodendrocyte progenitor cell proliferation and lineage progression are regulated by glutamate receptor-mediated K⁺ channel block. J Neurosci 16:2659-2670[Abstract/Free Full Text].
Gard AL, Pfeiffer SE (1990) Two proliferative stages of the oligodendrocyte lineage (A2B5+O4 $-$ and O4+GalC $-$ ) under different mitogenic control. Neuron 5:615-625[ISI][Medline].
Gehlert DR, Gackenheimer SL, Seeman P, Schaus J (1992) Autoradiographic localization of [³H]quinpirole binding to dopamine D2 and D3 receptors in rat brain. Eur J Pharmacol 211:189-194[Medline].
Hauser KF, McLaughlin PJ, Zagon IS (1987) Endogenous opioids regulate dendritic growth and spine formation in developing rat brain. Brain Res 416:157-161[ISI][Medline].
Howard S, Fisher R, Landry C (1997) Alterations in the spontaneous release of dopamine and the density of the DA D2 receptor mRNA after chronic postnatal exposure to cocaine. Brain Res Bull 43:101-106[Medline].
Howard S, Landry C, Fisher R, Bezouglaia O, Handley V, Campagnoni AT (1998) The postnatal localization and morphogenesis of cells expressing the dopaminergic D2 receptor gene in rat brain: expression in non-neuronal cells. J Comp Neurol 391:87-98[ISI][Medline].
Kettenmann H (1989) GABA triggers a Cl $-$ efflux from cultured glial cells. Acta Physiol Scand Suppl 582:50.
Laemmli UK (1970) Cleavage of structural proteins during the assembly of the head of the bacteriophage T4. Nature 227:680-685[Medline].
Landwehrmeyer B, Mengod G, Palacios JM (1993a) Differential visualization of dopamine D2 and D3 receptor sites in rat brain. A comparative study using in situ hybridization histochemistry and ligand binding autoradiography. Eur J Neurosci 5:145-153[ISI][Medline].
Landwehrmeyer B, Mengod G, Palacios JM (1993b) Dopamine D3 receptor mRNA and binding sites in human brain. Brain Res Mol Brain Res 18:187-192[Medline].
Larson ER, Ariano MA (1995) D3 and D2 dopamine receptors: visualization of cellular expression patterns in motor and limbic structures. Synapse 20:325-337[ISI][Medline].
Lauder JM (1993) Neurotransmitters as growth regulatory signals: role of receptors and second messengers. Trends Neurosci 16:233-240[ISI][Medline].
Levesque D, Diaz J, Pilon C, Martres MP, Giros B, Souil E, Schott D, Morgat JL, Schwartz JC, Sokoloff P (1992) Identification, characterization, and localization of the dopamine D3 receptor in rat brain using 7-[³H]hydroxy-N,N-di-n-propyl-2-aminotetralin. Proc Natl Acad Sci USA 89:8155-8159[Abstract/Free Full Text].
Lo Turco JJ, Blanton MG, Kriegstein AR (1991) Initial expression and endogenous activation of NMDA channels in early neocortical development. J Neurosci 11:792-799[Abstract].
Mattson MP (1988) Neurotransmitters in the regulation of neuronal cytoarchitecture. Brain Res Rev 13:179-212.
Mattson MP, Lee RE, Adams ME, Guthrie PB, Kater SB (1989) Interactions between entorhinal axons and target hippocampal neurons: a role for glutamate in the development of hippocampal circuitry. Neuron 1:865-876.
Montmayeur JP, Bausero P, Amlaiky N, Maroteaux L, Hen R, Borrelli E (1991) Differential expression of the mouse dopamine receptor isoforms. FEBS Lett 278:239-243[ISI][Medline].
Nomura Y, Naitoh F, Segawa T (1976) Regional changes in monoamine content and uptake of the rat brain during postnatal development. Brain Res 101:305-315[ISI][Medline].
Peters A, Palay S, Webster H (1991) In: The fine structure of the nervous system. Oxford: Oxford UP.
Richtland NM, Kelsoe JR, Segal DS, Kuczenski R (1995) Regional quantification of D1, D2, and D3 dopamine receptor mRNA in rat brain using a ribonuclease protection assay. Mol Brain Res 33:97-103[Medline].
Sambrook J, Frisch EF, Maniatis T (1989) In: Molecular cloning: a laboratory manual. Cold Spring Harbor, NY: Cold Spring Harbor Laboratory.
Sibley DR, Monsma Jr FJ, Shen Y (1992) Molecular neurobiology of dopaminergic receptors. Int Rev Neurobiol 35:391-415.
Sokoloff P, Giros B, Martres MP, Bouthenet ML, Schwartz JC (1990) Molecular cloning and characterization of a novel dopamine receptor (D3) as a target for neuroleptics. Nature 347:146-151[Medline].
Sokoloff P, Giros B, Martres MP, Andrieux M, Besancon R, Pilon C, Bouthenet ML, Souil E, Schwartz JC (1992) Localization and function of the D3 dopamine receptor. Arzneimittelforschung 42:224-230[Medline].
Swarzenski BC, Tang L, Oh YJ, O'Malley KL, Todd RD (1994) Morphogenic potentials of D2, D3, and D4 dopamine receptors revealed in transfected neuronal cell lines. Proc Natl Acad Sci USA 91:649-653[Abstract/Free Full Text].
Temple S, Raff M (1985) Differentiation of a bipotential glial progenitor cell in a single cell microculture. Nature 313:223-225[Medline].
Todd RD (1992) Neural development is regulated by classical neurotransmitters: dopamine D2 receptor stimulation enhances neurite outgrowth. Biol Psychiatry 31:794-807[ISI][Medline].
Towbin H, Staehlin T, Gordon J (1979) Electrophoretic transfer of proteins from polyacrylamide gels to nitrocellulose sheets: procedure and some applications. Proc Natl Acad Sci USA 76:4350-4354[Abstract/Free Full Text].
Van Tol HHM, Bunzow JR, Guan HC, Sunahara RK, Seeman P, Niznik HB, Civelli O (1991) Cloning of the gene for a human dopamine D4 receptor with high affinity for the antipsychotic clazapine. Nature 350:610-615[Medline].
Von Blankenfeld G, Trotter J, Kettenmann H (1991) Expression and developmental regulation of GABA_A receptor in cultured murine cells of the oligodendrocyte lineage. Eur J Neurosci 3:310-316[ISI][Medline].

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