Specification of Distinct Dopaminergic Neural Pathways: Roles of the Eph Family Receptor EphB1 and Ligand Ephrin-B2

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The Journal of Neuroscience, March 15, 1999, 19(6):2090-2101

Specification of Distinct Dopaminergic Neural Pathways: Roles of the Eph Family Receptor EphB1 and Ligand Ephrin-B2
Yong Yue¹, David A. J. Widmer², Alycia K. Halladay², Douglas Pat Cerretti³, George C. Wagner², Jean-Luc Dreyer⁴, and Renping Zhou¹
¹ Laboratory for Cancer Research, College of Pharmacy, and ² Department of Psychology, Rutgers University, Piscataway, New Jersey 08855, ³ Immunex Corporation, Seattle, Washington 98101, and ⁴ Department of Biochemistry, University of Fribourg, 1700 Fribourg, Switzerland

  ABSTRACT

Top
Abstract
Introduction
References

Dopaminergic neurons in the substantia nigra and ventral tegmental area project to the caudate putamen and nucleus accumbens/olfactorytubercle, respectively, constituting mesostriatal and mesolimbicpathways. The molecular signals that confer target specificityof different dopaminergic neurons are not known. We now reportthat EphB1 and ephrin-B2, a receptor and ligand of the Eph family,are candidate guidance molecules for the development of thesedistinct pathways. EphB1 and ephrin-B2 are expressed in complementarypatterns in the midbrain dopaminergic neurons and their targets,and the ligand specifically inhibits the growth of neurites andinduces the cell loss of substantia nigra, but not ventral tegmental,dopaminergic neurons. These studies suggest that the ligand-receptorpair may contribute to the establishment of distinct neural pathwaysby selectively inhibiting the neurite outgrowth and cell survivalof mistargeted neurons. In addition, we show that ephrin-B2 expressionis upregulated by cocaine and amphetamine in adult mice, suggestingthat ephrin-B2/EphB1 interaction may play a role in drug-inducedplasticity in adults aswell.

Key words: axonal guidance; dopaminergic pathways; Eph family receptors; ephrins; drug addiction; plasticity

  INTRODUCTION

Top
Abstract
Introduction
References

The midbrain dopaminergic neurons are located primarily in two adjacent regions, the more lateral substantia nigra and themore medial ventral tegmental area, and project to the forebrain,forming several distinct pathways (Ungerstedt, 1971; Moore andBloom, 1978; Lindvall and Bjorklund, 1983; Di Chiara et al., 1992;Heimer et al., 1995). Ventral tegmental dopaminergic neurons sendtheir axons to the ventromedial striatum (which includes nucleusaccumbens and olfactory tubercle), constituting the mesolimbicpathway, and to the cortex (mesocortical pathway) (Simon et al.,1976, 1979; Nauta et al., 1978; Beckstead et al., 1979). In contrast,substantia nigra dopaminergic neurons selectively project to dorsolateralstriatum (caudate putamen) in an orderly medial-to-lateral arrangement,forming the nigrostriatal pathway (Carter and Fibiger, 1977; Fallonet al., 1978; Nauta et al., 1978; Beckstead et al., 1979; vander Kooy, 1979). Although these pathways have been identifiedfor nearly three decades, the underlying molecular mechanismsfor the development of these distinct pathways are stillunknown.

The Eph family receptor tyrosine kinases and their ligands have been implicated in guiding axons during the development ofthe nervous system (for review, see Harris and Holt, 1995; Tessier-Lavigne,1995; Friedman and O'Leary, 1996; Orioli and Klein, 1997; Pasquale,1997; Flanagan and Vanderhaeghen, 1998; Zhou, 1998). The Eph familyis the largest known group of receptor tyrosine kinases, includingat least eight ligands and 14 receptors (Zhou, 1998). This familyis unique among tyrosine kinase receptors in that all of the ligandsare membrane-anchored and in that the association is requiredfor activity (Davis et al., 1994). The soluble ligands lack biologicalactivity and can function as antagonists (Gao et al., 1996). Therequirement of membrane anchorage makes the Eph family ligandsuniquely qualified as local guidance cues for axonaltargeting.

In vivo and in vitro observations indicate that the Eph family ligands and receptors play key roles in the specification oftopographic projections. In the retinotectal and hippocamposeptalsystems, Eph family ligands and receptors are expressed in projectingand target fields in opposing gradients (Cheng et al., 1995; Drescheret al., 1995; Gao et al., 1996; Zhang et al., 1996). Consistentwith the expression patterns, ligand-receptor interactions repeland/or inhibit the growth of receptor-positive axons, thus contributingto the specification of topographic projection maps (Drescheret al., 1995; Gao et al., 1996, 1998; Nakamoto et al., 1996).

To examine the roles of the Eph family ligands and receptors in the development of the ascending midbrain dopaminergic pathways,we investigated the developmental expression of these guidancemolecules in the dopaminergic neurons and their projection targets,including the caudate putamen, nucleus accumbens, and olfactorytubercle. We further examined the biological effects of the Ephligands on dopaminergic neurons and their regulation by cocaineand amphetamine in vivo. Our studies indicate that the Eph familyreceptors and ligands may play important roles in regulating theformation of distinct dopaminergic pathways and may contributeto drug-induced neuralplasticity.

  MATERIALS AND METHODS

Animals and preparation of tissue sections. CD-1 mice from embryonic day (E) 14 to postnatal day (P) 60 (adult) were usedin in situ hybridization experiments. The day of vaginal plugoccurrence was defined as E1 and the day of birth as P1. At leastthree animals were investigated at each age group. Whole embryosand brains of postnatal mice were dissected under carbon dioxideanesthesia and frozen on dry ice. Coronal and sagittal sectionsof 16 µm thickness were cut on a cryostat at $-$ 23°C and mountedon slides coated with 2% triethoxy-3-aminopropyl saline (Sigma,St. Louis, MO). Then the slides were stored at $-$ 80°C beforeuse.

In situ hybridization. mRNA expression was detected with either [³⁵S]-labeled in vitro transcribed riboprobes or end-labeled oligonucleotideprobes. In situ hybridization was performed as described (Zhanget al., 1997). The optimal exposure time of hybridized sectionsto autoradiographic emulsion was determined by exposing the sectionsto x-ray film for various time periods before dipping. For quantitativein situ hybridization, complete sets of brain sections from differentage or treatment groups were analyzed in the same experiment withthe same probe. Different samples were compared only within thesameexperiment.

Developmental expression of nine Eph family tyrosine kinase receptors was investigated via in situ hybridization. Only EphB1showed specific differential expression in the midbrain dopaminergicneurons. EphB1 mRNA was detected with a riboprobe transcribedin vitro from a 2.4 kb mouse EphB1 cDNA containing most of thecoding region cloned in a pBluescript SK plasmid. Antisense riboprobewas synthesized with T7 RNA polymerase for hybridization, anda sense control probe was generated with T3 RNA polymerase. Thesynthesized riboprobes were hydrolyzed to smaller fragments (~0.2kb) by 0.2 M bicarbonate at 60°C for 41.6 min beforehybridization.

To examine the expression of the ligands of EphB1, we performed in situ hybridization analyses with probes of all three ephrin-Bligands. Only ephrin-B2 showed differential expression in thedopaminergic target fields. Ephrin-B2 mRNA was detected with ariboprobe made from a 1 kb human ephrin-B2 cDNA containing thefull coding region in pBluescript SK. Human ephrin-B2 has a 93% homology with mouse ephrin-B2 in thenucleotide level (Bergemann et al., 1995; Cerretti et al., 1995).

Quantitative analysis of EphB1 hybridization signals in the midbrain dopamine system and of ephrin-B2 signals in the striatumwas performed with ImagePro 1.3 image analysis software. To avoidbias introduced by the variations of cell density in differentregions, we quantitated only areas with comparable cell densityfor silver grain density, expressed as a percentage of the areacovered by silver grains (area fraction analysis). For each experimentalgroup, hybridization and measurements were done on three animalsand on both sides of the regions of interest over multiple sectionscovering the entire anterior-posteriorextension.

6-Hydroxydopamine treatment. Five late-pregnant CD-1 mice obtained from Charles River Laboratories (Wilmington, MA) were housedindividually in pan cages until pups were born. On day 3 of life,pups in all groups were given a subcutaneous injection of 25 mg/kgpargyline plus 25 mg/kg imipramine (Sigma). Under surgical anesthesia60 min later the pups were injected in the left ventricle with50 or 100 µg of 6-hydroxydopamine base dissolved in 5 µl of 0.1%ascorbic acid. On day 6 the procedure was repeated with the samedose in the right ventricle. Ventricle position was determinedas ± 1.0 mm medial/lateral from bregma and $-$ 2.5 mm ventral tothe skull surface. Pups then were allowed to recover for 10 d,at which time they were killed. For EphB1 in situ hybridizationanalysis the whole brain was dissected and frozen on dry ice.For neurochemical analysis, separate animals were killed, andthe striatum was dissected and frozen in liquid nitrogen untilassay.

Levels of dopamine and the metabolites dihydroxyphenylacetic acid (DOPAC) and homovanillic acid (HVA) were determined by usingHPLC, as described previously (Halladay et al., 1998).

Construction of ephrin-B2-expressing cell line. Human full-length ephrin-B2 was cloned into a retroviral vector pLIG, whichcontains a $beta$ -galactosidase gene fused to an aminoglycoside phosphotransferasefor G418 resistance (Lillian, 1996). Then the construct was transfectedinto National Institutes of Health-3T3 (NIH-3T3) cells. G418-resistantcolonies were screened for ephrin-B2 expression, using immunocytochemicalstaining with polyclonal anti-ephrin-B2 antibody (Santa Cruz,CA). Positive stainings were found in the ephrin-B2-transfectedcells. In contrast, no significant staining was observed in parentalor vector-transfected NIH-3T3cells.

Neuron culture and staining. The substantia nigra and ventral tegmental area of E18 rat embryos were dissected from the lateraltwo-thirds and the medial one-third of the ventral mesencephalon,respectively, under a microscope in PBS. The precise positionsof substantia nigra and ventral tegmental area were determinedby tyrosine hydroxylase (TH) immunohistochemical staining of E18rat midbrain sections. Neurons then were dissociated and coculturedwith monolayer control NIH-3T3 cells or ephrin-B2-expressing fibroblastsin DMEM supplemented with fetal bovine serum (10%), penicillin(50 U/ml), and streptomycin (50 µg/ml). Neurons were culturedfor various times and stained with a monoclonal anti-TH antibody(Chemicon, Temecula, CA). The number of neurons and the lengthsof neurites were measured with a Zeiss Telaval 31 microscope (Oberkochen,Germany). For quantitation of each sample, 20 random fields werechosen from top to bottom and from the left to right sides ofculture wells to represent the entireculture.

Drug treatment. From 30 to 180 mg/kg body weight of cocaine or D-amphetamine was injected subcutaneously in the neck of micein four divided doses over 6 hr. The mice were killed 6 hr or1, 4, 7, or 14 d after treatment, and the expression of ephrin-B2in the striatum was analyzed with in situhybridization.

  RESULTS

Expression of Eph family receptor EphB1 in the midbrain dopaminergic neurons

To examine the roles of the Eph family receptors in the development of the midbrain dopaminergic system, we investigated theexpression of nine Eph family receptors that have been shown tobe transcribed in the nervous system (for review, see Zhou, 1998),using in situ hybridization in P7 mouse brain. These studies showedthat seven Eph receptors, EphA3, EphA4, EphA6, EphA7, EphA8, EphB2,and EphB3, were not expressed at significant levels in the midbraindopaminergic neurons (Table 1). One receptor, EphA5, was transcribedat moderate levels in both the substantia nigra and the ventraltegmental area, consistent with a previous report (Maisonpierreet al., 1993) (Table 1). Only the remaining receptor, EphB1,was transcribed differentially in the ventral mesencephalon (Fig.1). EphB1 expression was restricted primarily to the substantianigra. Few transcripts were detected in the ventral tegmentalarea. Although thionine staining showed a comparable cell density(Fig. 1A), the hybridization signals were significantly higher(~4.8-fold) in the substantia nigra than in the ventral tegmentalarea (Figs. 1B, 2). The difference in EphB1 expression was notattributable to the lack of dopaminergic neurons in the ventraltegmental area, because TH immunohistochemical staining usingneighboring serial sections showed that the enzyme was found inboth the substantia nigra and the ventral tegmental area (Fig.1C).


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Table 1. Expression of Eph family receptors in the P7 midbrain dopamine neurons

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Figure 1. Complementary expression of the Eph family receptor EphB1 and ligand ephrin-B2 in the ascending mesencephalic dopamine systems. A, B, Bright- and dark-field photomicrographs, respectively, of a coronal section of a P2 mouse brain through the ventral mesencephalon hybridized with an antisense EphB1 probe. Hybridized sections were counterstained with thionine to identify the histological patterns. C, Photomicrograph of a neighboring section stained with anti-tyrosine hydroxylase (TH) immunocytochemistry to reveal the substantia nigra and ventral tegmental area. Note that TH staining was observed in both the substantia nigra and the ventral tegmental area, indicating the presence of dopaminergic neurons in both areas. D, E, Bright- and dark-field photomicrographs, respectively, of a P7 coronal mouse brain section through the striatum hybridized with an antisense ephrin-B2 riboprobe and counterstained with thionine. The circled areas are quantitated in Figure 2. ac, Anterior commissure; cc, corpus callosum; LCP, lateral caudate putamen; LS, lateral septum; LV, lateral ventricle; MCP, medial caudate putamen; NA, nucleus accumbens; OT, olfactory tubercle; PC, piriform cortex; SN, substantia nigra; VTA, ventral tegmental area. Scale bars, 0.46 mm.

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Figure 2. Quantitation of the expression of EphB1 in the midbrain and ephrin-B2 in the striatum. The areas quantitated are indicated in Figure 1. The data presented are the averages of expression levels from three different animals (±SEM; *p < 0.02; ANOVA). LCP, Lateral caudate putamen; MCP, medial caudate putamen; NA, nucleus accumbens; OT, olfactory tubercle; SN, substantia nigra; VTA, ventral tegmental area.

To demonstrate further that the Eph receptor was expressed in the dopaminergic neurons, we examined the levels of EphB1 expressionin neonatal mice treated with 6-hydroxydopamine, which selectivelydestroys dopamine neurons (Stodgell et al., 1998). The extentof lesion was confirmed by significant decreases in the levelsof dopamine and its metabolites, DOPAC and HVA, in the striatum(Fig. 3A). In situ hybridization analysis showed that the decreasein the levels of dopamine and its metabolites was paralleled bya decrease in EphB1 expression levels in the substantia nigra(Fig. 3B). Thus, EphB1 mRNA is transcribed selectively in thesubstantia nigra dopaminergic neurons. The expression was observedin E18, the earliest stage examined in this study, and persiststhrough adult, although higher levels were found from E18 to P7(Table 2).

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Figure 3. Reduction of EphB1 expression in the substantia nigra by 6-hydroxydopamine. A, Reduction of the levels of dopamine and the metabolites (DOPAC and HVA) in the striatum of 6-hydroxydopamine-lesioned mice. The data collected are from two animals for each treatment. B, Reduction of EphB1 hybridization signals in the 6-hydroxydopamine-lesioned substantia nigra. The experiments were repeated three times, and two animals were used in each experiment. *p < 0.02; ANOVA.


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Table 2. Developmental expression of EphB1 and ephrin-B2 in the ascending midbrain DA systems

Expression of Eph family ligand ephrin-B2 in the striatum

EphB1-positive substantia nigra neurons are known to project to the caudate putamen, but not to the nucleus accumbens andolfactory tubercle. In contrast, the EphB1-negative ventral tegmentalarea dopaminergic neurons project primarily to the nucleus accumbensand olfactory tubercle. To test the possibility that the receptorEphB1 and its ligands contribute to target specificity of themidbrain dopaminergic neurons, we examined the expression patternsof all of the ephrin-B subclass ligands, ephrin-B1 to ephrin-B3,in the target regions of these neurons. In situ hybridizationstudies showed that only ephrin-B2 was expressed at high levelsin the striatum. The highest levels of expression were detectedin the nucleus accumbens and olfactory tubercle (the ventromedialstriatum) (see Figs. 1D,E, 2). Only very low levels were foundin the caudate putamen. Thus, ephrin-B2 mRNA was differentiallyexpressed in the striatum. Ephrin-B2 expression in the ventromedialstriatum was detected at low levels at E18 to P1 and reached thehighest level at approximately P7 (Table 2). Low levels of expressionpersisted in adult (Table 2). These observations indicate thatephrin-B2 expression is complementary to that of EphB1, suggestingthat the ligand-receptor interaction may restrict the substantianigra dopaminergic neurons from projecting to the ligand-richareas, such as the nucleus accumbens and olfactorytubercle.

Ephrin-B2 selectively inhibits neurite outgrowth of the substantia nigra, but not the ventral tegmental area, dopaminergic neurons

The hypothesis that negative interaction between EphB1 and ephrin-B2 serves to restrict substantia nigra dopaminergic neuronsfrom projecting to nucleus accumbens is consistent with knownfunctions of the Eph ligands. This hypothesis predicts that axonalgrowth from substantia nigra, but not from the ventral tegmentalarea, is inhibited by ephrin-B2. To test this prediction, we examinedthe effect of ephrin-B2 on dopaminergic neurite outgrowth witha coculture assay. In this assay, ephrin-B2 was stably expressedon the surface of NIH-3T3 cells, because the biologically activeligands require membrane anchorage. Dopaminergic neurons fromthe substantia nigra and ventral tegmental area of E18 rat embryonicbrain were dissected and overlaid on a confluent monolayer ofcontrol or ephrin-B2-expressing cells. Dopaminergic neurons weredetected with TH immunocytochemical staining after 2 d in culture.These studies showed that the ventral tegmental dopaminergic neuronsgrew long neurites on both the control and the ephrin-B2-expressingcells (Fig. 4A,B). However, neurite outgrowth from substantianigra dopaminergic neurons was reduced significantly on ephrin-B2-expressingcells (Fig. 4C), although these neurons grew well on the controlcells (Fig. 4D). The average neuritic length of the substantianigra neurons on ephrin-B2 cells was only 50% of that on controlcells (Fig. 5A). The inhibition was observed throughout the lengthdistribution; for example, >70% of substantia nigra axons on controlcells were longer than 100 µm. In contrast, only ~19% of the substantianigra axons were longer than 100 µm when they were coculturedwith ephrin-B2-expressing cells (data not shown). No significantinhibition on ventral tegmental dopaminergic neurite outgrowthwas observed (Fig. 5A).

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Figure 4. Ephrin-B2 inhibits the neurite outgrowth of rat E18 substantia nigra neurons. Medial (ventral tegmental area) or lateral (substantia nigra) mesencephalic dopaminergic neurons were dissected and cocultured with a confluent monolayer of ephrin-B2-expressing cells for 48 hr. Dopaminergic neurons were detected by immunocytochemical staining with an anti-TH antibody. A, B, Ventral tegmental dopaminergic neurons cocultured with ephrin-B2-expressing or control cells, respectively. C, D, Substantia nigra DA neurons cultured on the ephrin-B2-expressing or control cells, respectively. E, F, Substantia nigra dopaminergic neurons cultured on ephrin-B2-expressing or control cells in the presence of 6 µg/ml of ephrin-B2-Fc. Dopaminergic neurons are stained darkly. Ephrin-B2-expressing or control NIH-3T3 cells appear as faintly stained background. Scale bar, 30 µm.

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Figure 5. Quantitative analysis of ephrin-B2 effects on the mesencephalic dopaminergic neuritic outgrowth. A, Average neuritic length of the ventral tegmental (VTA) and substantia nigra (SN) dopaminergic neurons cocultured with ephrin-B2-expressing or control cells. The data shown are the averages of neuritic length (±SEM). The number of neurites quantitated is indicated above each column. Data were collected from six independent experiments. The difference in the neuritic length of substantia nigra neurons between the control and ephrin-B2-expressing cells is significant (Student's t test; p < 0.005). B, Soluble ephrin-B2 reduces the inhibitory effect on substantia nigra DA neurite outgrowth by ephrin-B2-expressing cells. Dopaminergic neurons were cocultured with the ephrin-B2-expressing cells in the presence of various concentrations of the soluble ligand as indicated. Neuritic length was measured and tabulated as in A. The data presented are from four independent experiments. Note that the soluble ligand increases the length of DA neurites in a dose-dependent manner. *p < 0.001; ANOVA.

It has been shown previously that soluble Eph ligands are antagonists for native membrane-bound ligands (Gao et al., 1996).To examine the specificity of inhibition, we added soluble ephrin-B2to the coculture. The presence of soluble ligand reduced the inhibitiveeffects of ephrin-B2 on neurite outgrowth in a dose-dependentmanner (Figs. 4E, 5B). The presence of 6.0 µg/ml soluble ephrin-B2in large part reversed the inhibition on the substantia nigraneurite outgrowth by ephrin-B2, indicating that the inhibitionis specific. Thus, the interaction between EphB1 and ephrin-B2resulted in selective inhibition of neurite outgrowth from thesubstantia nigra dopaminergic neurons, which express high levelsof EphB1, but had no effect on the ventral tegmental area neurons,which express only low levels of thereceptor.

Induction of cell loss of the substantia nigra dopaminergic neurons by ephrin-B2

In addition to the inhibition of neurite outgrowth of the substantia nigra neurons, ephrin-B2 induced a significant decreaseof the substantia nigra neuron number in the coculture (Fig. 6A).In the presence of ephrin-B2 the number of the tyrosine hydroxylase-positivesubstantia nigra neurons was only 41% of that in the control.However, there was no significant reduction in the number of ventraltegmental dopaminergic neurons when they were cocultured withephrin-B2-expressing cells, as compared with control cells (Fig.6A). The reduction in dopaminergic neuron number on ephrin-B2-expressingcells was not attributable to a decrease in adhesion, becausethe number was similar to the control after 12 hr of coculture(Fig. 6B). However, significant neuron loss was apparent by 48hr of culture. By 72 hr, only 57% dopaminergic neurons survived,in comparison with an 80% survival rate on control cells (Fig.6B). Furthermore, soluble ephrin-B2 increased the substantia nigradopaminergic neuron number in a dose-dependent manner (Fig. 6C).To examine whether the decrease in cell number was attributableto apoptosis, we added methylated Boc-Asp-FMK (BAF; Enzyme SystemProducts, Livermore, CA), a general caspase inhibitor, to theculture medium. BAF significantly increased both the survivalrate and the neuritic length of the substantia nigra dopaminergicneurons (Fig. 7). These observations suggest that ephrin-B2 notonly inhibits the growth of neurites from the substantia nigradopaminergic neurons but also induces the loss of these neurons.

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Figure 6. Selective induction of the cell death of the substantia nigra dopaminergic neurons by ephrin-B2. Ventral tegmental (VTA) or substantia nigra (SN) mesencephalic neurons were dissected and cocultured with control or ephrin-B2-expressing cells. After various times of coculture the cells were fixed and stained with anti-TH antibody to identify the dopaminergic neurons. A, Ephrin-B2 decreases the survival of the substantia nigra dopaminergic neurons. The cocultures were maintained for 48 hr in this set of six experiments. The difference in the substantia nigra neuron number between control and ephrin-B2 cultures is significant; *p < 0.01; Student's t test. B, Time course of neuronal loss. The differences in the neuron number between control and ephrin-B2 cultures at 48 and 72 hr are significant (three experiments; *p < 0.05; Student's t test). C, Inhibition of cell death by a specific ligand antagonist: the soluble form of ephrin-B2. Neurons were cocultured for 48 hr. The data presented represent the average of four different experiments (±SEM). The differences among the number of TH-positive neurons cocultured with ephrin-B2-expressing cells in the presence of 0, 3, or 6 µg/ml soluble ephrin-B2 are significant. *p = 0.001; ANOVA.

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Figure 7. An apoptosis inhibitor, Boc-Asp-FMK (BAF), reduces the inhibitory effects of ephrin-B2. Substantia nigra DA neurons were cocultured with ephrin-B2-expressing cells or control NIH-3T3 cells in the presence of various concentrations of BAF. After 48 hr of coculture the DA neurons were detected with anti-TH antibody and quantitated for the number of surviving neurons and the lengths of neurites. A, BAF increases the number of TH-positive neurons. B, BAF increases the average neuritic length. The number of neurites quantitated is indicated above each column. C, Neuritic length distribution in the presence of BAF. The distribution was plotted with data from B. The Control represents the neurite length distribution of substantia nigra DA neurons grown on control-transfected NIH-3T3 cells. The absence of BAF (0 µM) on ephrin-B2-transfected cells represents the condition in which the most potent inhibition of neurite outgrowth was obtained. The data presented are the average of three separate experiments. *p < 0.001; ANOVA.

Induction of ephrin-B2 expression in the striatum by addictive drugs

Our observations indicate that ephrin-B2 and EphB1 may regulate the development of the ascending midbrain dopaminergic pathwaysby negatively regulating neurite outgrowth and survival of theEphB1-positive neurons in the substantia nigra. To examine potentialroles in plasticity of the dopaminergic systems, we analyzed theeffects of acute treatment of drugs of addiction. Subcutaneousinjection of a total of 120 mg/kg cocaine or D-amphetamine dramaticallyinduced ephrin-B2 expression in the striatum (Fig. 8). Ephrin-B2induction by cocaine was dose-dependent, reaching a saturationconcentration at 120 mg/kg (total dose) (Fig. 9A). Quantitativeanalyses indicated that the induction appeared to be strongerin the nucleus accumbens, moderate in medial caudate putamen,and lowest in lateral caudate putamen (see Fig. 8D). The inductionwas evident by 6 hr and reached the highest level by 24 hr afterinjection (Fig. 9B). The level of ephrin-B2 decreased slowly ascompared with that of the control over a period of 7 d after thefirst 24 hr. Similar results have been obtained with mice treatedwith amphetamine (see Fig. 8D). The ability of addictive drugssuch as cocaine and amphetamine to induce the expression of ephrin-B2indicates that the Eph family ligand also may play a role in plasticityof the adult midbrain dopaminergic pathways.

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Figure 8. Induction of ephrin-B2 in the striatum by cocaine and amphetamine. Adult mice were injected subcutaneously with a total dose of 120 mg/kg cocaine or D-amphetamine. The mice were killed 24 hr later and analyzed for ephrin-B2 expression with in situ hybridization. Four striatal areas, the nucleus accumbens (NA), medial caudate putamen (MCP), lateral (LCP) caudate putamen, and the olfactory tubercle (OT), were quantitated. A, B, Bright- and dark-field photomicrographs, respectively, of a control (saline-injected) adult mouse brain section through the striatum hybridized with an antisense ephrin-B2 probe. C, Dark-field photomicrograph of an ephrin-B2-hybridized section through the striatum of a cocaine-treated (24 hr after treatment at 120 mg/kg total dose) adult mouse brain. D, Quantitative analysis of ephrin-B2 induction by cocaine and amphetamine. The hybridization signals were measured for the percentage of the area covered by the silver grains. The data presented represent the average of three different animals in each experimental group. The areas quantitated are indicated in Figure 1D. The differences in signal density between control and drug-treated animals are significant. *p < 0.001; **p < 0.05; ANOVA. ac, Anterior commissure; cc: corpus callosum; Ctx, cerebral cortex; LV, lateral ventricle. Scale bar, 0.62 mm.

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Figure 9. Dose-response and time course of ephrin-B2 induction by cocaine. A, Dose-response of ephrin-B2 induction. Different doses of cocaine (30-180 mg/kg) were injected subcutaneously (in four divided doses). At 24 hr after injection the mice were killed and analyzed for ephrin-B2 expression, as in Figure 8. The nucleus accumbens showed the highest level of induction. B, Time course of ephrin-B2 induction. Mice treated with 120 mg/kg cocaine (total dose) were killed at various times, as indicated, for analysis of ephrin-B2 expression as in A. The data for each dose or time point represent the average of three different animals in the same treatment group. Animals for each experiment were examined in the same in situ analysis with the same riboprobe. LCP, Lateral caudate putamen; MCP, medial caudate putamen; NA, nucleus accumbens; OT, olfactory tubercle. *p < 0.001; **p < 0.005; ANOVA.

  DISCUSSION

The current study has examined the roles of a specific Eph ligand and receptor in regulating the axonal growth of developingdopaminergic neurons from the ventral mesencephalon. Our resultsshow that EphB1 and ephrin-B2 are transcribed in mutually exclusivepatterns in different dopaminergic neuronal populations and theirtargets, constituting distinct neural pathways. Furthermore, ephrin-B2specifically inhibits axonal growth and induces cell loss of thereceptor-rich substantia nigra dopaminergic neurons while havingno negative effects on the ventral tegmental area neurons. Theseobservations indicate that ephrin-B2 may function to prevent thesubstantia nigra dopaminergic neurons from innervating the ligand-richventromedial striatum by inhibitory interactions, thus contributingto the specification of distinct neural pathways. We further reportthat addictive drugs, cocaine and amphetamine, induce ephrin-B2expression in adult striatum. These observations together suggestthat the Eph family ligand and receptor may participate both inthe elaboration of dopaminergic circuits during development andin drug-induced plasticity inadult.

EphB1 and ephrin-B2 expression and the ascending dopaminergic pathways

A large body of evidence indicates that the mesolimbic pathway plays a key role in the motivational aspects of drug addictionas well as emotions and goal-oriented behavior in general (Koob,1992; Self and Nestler, 1995; Hyman, 1996). In contrast, the nigrostriatalpathway appears to be essential for motor functions (Di Chiaraet al., 1992), the degeneration of which is a hallmark of Parkinson'sdisease. The correlation of the topographic distribution of dopaminergicaxon terminals in the striatum and the functional differentiationof the psychological and motor functions suggests that the topographicarrangement is critical to the functions of the midbrain dopaminergicsystems.

Although it has been known for nearly 30 years that the ascending midbrain dopaminergic neurons project to their striataltargets in a topographic manner, the signals regulating the projectionhave not been identified. In this study we show that EphB1, areceptor of the Eph family, is expressed at high levels in thesubstantia nigra but at low levels in the ventral tegmental area.Complementary to EphB1 expression, ephrin-B2, a ligand of thereceptor (Bergemann et al., 1995; Cerretti et al., 1995; Brambillaet al., 1996), is transcribed at high levels in the ventromedialregion of the striatum, including the nucleus accumbens and olfactorytubercle, but at low levels in the dorsolateral striatum. Thus,substantia nigra dopaminergic neurons expressing high levels ofthe receptor EphB1 project to the dorsolateral striatum, whichexpresses low levels of the ligand ephrin-B2. Conversely, ventraltegmental neurons, which express low levels of the receptor, projectto the ventromedial striatum, including the nucleus accumbensand the olfactory tubercle, where high levels of ephrin-B2 aretranscribed (Fig. 10). The complementary expression of receptorand ligand in presynaptic and postsynaptic fields is reminiscentof the complementary expression of other Eph receptors and ligandsin retinotectal system and hippocamposeptal system and is consistentwith their known roles as negative guidance cues in topographicmap formation (for review, see Pasquale 1997; Flanagan and Vanderhaeghen,1998; Zhou, 1998) (also see Cheng et al., 1995; Drescher et al.,1995; Nakamoto et al., 1996; Monschau et al., 1997; Frisén etal., 1998).

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Figure 10. Schematic representation of the relationship between EphB1-ephrin-B2 expression and the topographic projection pattern of midbrain dopaminergic neurons to the striatal targets. In the central dopaminergic system EphB1 was detected at high levels (shown in red) in the substantia nigra (SN). In contrast, little expression was observed in the ventral tegmental system (VTA), which also contains large numbers of dopaminergic neurons. Complementary to EphB1 expression, its ligand, ephrin-B2, is expressed in the developing striatum at high levels (shown in blue) in the nucleus accumbens and olfactory tubercle, the ventromedial regions of the striatum, with only low levels of expression in the dorsolateral region, the caudate putamen (CP). We hypothesized that the interaction between EphB1 and ephrin-B2 may result in an inhibitive signal (indicated by an X) to restrict substantia nigra axons from innervating the ventromedial striatum, thus contributing to the establishment of the mesostriatal and mesolimbic pathways.

Ephrin-B2 regulates neurite outgrowth and cell survival of dopaminergic neurons

The prediction of growth-inhibiting effects of ephrin-B2 on substantia nigra neurons that are EphB1-positive is supportedby in vitro assays in this study. Neurite outgrowth of substantianigra dopaminergic neurons is inhibited by ephrin-B2. In contrast,the growth of ventral tegmental dopaminergic neurons, which normallyproject to the ligand-rich nucleus accumbens and olfactory tubercle,is not affected. These observations provide further support tothe notion that the ligands of the Eph family establish inhibitorydomains in the nervous system to prevent inappropriate innervation(Drescher et al., 1995; Gao et al., 1996, 1998; Nakamoto et al.,1996; Monschau et al., 1997; Frisén et al., 1998).

Interestingly, in the coculture assay, ephrin-B2 also induces a significant loss of dopaminergic neurons from the substantianigra, but not from the ventral tegmental area. There are at leasttwo possible explanations for the cell loss. Reduction of cellnumber could be attributable to a decrease in adhesion becauseof the reduction in neuritic length by ephrin-B2. Alternatively,ephrin-B2 induces the death of substantia nigra dopaminergic neurons.We consider the first explanation unlikely for the following reasons:(1) at 12 hr of culture the number of neurons on ephrin-B2-expressingand control cells is comparable, although neurites are very shortat this time; (2) in our previous study (Gao et al., 1996), hippocampalneurons lacking neurites (because of inhibition by ephrin-A2)do not detach from underlying cells; (3) ventral spinal cord neuronsundergo apoptotic cell death in the presence of ephrin-A5, asrevealed by both cell counts and TUNEL labeling (Y. Yue and R.Zhou, unpublished data). Thus, the reduction of the number ofsubstantia nigra dopaminergic neurons is likely attributable tocell death induced by ephrin-B2. Although much remains to be doneto establish a role of ephrin-B2 in inducing apoptotic cell death,the fact that Boc-Asp-FMK (BAF), a general apoptosis inhibitor,increases cell survival is consistent with this proposal. Furthermore,the anti-apoptotic gene bcl-2 has been shown to promote axon regeneration(Chen et al., 1997), suggesting that molecules regulating celldeath may regulate axonal growthalso.

Earlier studies of the retinotectal development demonstrate that the maturation of the retinotectal map is accompanied bythe death of retinal ganglia cells (Rager and Rager, 1976, 1978;Hughes and McLoon, 1979; McLoon and Lund, 1982; Jenkins and Straznicky,1986). Although it has been proposed that an insufficient numberof trophic factors present in the targets or the inability toform appropriate synaptic connections may be responsible for ganglioncell death (Hughes and McLoon, 1979), our observations raise thepossibility that the interaction between the Eph ligands and receptorsalso may play a role in eliminating mistargeted cells during thedevelopment of topographicmaps.

The timing of expression of the ligand-receptor pair is consistent with a function in establishing target specificity of dopaminergicneurons. Dopaminergic innervation occurs primarily in the first4 postnatal weeks (Loizou, 1969, 1972; Coyle and Axelrod, 1972;Olson et al., 1972; Seiger and Olson, 1973). High differentialexpression of both the ligand and the receptor was observed inthe early postnatal period, and peak ligand expression was foundin the P7 nucleus accumbens (Table 2). Thus, ephrin-B2 and EphB1may participate in the specification of distinct dopaminergicpathways by negatively regulating axonal growth and cell survivalof substantia nigra dopaminergicneurons.

Role of ephrin-B2 in drug-induced plasticity

Our observations that ephrin-B2 is induced by acute administration of cocaine and amphetamine suggest that the Eph ligandmay play a role in drug-induced plasticity. Addictive drugs suchas cocaine, amphetamine, and heroin exert their rewarding effectsof euphoria and pleasure in part via interactions with the dopaminergicsystem. Cocaine, for example, acts by inhibiting the dopaminetransporter and has no effects on knock-out mice lacking the transporter(Giros et al., 1996). It is thought that the reinforcing efficacyof drugs is derived by a release of dopamine into the accumbens,a notion supported by studies in which lesions are made or dopaminergicantagonists are injected in the accumbens (Roberts et al., 1980;Dworkin and Smith, 1987; Koob and Goeders, 1989; Koob, 1992; Robledoet al., 1992). The induction of ephrin-B2 by cocaine and amphetaminein the accumbens is consistent with a role inaddiction.

Drug addiction is thought to reflect plastic changes in the neural circuitry mediating the effect of the drug (Nestler etal., 1993; Hyman, 1996). There are at least two basic mechanismsunderlying plasticity in general. The first is biochemical changesin neurons and related circuits that, in turn, may lead to electrophysiologicalchanges. For instance, upregulation of the cyclic AMP pathwayhas been considered a key event in adaptation to opiates in locusceruleus and to cocaine in the nucleus accumbens (Nestler et al.,1993; Hyman, 1996). The second is structural changes of the synapses,neurons, or pathways involved. It has been shown that chronicmorphine treatment reduces the size of ventral tegmental dopamineneurons (Sklair-Tavron et al., 1996). Growth of new synapses hasbeen demonstrated in long-term memory, associated with rapid andtransient modulations of molecules such as NCAM-related cell adhesionmolecules, which also regulate axonal outgrowth and guidance inthe developing nervous system (for review, see Bailey and Kandel,1995).

Whether changes in neuronal connections are induced by drugs of abuse has not been examined. However, our observation thatthe Eph family ligand ephrin-B2 is upregulated in the dopaminetargets by acute cocaine treatment suggests that modulation ofthe topographic projection of the dopamine system may be a novelmechanism of drug-induced plasticity. Consequently, the ephrin-B2-EphB1interaction may play a role in both the development and plasticityof the dopaminergic brain rewardcircuit.

  FOOTNOTES

Received July 16, 1998; revised Nov. 23, 1998; accepted Dec. 22, 1998.

This research was funded by the National Institute on Drug Abuse (Grant 1RO1DA11480-01) and by an Exploratory Research grantfrom the National Institute of Environmental and OccupationalHealth Sciences. We thank W. Schultz for the critical readingof thismanuscript.
Correspondence should be addressed to Dr. Renping Zhou, Laboratory for Cancer Research, Department of Chemical Biology, Collegeof Pharmacy, Rutgers University, Piscataway, NJ08855.

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