An Evolutionarily Conserved Transmembrane Protein That Is a Novel Downstream Target of Neurotrophin and Ephrin Receptors

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The Journal of Neuroscience, January 1, 2001, 21(1):176-185

An Evolutionarily Conserved Transmembrane Protein That Is a Novel Downstream Target of Neurotrophin and Ephrin Receptors
Haeyoung Kong¹, Jim Boulter², Janet L. Weber³, Cary Lai³, and Moses V. Chao¹
¹ Molecular Neurobiology Program, Skirball Institute for Biomolecular Medicine, New York University School of Medicine, New York, New York, ² Department of Psychiatry and Behavioral Sciences, University of California, Los Angeles, California, and ³ Department of Neuropharmacology, The Scripps Research Institute, La Jolla, California

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Appropriate development of nervous system connectivity involves a variety of processes, including neuronal life-and-deathdecisions, differentiation, axon guidance and migration, and synaptogenesis.Although these activities likely require specialized signalingevents, few substrates unique to these neurotrophic functionshave been identified. Here we describe the cloning of ankyrinrepeat-rich membrane spanning (ARMS), which encodes a novel downstreamtarget of neurotrophin and ephrin receptor tyrosine kinases, Trkand Eph, respectively. The amino acid sequence of ARMS is highlyconserved from nematode to human, suggesting an evolutionarilyconserved role for this protein. The ARMS protein consists of1715 amino acids containing four putative transmembrane domains,multiple ankyrin repeats, a sterile $alpha$ motif domain, and a potentialPDZ-binding motif. In the rat, ARMS is specifically expressedin the developing nervous system and in highly plastic areas ofthe adult brain, regions enriched in Trks and Eph receptors. ARMScan physically associate with TrkA and p75 neurotrophin receptors.Moreover, endogenous ARMS protein is tyrosine phosphorylated afterneurotrophin treatment of pheochromocytoma 12 cells and primaryhippocampal neurons or ephrin B treatment of NG108-15 cells, demonstratingthat ARMS is a downstream target for both neurotrophin and ephrinreceptors.

Key words: neurotrophin; Trk; p75; ephrin; Eph; tyrosine kinase; tyrosine phosphorylation; ankyrin

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The formation of the nervous system requires appropriate connectivity of neurons and their targets both spatially and temporally.Two families of proteins that mediate these actions are the neurotrophinsand ephrins. Neurotrophins play a prominent role in the developmentof the vertebrate nervous system by influencing cell survival,differentiation, and cell death events (Levi-Montalcini, 1987;Lewin and Barde, 1996). Neurotrophins also exhibit acute regulatoryeffects on neurotransmitter release, synaptic strength, and connectivity(Thoenen, 1995; Bonhoeffer, 1996; McAllister et al., 1999). Inaddition to promoting axonal (Patel et al., 2000) and dendriticbranching, neurotrophins serve as chemoattractants for extendinggrowth cones in vitro (Letourneau, 1978; Gundersen and Barrett,1979; Gallo et al., 1997).

Ephrins comprise another class of ligands that function in axon guidance, cell migration, axon fasciculation, boundary formation,topographic mapping, and morphogenesis (Frisén et al., 1999).Ephrins are a family of eight proteins that are found associatedwith the plasma membrane, either via a glycosylphosphatidylinositollinkage (as seen in the A subfamily) or as transmembrane proteins(as seen in the B subfamily). Ephrins signal via receptor proteintyrosine kinases, but the biological outcomes are distinct frommitogenic factors such as platelet-derived growth factor and epidermalgrowth factor (EGF), both of which transmit signals via tyrosinephosphorylation (Brückner and Klein, 1998; Flanagan and Vanderhaeghen,1998; Holland et al., 1998). Ephrin receptor-associated moleculessuch as Crk, Nck, RasGAP, and Fyn are proposed links between thereceptor and downstream events such as cell adhesion and cytoskeletalchanges. In addition, Grb2, Grb10, and the p85 subunit of phosphatidylinositol-3kinase (PI-3 kinase) are used in ephrin receptor signal transduction(Mellitzer et al., 2000).

The neurotrophins [NGF, BDNF, neurotrophin-3 (NT-3), and NT-4/5] exert their effects via two classes of receptors (Kaplanand Miller, 2000). TrkA, TrkB, and TrkC serve as receptor tyrosinekinases for NGF, BDNF and NT-4, and NT-3, respectively (Chao,1992a). The p75 receptor is a member of the tumor necrosis factorreceptor superfamily (Smith et al., 1994) and binds to all neurotrophins.Most central and peripheral neurons express p75 together withone or more of the Trks. The p75 receptor, when coexpressed withTrkA, provides a positive influence on Trk function (Barker andShooter, 1994; Verdi et al., 1994) and determines the specificityof neurotrophin binding and responsiveness (Benedetti et al.,1994; Bibel et al., 1999; Brennan et al., 1999). An associationof p75 and Trk receptors has been detected by coprecipitation(Huber and Chao, 1995; Gargano et al., 1997; Bibel et al., 1999),and copatching of these receptors has been observed by the useof fluorescent-labeled antibodies (Ross et al., 1996).

Receptor tyrosine kinases frequently use a number of common intracellular signaling components such as phospholipase C- $gamma$ ,PI-3 kinase, and adaptor proteins such as Shc and Grb2. Commonto many of these proteins is their ability to bind to phosphorylatedtyrosines via domains such as the Src homology-2 (SH2) and phosphotyrosine-binding(PTB) domains. How these shared signaling components lead to differentbiological outcomes is not well understood (Chao, 1992b). Possiblemechanisms include receptor use of substrates in a differentialmanner (e.g., differential association/dissociation kinetics),competition for binding between different substrates (Meakin etal., 1999), or recruitment of unique target proteins, such asrAPS and SH2-B (Qian et al., 1998).

To define proteins associated with the neurotrophin receptors, we used the intracellular domain of the p75 neurotrophin receptoras bait in a two-hybrid screen of a dorsal root ganglion library.Here we report the properties of a novel transmembrane protein,designated ARMS (ankyrin, repeat rich, and membrane spanning),that contains a number of interesting features, including multipleankyrin repeats, four putative transmembrane domains, a sterile $alpha$ motif (SAM) domain, and a consensus PSD95/SAP90, DLG, and ZO1(PDZ)-binding motif. Interestingly, ARMS does not contain SH2or PTB domains, suggesting that it confers signaling specificitydownstream of receptor tyrosine kinases in a manner distinct fromclassical adaptor proteins. An analysis of the structure and distributionof this protein suggests that it may function during developmentof the nervous system. Most importantly, ARMS is phosphorylatedafter treatment with NGF, BDNF, and ephrin B2, suggesting thatit is a critical link between cell surface receptors and intracellularsignaling events for both the neurotrophin and the ephrinfamilies.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Materials. NGF was obtained from Harlan (Indianapolis, IN), BDNF was from Peprotech (Rocky Hill, NJ), NT-4/5 was a generousgift of Regeneron (Tarrytown, NY), EGF was obtained from Intergen(Purchase, NY), and K252a was from Calbiochem (La Jolla,CA).

Construction of the two-hybrid DRG library and yeast two-hybrid screen. A cDNA library was constructed into unique BstXI-NotIsites of a modified version of pJG4-5. Briefly, polyadenylatedRNA, which had been purified from adult mouse and postnatal day1 (P1) rat DRG by the use of Trizol (Life Technologies, Gaithersburg,MD) and the PolyA Tract System (Promega, Madison, WI), was usedas the template for reverse transcription (Life Technologies)with an oligo-dT-NotI primer. Subsequent ligation into pJG4-5and electroporation into DH5 $alpha$ yielded a library of ~10⁶ cfu and an average insert size of 1.5-2.0 kb. A two-hybrid interactionscreen, based on the LexA system (Gyuris et al., 1993), was performedin EGY48. The bait consisted of the entire cytoplasmic regionof rat p75 as an in-frame fusion with the LexA DNA-binding domain.Library cDNAs were expressed as in-frame fusions with the Gal4transcriptional activation domain. Approximately 90 million yeasttransformants were screened for their ability to survive in theabsence of leucine. Sequence analysis identified a novel cDNAclone of ~2.5 kb that corresponded to the C-terminal 250 aminoacids ofARMS.

Isolation of ARMS cDNA. Several rat brain libraries (young adult whole brain, adult whole brain, and adult hippocampus) werescreened to obtain the full-length ARMS cDNA. Criteria used toestablish the initiator methionine include the following: assessmentof multiple, independent cDNA fragments spanning the start site,an upstream, in-frame stop codon, and conformity to the Kozakconsensus sequence. The ARMS sequence has been deposited intothe GenBank database under accession number AF313464.

Northern blotting and in situ hybridization. Total RNA was extracted from various rat tissues using Trizol reagent (Life Technologies).Twenty micrograms of total RNA were loaded per lane (with theexception of pancreas and DRG RNAs, which were <10 µg/lane), electrophoresedthrough a 2.2 M formaldehyde and 1% agarose gel, transferred toa nylon membrane (Qiagen, Santa Clarita, CA), baked for 2 hr at80°C, and probed with a cDNA fragment of ARMS labeled with [³²P]dCTP using Ready-To-Go (Amersham Pharmacia Biotech, Piscataway,NJ). In situ hybridization was performed as described previously(Lai and Lemke, 1991). Briefly, 30 µm paraformaldehyde-fixed brainsections from adult rat or whole embryos were slide-mounted, hybridizedwith a ³³P-labeled cRNA probe generated by T7 RNA polymerase from a PCR-generatedARMS fragment, and washed at a final stringency of 0.1× SSC at60°C for 35 min. Emulsion-dipped slides were exposed for varioustimes (days to weeks) before developing and then counterstainedwiththionin.

Cell culture. Human embryonic kidney (HEK) 293 and 293T cells were maintained in DMEM containing 10% fetal bovine serum (FBS)supplemented with 100 U/ml penicillin, 100 µg/ml streptomycin,and 2 mM glutamine. Native pheochromocytoma (PC) 12 cells, TrkA-overexpressingPC12 cells (615) (Hempstead et al., 1992), and TrkB-overexpressingPC12 cells were maintained in DMEM containing 10% FBS and 5% heat-inactivatedhorse serum with 30 U/ml penicillin, 30 µg/ml streptomycin, 2mM glutamine, and 200 µg/mlG418.

SCG neurons were prepared from P2 rats and cultured on collagen-coated coverslips in C-medium (minimum essential medium containing10% FBS supplemented with 0.4% glucose and 2 mM L-glutamine) with150 ng/ml 2.5 S NGF (Harlan). To inhibit growth of non-neuronalcells, neurons were cultured in the presence of 24.6 mg/ml 5-fluoro-2-deoxyuridineand 24.4 mg/mluridine.

Dissociated primary cultures of hippocampal neurons from embryonic day 17 (E17) rats were prepared from timed-pregnant SpragueDawley rats following published procedures (Aibel et al., 1998).After dissection of the hippocampus, the meninges were removed.The tissue was briefly minced with fine forceps and then trituratedthrough a fire-polished Pasteur pipet. Cells were counted andplated in Neurobasal media supplemented with B27 (Life Technologies)on cell culture dishes coated overnight with 0.01 mg/ml poly-D-lysine.Cells were grown in a humidified incubator with 5% CO₂ at 37°C.

Antibodies. To characterize the expression of the ARMS protein, we generated a polyclonal antibody (892) against the C terminusof ARMS. A bacterially expressed GST fusion protein with the C-terminal180 amino acids of ARMS was purified and used as an antigen togenerate rabbit antiserum (Cocalico Biologicals, Reamstown, PA).The specificity of this antiserum was determined by Western blotanalyses of HEK293T cells transfected with a FLAG-tagged, full-lengthcDNA of ARMS. Lysates of transfected HEK293T cells, but not untransfectedcells, displayed a specific 190 kDa species after immunoblottingwith either an anti-FLAG antibody or anti-ARMS serum892.

Transfection of mammalian cells, immunoprecipitation, and immunoblotting. For transient transfection experiments, HEK293 orHEK293T cells plated at 70-80% confluency in 10 cm dishes weresubjected to calcium phosphate transfection with different combinationsof the mammalian expression plasmids containing cDNAs for ARMS,rat TrkA, and rat hemagglutinin (HA)-tagged p75 (Khursigara etal., 1999). PC12 615 cells or transiently transfected cells wereharvested and lysed in 1 ml of 10 mM Tris, pH 8.0, 150 mM NaCl,1 mM EDTA, and 1% NP-40 (TNE buffer) containing 0.12 mg/ml phenylmethylsulfonylfluoride, 2 µg/ml leupeptin, 1 µg/ml aprotinin, 10 mM NaF, and1 mM Na₃VO₄ for 30 min on ice. After centrifugation and removalof the insoluble fraction, the protein concentration of the supernatantwas determined by the Bio-Rad Protein Assay reagent (Bio-Rad,Hercules, CA) with bovine serum albumin as the standard. Celllysates of equivalent protein content were incubated for 4 hrto overnight with rotation at 4°C with either anti-pan-Trk polyclonalantibody, C14 (1.5 µg), or anti-ARMS 892 antiserum (1:100). Theimmune complexes were immobilized on protein A-Sepharose beads(Sigma, St. Louis, MO), washed six times with ice-cold TNE buffer,boiled in SDS-sample buffer, separated by SDS-PAGE, and transferredonto a polyvinylidene difluoride membrane (Millipore, Bedford,MA). Immunoblotting was performed by first blocking membranesin 20 mM Tris, pH 7.5, 500 mM NaCl, and 0.1% Tween 20 (TBST buffer)containing 5% BSA for pY99 and 5% nonfat milk for others and thenincubating for 2 hr at room temperature or overnight at 4°C inTBST buffer containing one of the following primary antibodies:anti-Trk 44 serum (1:2000); anti-phosphotyrosine pY99 antibody(0.1 µg/ml; Santa Cruz Biotechnology, Santa Cruz, CA); or anti-ARMS892 antiserum (1:1000). Membranes were washed with TBST bufferand then incubated with horseradish peroxidase-conjugated goatanti-rabbit (Roche Molecular Biochemicals, Indianapolis, IN) orgoat anti-mouse secondary antibodies (Jackson ImmunoResearch,West Grove, PA) at a dilution of 1:10,000 or 1:7500, respectively.Immunoreactive protein bands were detected by enhanced chemiluminescenceusing ECL reagents (Amersham PharmaciaBiotech).

Immunofluorescence analysis. SCG neurons were fixed with 4% paraformaldehyde and blocked with PBS containing 0.075% saponinand 10% FBS or normal goat serum. Cells were then incubated withanti-ARMS 892 (1:1000) or anti-Trk B-3 antibody (1 µg/ml) in blockingbuffer. Primary antibodies were visualized using fluorescence-conjugatedsecondary antibodies [indocarbocyanine-conjugated goat anti-mouseIgG (Jackson ImmunoResearch; 1:200) or FITC-conjugated goat anti-rabbitIgG (Jackson ImmunoResearch; 1:100)]. Images were collected ona Bio-Rad confocalmicroscope.

  RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Cloning of ARMS

Neurotrophins exert many biological activities, but few signaling molecules have been found to be specific for neurotrophinreceptor signaling. The majority of proteins that serve as substratesfor neurotrophin receptors are used by other receptor families.Effects on cellular and axonal migration, nerve regeneration,and apoptosis have been implicated for the p75 neurotrophin receptor,and effects on long-term potentiation and synaptic transmissionhave been attributed to the Trks. To define unique molecules inneurotrophin signaling, a two-hybrid screen was undertaken usinga rat dorsal root ganglion library as prey and the cytoplasmicdomain of p75 as bait. This report describes a p75-interactingprotein that is a downstream target for Trksignaling.

A positive cDNA clone was identified that encoded the C-terminal portion of a novel 1715 amino acid protein. The predictedamino acid sequence contained 11 contiguous, 33 amino acid ankyrinrepeats in the N-terminal domain and four putative membrane-spanningregions. We have designated this protein ARMS. The overall topologyof ARMS is decidedly different from that of other transmembraneproteins. Other distinguishing features of this protein includea SAM domain, a polyproline stretch, and a potential PDZ-bindingmotif (Fig. 1A,B). These motifs represent candidate protein-proteininteraction domains.

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Figure 1. ARMS represents a novel transmembrane protein. A, Predicted topology of ARMS. Transmembrane domains (labeled 1-4) and various intracellular motifs are depicted. B, Amino acid sequence and comparison of rat ARMS (rARMS) and human ARMS (hARMS) proteins. Residues marked with a dashed line denote 11 contiguous ankyrin repeats; bold-faced tyrosine (Y) residues (at positions 399, 409, 441, 444, and 466 of the rat sequence) are evolutionarily conserved among human, rat, Drosophila, and C. elegans; boxed residues are the putative transmembrane domains; italicized residues denote the polyproline stretch; shadowed residues constitute the SAM domain (amino acids 1152-1221); and the three carboxymost amino acids marked with asterisks (SIL) encode a potential PDZ-binding motif. Amino acids of the human sequence that differ from the rat sequence are shown. C, Comparison of various cytoplasmic regions of rat (r), human (h), Drosophila (d), and C. elegans (w) ARMS proteins. Part 1, N-terminal region between the ankyrin repeats and the first transmembrane domain with bold-faced evolutionarily conserved tyrosines (Y). Part 2, Cytoplasmic region between transmembrane domains 2 and 3. Parts 3, 4, Two C-terminal regions. Part 5, The SAM domain. Sequences for wARMS, dARMS, and hARMS were obtained from accession numbers Z68760, AAF46710, and BAA86564/CAB63746, respectively. Symbols: asterisk, identity; colon, strongly similar; period, weakly similar.

An extensive search of GenBank databases for proteins similar to ARMS identified many ankyrin-containing proteins; however,proteins sharing homology with ARMS in regions outside of theankyrin repeats were notably absent. Analysis of Caenorhabditiselegans, Drosophila, and human databases revealed ARMS orthologsin these organisms. The presence and conservation of ARMS sequencesfrom nematodes to humans suggest that this protein may serve evolutionarilyconserved functions. Between rat and human, the amino acid identityis 91%, and similarity is 94% (Fig. 1B). Comparison of ARMS sequencesamong human, rat, Drosophila, and C. elegans revealed similarityin overall structure: multiple ankyrin repeats in the N terminus,four putative transmembrane domains, SAM domains, and consensusPDZ-binding motifs at the three carboxymost amino acids (SIL inhuman and rat, TKL in Drosophila, and SDA in C. elegans). Despitethe relatively divergent C termini among the ARMS homologs, thepresence of potential PDZ recognition sequences in all of theseproteins indicates that conserved protein-protein interactionsfor ARMS mayexist.

Interestingly, the regions most highly conserved were not the transmembrane (TM) domains but certain regions surrounding them,namely, the ankyrin repeats, the N-terminal portion between theankyrin repeats and the first TM domain, the "loop" region betweenTM domains 2 and 3, and several stretches of amino acids in theC terminal downstream of TM4, including the SAM domain (Fig. 1C).The regions shown in Figure 1C range between 20 and 42% identicaland 56 and 77% similar, whereas the TM domains are only 1% identicaland 43% similar. It is interesting to note that embedded in thesesubdomains are conserved tyrosine residues; these potential phosphorylationsites are conserved among all four organisms examined (Fig. 1C,part 1). Although mutations in C. elegans and Drosophila ARMShave not yet been described, the C. elegans homolog F36H1.2 ismost similar to the ankyrin-related gene UNC-44 (28%), which hasa role in axon guidance, axonogenesis, and neuronal development(Otsuka et al., 1995).

Distribution of ARMS transcripts in rat

In rat tissue, expression of ARMS mRNA was assessed by Northern blot analysis using a probe directed against the membrane-spanningregions of ARMS (Fig. 2, top). A single transcript of ~7.0 kbwas detected. Although ARMS mRNA could be detected in severalnon-neuronal tissues, it was most abundant in the nervous system.

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Figure 2. Distribution of ARMS mRNA. Top, Northern analysis of ARMS. A single transcript of 7.0 kb was detected by Northern analysis using a ³²P-labeled ARMS cDNA probe (top blot). Each lane contained 20 µg of total RNA (with the exception of the pancreas and DRG lanes that contained <10 µg each) extracted from various rat tissue. Methylene blue staining of the 28 S ribosomal band as a loading control is shown (bottom blot). Middle, Distribution of ARMS mRNA in the adult rat CNS. A ³³P-labeled cRNA probe was used to assess ARMS mRNA expression. Areas of intense labeling include the mitral cell layer of the olfactory bulb (OB), all regions of the hippocampus (HP), the Purkinje cell layer of the cerebellum (CB), and gray matter (most notably in the ventral horn) of the spinal cord (SC). Bottom, Expression in adult rat DRG by in situ hybridization. A ³³P-labeled cRNA probe was used to assess mRNA distribution in DRG as depicted in the dark-field image (left). The majority of cell bodies of the DRG were positive for ARMS mRNA expression, but absences of expression were noted in the large-diameter DRG cell bodies depicted by the arrows in the dark-field and the corresponding phase (right) photographs. Scale bars: white, 1 mm; black, 50 µm.

We examined the expression of ARMS by in situ hybridization in adult rat brain. Several populations of neurons were foundto express ARMS mRNA, including mitral cells and cells of theglomerular layer of the olfactory bulb, all regions of the hippocampus,Purkinje cells of the cerebellum, and gray matter (most notablyin presumed large motor neurons) of the spinal cord (Fig. 2, middle).One shared property of these neuronal populations is their abilityto undergo synaptic changes throughoutadulthood.

During defined periods of rodent embryonic development, subpopulations of sensory neurons require distinct neurotrophins andtheir cognate receptors for survival (Pinon et al., 1996). Theneurotrophin receptor system remains functional through adulthood.Correspondingly, ARMS expression coincides with that of the Trksand p75. As shown by Northern analysis (Fig. 2, top) and in situhybridization (Fig. 2, bottom), ARMS expression persists in theadult DRG. In addition to an absence of silver grains over thenerve fibers, there was a notable absence of ARMS message in asubset of DRG cell bodies corresponding to large-diameter neurons.Although ARMS mRNA can be detected in all populations of DRG neurons,much lower expression in large-diameter neurons suggests a lessprominent role inproprioception.

More striking was the restricted expression of ARMS during development. In general, during rat nervous system development,the period of embryonic growth between E11 and E14 is a time ofmassive proliferation of the neuroepithelium. By E14, the firstsets of postmitotic neurons are undergoing differentiation. InE14 rat embryos, ARMS was expressed in both spinal cord and dorsalroot ganglia (Fig. 3, left). These neuronal populations are amongthe first in the nervous system to undergo differentiation, andit is during this window of development that these postmitoticneurons are actively seeking and making connections with theirtargets. Additionally, several neuroanatomical loci of the developingbrain expressed ARMS mRNA. In the midsagittal plane, the hippocampus,cortex, pons, and medulla were positive for ARMS expression (Fig.3, middle). Regions lateral to the midline such as the basal telencephalon,superior and inferior colliculus, principal trigeminal sensorynucleus, and multiple ganglia, including trigeminal, geniculate,vestibular, and superior cervical (Fig. 3, right), showed significantlevels of ARMS transcripts.

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Figure 3. Expression of ARMS mRNA. In situ hybridization of ARMS in E14 rat. Left, In a coronal section through the midsection of an E14 rat, only spinal cord (sc) and dorsal root ganglion (drg) were positive for ARMS. Middle, Right, In situ hybridization of ARMS in a midsagittal section and a more lateral section, respectively, of E14 rat is shown. ARMS mRNA expression was restricted to various brain regions such as the cortex (cx), hippocampus (hp), pons, medulla (med), basal telencephalon (bt), principal and spinal trigeminal nucleus (tn), superior and inferior colliculus (clc), and sc. Multiple ganglia expressed ARMS mRNA, such as the drg, trigeminal ganglion (tg), geniculate ganglion (gg), vestibular ganglion (vg), and superior cervical ganglion (scg). Scale bars, 1 mm.

Association of ARMS with NGF receptors

Because the ARMS protein was originally identified in a yeast two-hybrid assay from its association with the cytoplasmic domainof the p75 receptor, we tested whether ARMS was capable of aninteraction with p75 in cultured cells. We cotransfected an HA-taggedp75 cDNA and the ARMS cDNA in HEK293T cells. After immunoprecipitationwith an antibody (892) made against the C-terminal region of theARMS protein, the p75 receptor could be readily detected by Westernanalysis (Fig. 4A). This transfection experiment indicated thatARMS and p75 are capable of forming a complex in HEK293T cells.

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Figure 4. Association of ARMS with p75 and TrkA receptors. A, Interaction of p75 with ARMS. HEK293T cells were cotransfected with cDNAs encoding full-length ARMS (ARMS), HA-tagged p75 (HAp75), ARMS plus p75 (HAp75+ARMS), or empty vector (vector). Cells lysates were immunoprecipitated with anti-ARMS 892 antiserum and immunoblotted with anti-HA (top). Expression of p75 receptors was confirmed by immunoblotting with anti-p75 (9992; bottom). B, Coprecipitation of TrkA and ARMS. PC12 615 cells were treated for 10 min (m) and 25 hr (h) with NGF (100 ng/ml). Lysates were prepared and subjected to immunoprecipitation with anti-Trk C14 antibody, followed by immunoblotting with anti-ARMS antibody. Normal rabbit IgG was used as a negative control. The migration of the protein molecular weight standard, 217 kDa, is shown on the left. C, Colocalization of ARMS and TrkA. Immunofluorescence analysis of ARMS and TrkA receptor in sympathetic neurons is shown. SCG sympathetic neurons were grown in the presence of 150 ng/ml NGF, fixed, and immunostained as described in Materials and Methods. The ARMS protein and the TrkA receptor were subjected to double immunostaining using an anti-ARMS antiserum (left) and an anti-Trk B-3 monoclonal antibody (middle) and were analyzed by confocal microscopy. The yellow signal demonstrates overlap of the two signals (overlay; right). The arrow indicates cell surface colocalization of ARMS and TrkA. IP, Immunoprecipitation.

Previous studies indicated that p75 and the TrkA receptor can exist in a complex (Huber and Chao, 1995; Gargano et al., 1997;Bibel et al., 1999). To establish whether an interaction betweenTrkA and ARMS occurs, we performed an immunoprecipitation experimentin PC12 cells expressing elevated levels of TrkA (Hempstead etal., 1992). An NGF-dependent association between ARMS and theTrkA receptor was detected after immunoprecipitation of TrkA andimmunoblotting with the anti-ARMS antibody 892 (Fig. 4B). Theassociation between ARMS and TrkA persisted 25 hr after NGF treatment.The endogenous association of TrkA and ARMS indicates that ARMSmay exist in a ligand-dependent complex with Trkreceptors.

To investigate further the distribution and potential colocalization of ARMS and Trk in neuronal cells, we performed indirectimmunofluorescence experiments in primary cultures of rat sympatheticneurons. Using the 892 antibody against ARMS and a monoclonalantibody directed against Trk, we observed colocalization of ARMSand TrkA on the cell surface of sympathetic neurons (Fig. 4C,arrow). These results support our coimmunoprecipitation studiesthat suggest a physical association between Trk andARMS.

Tyrosine phosphorylation of ARMS by NGF

The high degree of correspondence in the expression of ARMS and neurotrophin receptors and the endogenous association withTrkA receptors led us to postulate that ARMS might function asa target for Trk receptor phosphorylation. To investigate thispossibility, we prepared cell lysates from NGF-treated PC12 cellsand immunoprecipitated the ARMS protein with anti-ARMS antiserum892. Phosphorylation of ARMS protein was visualized by immunoblottingwith an anti-phosphotyrosine antibody, pY99. Tyrosine phosphorylationof ARMS was detectable within a minute of NGF addition (Fig. 5A,top), closely following the time course of TrkA autophosphorylation(Fig. 5A, bottom). With continued NGF treatment, the phosphorylationof ARMS persisted for 25 hr (Fig. 5B). Pretreatment with the alkaloid-likecompound K252a (100 nM), which specifically inhibits NGF-mediatedactivity by selectively blocking the kinase activity of TrkA (Koizumiet al., 1988; Berg et al., 1992), completely abolished the tyrosinephosphorylation of ARMS. Hence, the ARMS protein represents anovel downstream target for the TrkA receptor tyrosine kinase.

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Figure 5. Tyrosine phosphorylation of ARMS. A, Phosphorylation of ARMS by NGF in PC12 cells is rapid and can be blocked by K252a. The antiserum 892 was used to immunoprecipitate endogenously expressed ARMS from PC12 615 cell lysates. Anti-phosphotyrosine antibody pY99 was used to assess tyrosine phosphorylation of the immunoprecipitated ARMS. Within 1 min of NGF treatment, phosphorylated ARMS (pARMS) could be detected, suggesting a direct phosphorylation by TrkA. Furthermore, 100 nM K252a potently blocked ARMS phosphorylation (top). In lysates of the same samples, TrkA autophosphorylation is shown using pY99 (bottom). B, Time course of ARMS phosphorylation by NGF in PC12 cells is shown. The phosphorylation peaks within 10 min and is sustained for at least 25 hr (top). Reprobing of the same blot with 892 demonstrated equivalent levels of immunoprecipitated ARMS from the various lysates (bottom).

To explore the specificity of ARMS phosphorylation, we compared the effects of EGF and NGF in PC12 cells. The phosphorylationof ARMS was considerably more robust after NGF treatment (Fig.6), even though both TrkA and EGF receptors were activated. Thesedata indicate that ARMS phosphorylation was a specific consequenceof NGF, but not EGF, receptor signaling. This may be a consequenceof a lack of association of ARMS with the EGF receptor. It isunlikely that ARMS phosphorylation was mediated via the MAP kinasepathway, because treatment of PC12 cells with EGF showed minimaltyrosine phosphorylation of ARMS after 10 min or 2 hr (Fig. 6).Also, ARMS phosphorylation was not elicited by other growth factors,such as insulin, FGF, and insulin growth factor-1, in PC12 cells(data not shown), indicating that unique proteins are phosphorylatedby the receptor tyrosine kinase TrkA.

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Figure 6. Specificity of ARMS phosphorylation. Top, Phosphorylation of ARMS is specifically induced after NGF, but not EGF, treatment of PC12 615 cells. Two time points, 10 min and 2 hr, were examined for tyrosine phosphorylation of ARMS using the following conditions: no ligand (CTRL), 50 ng/ml EGF, and 100 ng/ml NGF. To demonstrate the specificity of the ARMS antiserum 892 (I), preimmune antiserum (P) was used in parallel immunoprecipitations. Bottom, The amount of ARMS protein that was immunoprecipitated from the various lysates is shown.

Response to other trophic factors and ephrins

To test the ability of other Trk receptors to phosphorylate ARMS, we used PC12 cells stably expressing the TrkB receptor.After treatment of these cells with BDNF (100 ng/ml), ARMS wastyrosine phosphorylated, demonstrating that ARMS can be phosphorylatedby TrkB as well as TrkA (Fig. 7). That expression of ARMS is localizedto some central regions in which TrkA is not expressed, such asthe hippocampus, can be reconciled by the presence of TrkB, whichis widely expressed in the adult CNS and which serves as a receptorfor BDNF and NT-4/5 (Farinas et al., 1998).

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Figure 7. Phosphorylation of ARMS by other neurotrophins. The neurotrophins BDNF and NT-4/5 induce phosphorylation of ARMS via the TrkB receptor. PC12 cells stably expressing TrkB were treated with either 100 ng/ml BDNF or 100 ng/ml NT-4/5, and the phosphorylation of ARMS was measured as described in Figure 5. Top, BDNF and, to a lesser extent, NT-4/5 were able to induce tyrosine phosphorylation of ARMS. Bottom, Immunoprecipitated ARMS from each lysate is shown.

To verify the ability of BDNF to induce phosphorylation of ARMS in neurons, primary cultures of hippocampal neurons were established.Hippocampal neurons express the TrkB receptor. After treatmentwith BDNF, ARMS was immunoprecipitated from hippocampal lysatesand assessed for tyrosine phosphorylation by immunoblotting withan anti-phosphotyrosine antibody. A similar phosphorylation ofARMS after BDNF treatment in hippocampal neurons was observed(Fig. 8). Thus, in a primary neuronal culture, ARMS is a downstreamtarget of TrkB after activation by BDNF.

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Figure 8. Induction of ARMS phosphorylation in hippocampal neurons by BDNF. Primary cultures of E17 hippocampal neurons were prepared and treated with 50 ng/ml BDNF for the indicated times. Top, Phosphorylation of ARMS was assessed by immunoprecipitation with anti-ARMS 892 antiserum and Western blotting with anti-phosphotyrosine pY99 antibody. Bottom, Equal amounts of ARMS protein were immunoprecipitated from each lysate as shown by reprobing the same blot with 892. C, Control.

The expression of ARMS during developmental periods of axon outgrowth and synaptogenesis raises the possibility that ARMSis downstream of other known axon guidance regulators. We thereforeexamined the ephrin family because of its well established invitro and in vivo guidance function. As seen in Figure 9A, theARMS protein is potently tyrosine phosphorylated by ephrin B2in a neuronal/glioma hybridoma cell line, NG108-15, that stablyexpresses EphB2 receptor. EphB2 receptor autophosphorylation andactivation occur over a time period of 30-40 min (Holland et al.,1997), in contrast to a much more rapid activation for Trks. Significantly,the phosphorylation of ARMS followed a time course similar tothe time course of Eph receptor autophosphorylation (Fig. 9B).

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Figure 9. Phosphorylation of ARMS by ephrins. A, Ephrin B2 induces ARMS tyrosine phosphorylation in NG108-15 cells expressing EphB2 receptor. Lysates were made from untreated or ligand-stimulated NG108-15 cells (using aggregated ephrin B2; 30-40 min) and immunoprecipitated with 892 antiserum or preimmune (PI) serum. Tyrosine phosphorylation was assessed with pY99 in subsequent Western blots (top). Equivalent amounts of ARMS were immunoprecipitated (bottom). B, Tyrosine phosphorylation of ARMS by ephrin B2 peaks at 30 min. Thus, the time course of ARMS tyrosine phosphorylation closely parallels that of receptor autophosphorylation.

Unlike the Trk receptors, which are activated after dimerization by their respective ligands, Eph receptors are aggregatedinto multimeric complexes to be biologically active. This differentialproperty of receptor aggregation may account for the differentialtime courses observed between neurotrophins and ephrins. Interestingly,the time course of TrkA and EphB2 phosphorylation of ARMS suggeststhat ARMS may be phosphorylated directly by the kinase domainsof the receptors themselves and not via downstream intermediates.The integral membrane nature of ARMS and its potentially closeproximity to receptor tyrosine kinases could facilitate such aprocess. Most important, these results suggest that ARMS is phosphorylatedby receptor tyrosine kinases with established roles in axonaltargeting and guidance. It remains to be determined whether ephrin-Ephclustering and subsequent ARMS phosphorylation are involved inattractive or repulsive effects during axonguidance.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

ARMS: a novel downstream target for receptor tyrosine kinases

Although the signaling properties of the Trk receptor tyrosine kinases have been studied extensively, there remain many neurotrophin-stimulatedactivities in which molecular mechanisms have not been fully defined.These include internalization and transport of receptors, growthcone guidance, and axonal and dendritic branching. A number ofcommon substrates, including phospholipase C- $gamma$ , PI-3 kinase, andShc and Grb2 adaptor proteins, are used by many receptor tyrosinekinases, raising the question of how phosphorylation events leadto different biological outcomes (Chao, 1992b). One possibilityis that unique substrates exist that determine the specific natureof neurotrophinresponses.

Here we describe the properties of a novel tyrosine-phosphorylated transmembrane protein. The ARMS protein is highly expressedin many neuronal populations and functions as a downstream targetfor both Trks and Eph receptors. A common feature of ARMS, p75,TrkA, and Eph receptors is that they all contain putative C-terminalPDZ-binding motifs. It is therefore possible that these proteinsare localized to the same subcellular compartment by PDZ domain-containingmolecules, and this localization may contribute to signaling eventsboth developmentally and in adulthood. Indeed, the EphB2 receptorhas been found to be associated with PDZ-containing proteins,and this association is thought to be important for receptor functionat neuronal synapses (Torres et al., 1998) and for vestibularaxon guidance and ionic homeostasis in the inner ear (Cowan etal., 2000).

At E14, trigeminal and vestibular axons migrate toward their peripheral targets and commence synapse formation. High levelsof ARMS mRNA expression in these subpopulations suggest that ARMSmay participate in axonogenesis or axon guidance. A notable absenceof ARMS mRNA expression was observed in germinal zones of thedeveloping brain, regions that are extensively proliferating.A general conclusion that can be drawn from the in situ hybridizationstudies described here is that ARMS-positive neuron populations,for the most part, are postmitotic and postmigratory. For example,the somatic and visceral motor neurons of the spinal cord areborn by E12 and E13 but by E14 are already undergoing axonogenesis(Paxinos, 1995). It is during this postmigratory, differentiativestage that ARMS is highly expressed. Conversely, the presumptiveolfactory bulb, which is devoid of neurons at this stage of development,is negative for ARMS expression; the absence of ARMS expressionin premigratory neuronal populations supports the observationthat ARMS expression may be restricted to postmitotic and postmigratoryneurons. These findings suggest that ARMS may be involved in postmigratoryevents, such as axon guidance orsynaptogenesis.

We observed expression of ARMS in the adult CNS in regions such as the olfactory bulb, hippocampus, Purkinje cells of thecerebellum, and spinal cord motor neurons. The most significantcommon attribute of these neuronal populations is their abilityto undergo continued synaptic changes throughout adult life. Neuronsof the olfactory bulb are continually renewed and hence must formnew synapses, hippocampal neurons can undergo synaptic remodelingand long-term potentiation, Purkinje cell dendrites are highlyplastic because of their constant structural remodeling, and motorneurons have the capacity to regenerate and to form new synapseswith peripheral targets in adults. Peripheral neurons have regenerativeproperties throughout adulthood, and this process requires axonoutgrowth and new synapse formation. Neurotrophins and ephrinsare likely candidates in spinal cord regeneration (Frisén etal., 1992; Miranda et al., 1999), and it remains to be determinedwhether ARMS is also used in thisprocess.

Colocalization of ARMS with neurotrophin and ephrin receptors

The in vivo use of ARMS by the neurotrophin and ephrin receptors is supported by coexpression of these proteins during development.For example, Trk and p75 expression can be detected in all peripheralganglia of neural crest origin (e.g., superior cervical and dorsalroot), spinal cord, and brainstem, regions also high in ARMS mRNA(Yan and Johnson, 1988; Snider, 1994). In the adult, ARMS andp75 expression overlaps most notably in the olfactory bulb, Purkinjecells of the cerebellum, and motor neurons of the spinal cord.Additionally, Trk receptors are found throughout the nervous systemin regions that also express ARMS. For example, TrkA and ARMSare both expressed in the small-diameter sensory neurons of theDRG (Averill et al., 1995; Wright and Snider, 1995). Adult hippocampus,cerebellar Purkinje cells, and motor neurons of the spinal cordare a few regions in which the expression of ARMS and TrkB significantlyoverlaps (Yan et al., 1997).

In a similar manner, Eph receptor and ARMS expression overlaps in adult hippocampus and spinal motor neurons. During development,the Eph receptors are also found in ganglia of neural crest origin(e.g., sensory and vestibular) and in the tectum (Flanagan andVanderhaeghen, 1998), regions that also express ARMS. Ephrinsand their receptors have a well known function in establishmentof the retinotectal pathway, and the expression of ARMS in thetectum suggests that ARMS plays a role in thisprocess.

Because of the multiple cell populations that express Trks, Eph receptors, and ARMS, such as sensory and motor neurons, ourfindings raise the possibility of cross-talk between these tworeceptor systems. ARMS may serve to link or modulate these twosignaling pathways in a cooperative or competitive manner. Thiscould potentially be achieved by receptor phosphorylation of similaror different tyrosine residues of ARMS and/or association withother membrane proteins. It is plausible that ARMS may serve asan adaptor protein, because of its PDZ-binding motif and otherprotein interaction domains that would allow for recruitment ofmultiple, diverseproteins.

Other potential functions

The predicted integral membrane structure of ARMS led us to hypothesize that ARMS may function as an ion channel. The fourpredicted transmembrane domains of the ARMS protein and its overallstructure are reminiscent of the transient receptor potentialfamily of ion channels and the vanilloid (capsaicin) receptorVR1 (Caterina et al., 1997; Harteneck et al., 2000). These channelscontain six transmembrane domains with intracellular N and C terminiand N-terminal ankyrin repeats. Although we have not detectedARMS channel activity in gene transfer experiments, it remainspossible that this protein may also serve as a subunit of a channelor is involved in clustering or maintenance of ion channels. Sucha possibility has been suggested by the ability of BDNF to elicithippocampal, cortical, and cerebellar depolarization on a veryrapid time scale (Kafitz et al., 1999), presumably via activationof sodium channels. Although the mechanism of this activationis unknown, phosphorylation of ARMS by TrkB suggests a role forARMS in neurotrophin-mediated regulation of neuronalactivity.

The ARMS protein is a novel, neuron-enriched protein that is highly conserved throughout evolution. ARMS is expressed in postmitoticneurons during the stage of development in which extensive axonpathfinding is occurring and is also expressed during adulthoodin "plastic" regions of the brain. The presence of multiple proteininteraction domains strongly supports a role for ARMS in recruitingproteins to Trk receptor tyrosine kinases. Indeed, coimmunoprecipitationstudies indicate that ARMS may be an integral part of a higherorder Trk-p75 receptor complex. These interactions may not belimited to neurotrophin signaling, because the Eph receptor familyis also capable of phosphorylating the ARMS protein. Further studiesto characterize the proteins that interact with ARMS and the consequencesof ARMS-targeted deletion will likely help elucidate the roleof this evolutionarily conservedprotein.

  FOOTNOTES

Received Aug. 7, 2000; revised Oct. 6, 2000; accepted Oct. 16, 2000.

This work was supported by National Institutes of Health Grants NS 21072 and HD 23315 to M.V.C., NS 10489 to H.K., DA 11836-02to J.B., and NS 32367 to C.L. We thank J. Lee and A. MacDermottfor their help and expertise in electrophysiological studies;Y. Amarillo and B. Rudy for help in oocyte studies; S. Chan forTrkB studies; D. Julius and A. Brake for reagents and insightfuldiscussions throughout the course of these studies; H. Yano forsympathetic cultures; W. Walwyn for DRG sections; and E. Beckerand E. Skolnik for NG108-15 cells, reagents, and helpfuldiscussions.
Correspondence should be addressed to Dr. Moses V. Chao, Skirball Institute for BIOMOL">Biomolecular Medicine, New York UniversityMedical Center, 540 First Avenue, New York, NY 10016. E-mail:chao{at}saturn.med.nyu.edu.

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