Truncated Soluble Nogo Receptor Binds Nogo-66 and Blocks Inhibition of Axon Growth by Myelin

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

HOME | SEARCH | ARCHIVE | SUBSCRIBE | CONTACT | HELP

This Article

Abstract

Full Text (PDF)

Submit an eLetter

Alert me when this article is cited

Alert me when eLetters are posted

Alert me if a correction is posted

Citation Map

Services

Email this article to a friend

Similar articles in this journal

Similar articles in ISI Web of Science

Similar articles in PubMed

Alert me to new issues of the journal

Download to citation manager

Citing Articles

Citing Articles via HighWire

Citing Articles via ISI Web of Science (82)

Citing Articles via Google Scholar

Google Scholar

Articles by Fournier, A. E.

Articles by Strittmatter, S. M.

Search for Related Content

PubMed

PubMed Citation

Articles by Fournier, A. E.

Articles by Strittmatter, S. M.

Previous Article  |  Next Article

The Journal of Neuroscience, October 15, 2002, 22(20):8876-8883

Truncated Soluble Nogo Receptor Binds Nogo-66 and Blocks Inhibition of Axon Growth by Myelin
Alyson E. Fournier, Graham C. Gould, Betty P. Liu, and Stephen M. Strittmatter
Department of Neurology and Section of Neurobiology, Yale University School of Medicine, New Haven, Connecticut 06510

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

CNS myelin contains axon outgrowth inhibitors, such as Nogo, that restrict regenerative growth after injury. An understandingof the mechanism of Nogo signaling through its receptor (NgR)is critical to developing strategies for overcoming Nogo-mediatedinhibition. Here we analyze the function of NgR domains in outgrowthinhibition. Analysis of alkaline phosphatase (AP)-Nogo bindingin COS-7 cells reveals that the leucine-rich repeat domain isnecessary and sufficient for Nogo binding and NgR multimerization.Viral infection of embryonic day 7 chick retinal ganglion cellswith mutated NgR demonstrates that the NgR C-terminal domain isrequired for inhibitory signaling but not ligand binding. TheNgR glycosylphosphatidylinositol domain is not essential for inhibitorysignaling but may facilitate Nogo responses. From this analysis,we have developed a soluble, truncated version of the Nogo receptorthat antagonizes outgrowth inhibition on both myelin and Nogosubstrates. These data suggest that NgR mediates a significantfraction of myelin inhibition of axonoutgrowth.

Key words: Nogo; myelin; axon inhibition; Nogo receptor; CNS; leucine-rich repeat

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

The inability of injured CNS neurons to spontaneously regenerate is caused in part by the presence of myelin-associated inhibitorymolecules at the CNS injury site. Multiple inhibitors have beenidentified in myelin (McKerracher et al., 1994; Mukhopadhyay etal., 1994; Niederost et al., 1999), and one of the most potentinhibitors may be Nogo (Caroni and Schwab, 1988a; Chen et al.,2000; GrandPre et al., 2000; Prinjha et al., 2000). This contentionis supported by experiments showing that treatment with the inhibitorneutralization (IN-1) antibody, which recognizes Nogo-A, enhancedneurite outgrowth and functional recovery after CNS spinal cordinjuries in rats (Caroni and Schwab, 1988b; Schnell and Schwab,1990). However, IN-1 recognizes several other proteins in CNSmyelin extracts; therefore, experiments with specific Nogo reagentsare necessary to determine the relative contribution of Nogo tomyelin-based axoninhibition.

Nogo is a member of the reticulon protein family, and its inhibitory activity has been demonstrated in multiple assays inboth non-neuronal and neuronal cells (Chen et al., 2000; GrandPreet al., 2000; Prinjha et al., 2000; Fournier et al., 2001). Themechanism of action of Nogo inhibition may be complex, becausetwo different inhibitory domains have been identified in the Nogoprotein. Both the N-terminal portion of Nogo-A (Amino-Nogo; residues1-1024) (Chen et al., 2000; Prinjha et al., 2000) and a 66 aminoacid hydrophilic protein segment in the C-terminal region of Nogo(Nogo-66) (GrandPre et al., 2000; Fournier et al., 2001) haveinhibitory activity. Although both domains may have importantbiological activities, Nogo-66 is expressed on the surface ofoligodendrocytes (GrandPre et al., 2000) and has specific inhibitoryeffects on neurons in a soluble form. Because the epitope recognizedby IN-1 is not defined, the relative contribution of Amino-Nogoand Nogo-66 to myelin action on axons is poorly defined by publishedstudies.

A receptor for Nogo-66 (NgR) has been identified (Fournier et al., 2001). NgR is a 473 amino acid protein containing a signalsequence, a leucine-rich repeat (LRR)-type N-terminal domain,eight LRR domains, a cysteine-rich LRR-type C-terminal flankingdomain, a unique C-terminal region, and a glycosylphosphatidylinositol(GPI) anchorage site. The LRR domains of the NgR share moderateamino acid sequence similarity to many other LRR-containing proteins.Because other LRR proteins serve a wide variety of functions (Buchananand Gay, 1996), they offer little insight into the mechanism ofNgRsignaling.

The presence of a GPI anchor in the NgR raises several issues with regard to NgR signaling mechanisms. First, the GPI-linkednature of NgR suggests an interaction with a transmembrane receptorsubunit capable of intracellular signal transduction. Second,the GPI domain might play a critical role in lipid raft localizationand signal transduction as shown for glial cell line-derived neurotrophicfactor (GDNF) family receptors (Tansey et al., 2000). Third, theGPI anchor may provide an NgR cleavage site for the release ofsoluble NgR from the cell surface. Such cleavage might renderthe affected cell insensitive to Nogo and/or modulate Nogo signalingon adjacentcells.

In this study, we attempt to clarify the mechanism of NgR action by systematically deleting NgR domains and testing thesedeletion mutants in both ligand binding and Nogo signaling assays.By studying alkaline phosphatase (AP)-Nogo binding in COS-7 cells,we have determined that all of the NgR LRR domains are requiredfor Nogo binding. We have also identified a domain in the C-terminalportion of NgR that is necessary but not sufficient for NgR signaling.The GPI linkage of NgR is not critical for Nogo signaling butmay play a modulatory role in inhibitory signaling. This analysishas led to the identification of a soluble, truncated NgR (NgREcto)that antagonizes the neurite outgrowth-inhibitory effects of Nogo.NgREcto also antagonizes myelin-dependent inhibition, suggestingthat signaling through the NgR mediates a significant proportionof myelininhibition.

  MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nogo receptor deletion mutants and chimeras. Myc-tagged mouse wild-type NgR (WTNgR) in pSecTag2Hygro (Invitrogen, Burlingame,CA) (Fournier et al., 2001) was used as a template for NgR deletionand chimeric mutants. To generate NgR with the CT region deleted(NgR $Delta$ CT), the LRR region (residues 1-310) and GPI region (residues445-473) were amplified separately, ligated together at a NotIsite, and then ligated into the BamH1/XhoI sites of pSecTag2.LRR deletions were generated using the ExSite PCR-based site-directedmutagenesis kit (Stratagene, La Jolla, CA). Deletions were asfollows: NgR $Delta$ NT, residues 1-57; NgR $Delta$ 1-2, residues 58-105; NgR $Delta$ 3-4,residues 106-154; NgR $Delta$ 5-6, residues 155-202; NgR $Delta$ 7-8, residues203-250; and NgR $Delta$ LRRCT, residues 260-310. NgRCT (residues 310-445)was amplified and cloned into the BamH1/EcoR1 site of pGEXTAG2.Cloning of HSVPlexA1 (herpes simplex virus-plexin A1) has beendescribed previously (Takahashi et al., 1999). To construct HSVWTNgR,HSVNgRCT, and HSVNgR $Delta$ CT, the corresponding NgR was amplified withthe signal sequence from pSecTag2 and ligated into the HindIII/SalIsites of pHSVPrPUC. The HSV transfer vector for the NgRL1 chimericprotein was constructed by substituting the cDNA encoding aminoacids 1-451 of mouse NgR for the neuropilin-1 coding region inthe HSV-NP1-L1 vector (Nakamura et al., 1998).

Purified NgREcto protein was a generous gift from Biogen Inc. (Cambridge, MA). To construct NgREcto, cDNA encoding amino acids1-310 of rat NgR was cloned by PCR into the expression vectorPV90, and the resulting plasmid was transfected into CHO cells.Amino acid substitutions were present, resulting in the followingsequence: MKRASAGGSR LLAWVLWLQA WRVATPCPGA CVCYNEPKVT TSCPQQGLQAVPTGIPASSQ RIFLHGNRIS YVPAASFQSC RNLTILWLHS NALAGIDAAA FTGLTLLEQLDLSDNAQLRV VDPTTFRGLG HLHTLHLDRC GLQELGPGLF RGLAALQYLY LQDNNLQALPDNTFRDLGNL THLFLHGNRI PSVPEHAFRG LHSLGRLLLH QNHVARVHPH AFRDLGRLMTLYLFANNLSM LPAEVLVPLR SLQYLRLNDN PWVCGCRARP LWAWLQKFRG SSSEVPCNLPQRLAGRDLKR LAASDLQGCA. A clone derived by limiting dilution thatwas expressing high levels of NgREcto was expanded in serum-freeculture medium. Conditioned medium was collected, and NgREctowas purified by cation-exchange chromatography on an SP-Sepharosecolumn. The resultant protein was ~85% pure. N-Terminal sequenceanalysis of the rat NgR1 (1-310) product verified that the matureprotein started with Cys-27, which matched the predicted startsite.

Preparation of recombinant proteins. To construct the AP-NgR vector, the NgR coding sequence from residues 27-451 was ligatedin frame with the signal sequence-histidine 6 (His6)-AP sequenceof pAP-6. To express AP-NgR, plasmid was transfected into HEK293Tcells, and conditioned medium was collected after 4 d. Secretedprotein was purified by Ni²⁺ affinity chromatography (Nakamura et al., 1998). AP-Nogo or AP-NgRbinding in COS-7 cells was assessed as described previously (Takahashiet al., 1998; Fournier et al., 2001).

Growth cone collapse and neurite outgrowth assays. Preparation of embryonic day 7 (E7) chick retinal explant cultures andrecombinant HSV preparations have been described in detail previously(Fournier et al., 2000a). Retinal explants were grown for 12 hrand then incubated for an additional 24 hr with HSVNgR preparations.Explants were treated for 30 min with 0, 50, 250, or 500 nM glutathioneS-transferase (GST) Nogo-66 (GrandPre et al., 2000), fixed, andstained with phalloidin (Molecular Probes, Eugene, OR). Growthcone collapse was assayed as described previously (Luo et al.,1993). For neurite outgrowth assays on Nogo, myelin, or aggrecansubstrates, Permanox chamber slides (Fisher Scientific, Pittsburgh,PA) were coated with 100 µg/ml poly-L-lysine and washed, and then3 µl drops of PBS containing 0, 50, or 150 ng of GSTNogo-66, myelin,or aggrecan with or without 500 ng of NgREcto were spotted anddried. After three PBS washes, slides were coated with 10 µg/mllaminin. Dissociated E13 chick dorsal root ganglia (DRG) neuronswere grown for 4-8 hr, fixed, and stained with phalloidin, andneurite outgrowth lengths were assessed using NIH Image. GSTNogo-66and myelin were prepared as described previously (Fournier etal., 2000b; GrandPre et al., 2000). Aggrecan was obtained fromSigma (St. Louis,MO).

Analysis of membrane fractions on flotation gradients. HEK293T cells were cultured in 6 cm culture dishes and transfectedwith HSVWTNgR or HSVNgRL1 plasmids. After 48 hr, cells were rinsedwith PBS and then lysed on ice with 375 µl precooled TNE buffer(in mM: 50 Tris-HCl, pH 7.4, 150 NaCl, and 5 EDTA) containing0.1% Triton X-100, 10 mM NaF, and protease inhibitors (TNEX).Cells were homogenized by passing the ice-cold lysates througha 27 gauge needle 10 times. Extracts were adjusted to 35% OptiPrep(Invitrogen, Gaithersburg, MD) by adding 525 µl of 60% OptiPrep-0.1%Triton X-100, placed in an ultracentrifuge tube, and overlaidwith 8.75 ml of 30% OptiPrep in TNEX and 1 ml of TNEX. After centrifugation(4 hr; 200,000 × g; 4°C), seven fractions were collected, precipitatedin TCA, washed with acetone, air dried, and resuspended in Laemmli'ssample buffer. Fractions were analyzed by 8% SDS-PAGE and immunoblottingwith the NgR antibody (Fournier et al., 2001). For detection oftransferrin receptor, a mouse monoclonal antibody (Zymed, SanFrancisco, CA) was used. Caveolin was detected with a rabbit polyclonalantibody (Upstate Biotechnology, Lake Placid,NY).

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Leucine-rich repeats are required for AP-Nogo binding

To better understand structure-function relationships for the NgR, deletion mutants were generated and tested for Nogo binding.NgR contains a signal sequence, an LRR-type N-terminal region(LRRNT) (Pfam accession number PF01462), eight LRR domains (LRR1-8)(Pfam accession number PF00560), an LRR-type C-terminal domain(LRRCT) (Pfam accession number PF01463), a unique C-terminal domain,and a GPI linkage domain (Fournier et al., 2001). Domains of theNgR were systematically deleted using PCR-based site-directedmutagenesis (Fig. 1a). Individual NgR mutants expressed in COS-7cells exhibit the predicted mobility as verified by Myc immunoblots(data not shown). The ability of individual NgR mutants to bindto Nogo-66 was assessed using an AP-Nogo binding assay (Fournieret al., 2001). COS-7 cells were transfected with individual NgRdeletion mutant constructs, treated with AP or AP-Nogo conditionedmedium, and assayed for AP binding. AP-Nogo binding was detectedin WTNgR or NgR $Delta$ CT (Fig. 1b). NgR deleted in any pair of the LRRs(NgR $Delta$ 1-2, NgR $Delta$ 3-4, NgR $Delta$ 5-6, NgR $Delta$ 7-8, and NgRLRR $-$ ) or in the N-terminalor LRR-type C-terminal flanking regions of the LRRs (NgR $Delta$ NT andNgR $Delta$ LRRCT, respectively) does not support AP-Nogo binding. TheAP-Nogo binding pattern suggests that dispersed amino acid residueswithin the NgR LRR region are required for AP-Nogo binding. Alternatively,mutations in individual LRR regions may disrupt the tertiary structureof the NgR, resulting in a loss of AP-Nogo binding. For otherLRR-containing receptors, similar deletions do not disrupt thefunction of remaining repeats (Song et al., 2001a,b), suggestingthat multiple LRRs participate directly in Nogo-66 binding.

View larger version (70K):
[in this window]
[in a new window]
Figure 1. Nogo binding to NgR deletion mutants. a, Schematic of WTNgR (WT) and the NgR deletion mutants used in this study. NgR mutants include deletions of the N-terminus ( $Delta$ NT), LRR domains 1 and 2 ( $Delta$ 1-2), 3 and 4 ( $Delta$ 3-4), 5 and 6 ( $Delta$ 5-6), 7 and 8 ( $Delta$ 7-8), the LRR C-terminus ( $Delta$ LRRCT), the C-terminus ( $Delta$ CT), and the complete LRR domain (LRR $-$ ). b, COS-7 cells transfected with NgR deletion mutant plasmids were stained for Myc immunoreactivity or tested for 20 nM AP or AP-Nogo binding. All NgR mutant proteins were expressed in COS-7 cells as shown by Myc immunoreactivity. Only WTNgR- and NgR $Delta$ CT-transfected COS-7 cells bound to AP-Nogo. Scale bar, 100 µm. c, Quantification of AP-Nogo or AP binding to COS-7 cells transfected with NgR deletion mutants.

NgRCT domain is required but not sufficient for NgR-dependent inhibition

Although the NgRCT domain is not required for Nogo binding, we considered the possibility that it participates in Nogo-dependentinhibition of axon growth. E7 retinal ganglion cells (RGCs) wereinfected with recombinant HSVNgR $Delta$ CT preparations, and growth conecollapse in response to GSTNogo-66 was assessed (Fig. 2a,b). Underthese conditions, wild-type NgR supports Nogo-66-dependent growthcone collapse. RGCs infected with NgR $Delta$ CT are not sensitive toNogo in the growth cone collapse assay. The CT region of NgR istherefore required for effective NgR inhibitory signaling.

View larger version (52K):
[in this window]
[in a new window]
Figure 2. The CT region of NgR is necessary but not sufficient for Nogo inhibition. a, E7 retinal explants were infected with a recombinant viral preparation of the NgR $Delta$ CT. NgR $Delta$ CT-infected RGCs were insensitive to a 40 min treatment with 500 nM GSTNogo-66. Expression of NgR $Delta$ CT in RGC neurites and growth cones was verified by Myc immunostaining. Scale bar, 50 µm. b, Quantification of the growth cone collapse response of RGCs to GSTNogo-66 after viral infection with NgR $Delta$ CT, WTNgR, or a control plexinA1 virus (Plexin). Means ± SEM from 4-10 experiments are reported. Student's t tests comparing WTNgR or NgR $Delta$ CT to control plexinA1 values at the indicated Nogo concentration are reported. *p < 0.001. c, E7 RGC explants were infected with recombinant viral preparations of control HSV particles (HSV) or HSVNgRCT. NgRCT alone does not cause growth cone collapse. Scale bar, 100 µm. d, Quantification of E7 RGC growth cone collapse after control HSV or HSVNgRCT infection. Means ± SEM for three experiments are reported. e, Neurite outgrowth of dissociated E13 DRGs plated on control or Nogo substrates and treated with 500 nM soluble GST or GSTNgRCT. GSTNgRCT does not inhibit neurite outgrowth on control spots or modify the response of E13 DRGs to Nogo inhibition. Scale bar, 200 µm. f, Nogo dose-response of E13 DRG neurite outgrowth in the presence of GST or GSTNgRCT. Neurite outgrowth is calculated as micrometers of growth per cell. Means ± SEM from three experiments are reported.

One possibility is that the CT domain of NgR binds to a transducing receptor component to initiate an intracellular signalingcascade after ligand binding. This would explain why NgR deletedin the CT region is signaling incompetent. If this were the case,it is also possible that the CT region of NgR is capable of constitutivereceptor activity. To test this possibility, recombinant viralpreparations expressing GPI-anchored NgRCT were used to infectE7 RGCs (Fig. 2c,d). Expression of NgRCT does not cause growthcone collapse in infected RGCs. In a second assay, NgRCT was purifiedas a soluble GST fusion protein (GSTNgRCT) and tested for itsability to disrupt signaling in a dominant negative manner. E13chick DRGs were dissociated and plated in the presence or absenceof 500 nM soluble GST or GSTNgRCT. In this assay, GSTNogo-66 inhibitsneurite outgrowth (Fournier et al., 2001). Soluble GSTNgRCT doesnot alter neurite outgrowth lengths on control substrates, nordoes it attenuate or enhance the response of dissociated E13 DRGson Nogo substrates (Fig. 2e,f). Together, these experiments indicatethat the CT region of NgR is necessary but not sufficient forNgR-dependentinhibition.

NgR GPI domain is not required for NgR signaling

In some cases, GPI anchors are critical for receptor function. The GPI anchor of GDNF receptor- $alpha$ 1 (GFR $alpha$ 1) plays a criticalrole in localizing receptor components to lipid rafts and permittingreceptor tyrosine kinase (RET) activation (Tansey et al., 2000).To assess the role of the GPI anchor in mediating inhibitory Nogosignals, a chimeric NgR was generated by exchanging the NgR GPIdomain with the transmembrane domain of the L1 cell adhesion molecule(Nieke and Schachner, 1985) in a pHSVPrPUC vector (HSVNgRL1).GPI-linked proteins localize to detergent-insoluble sphingolipidand cholesterol-rich lipid microdomains that exist as phase-separated"lipid rafts" in the plasma membrane (Simons and Ikonen, 1997;Brown and London, 1998). Sphingolipids and cholesterol in cellmembranes are resistant to solubilization with nonionic detergentsat 4°C, allowing lipid rafts to be isolated as detergent-resistantmembrane fractions (Brown and Rose, 1992).

HEK293T cells were transfected with HSVWTNgR or HSVNgRL1, and membrane fractionation on flotation gradients was performed(Fig. 3). As expected for a GPI-anchored protein, WTNgR localizesprimarily to the caveolin-positive lipid raft fractions. In contrast,the vast majority of chimeric NgRL1 localizes to the caveolin-negativefractions, and the small proportion cosedimenting with caveolinis likely to reflect incomplete separation rather than any raftlocalization. The ability of NgRL1 to bind to Nogo with an affinitysimilar to that of the WTNgR was verified by assaying AP-Nogobinding in transfected COS-7 cells (Fig. 3c,d). To test the signalingcapability of NgRL1, recombinant HSVNgRL1 preparations were producedand used to infect E7 RGCs. Infected RGCs were treated with GSTNogo-66,and growth cone collapse was assessed (Fig. 4). At high concentrationsof Nogo, NgRL1 transduces Nogo signals as efficiently as WTNgR.However, a 50 nM Nogo dose collapses RGC growth cones infectedwith WTNgR, whereas NgRL1-infected RGCs are unresponsive. Therefore,NgRL1 mediates Nogo signaling less efficiently than WTNgR. TheGPI anchorage site may play a modulatory role in Nogo signaling.

View larger version (82K):
[in this window]
[in a new window]
Figure 3. Characterization of NgRL1. a, Cell lysates from HEK293T cells transfected with HSVWTNgR or HSVNgRL1 plasmids were fractionated on flotation gradients. WTNgR is found almost exclusively in the caveolin-positive detergent-insoluble fraction. b, NgRL1 is in multiple membrane fractions, with a small proportion in the caveolin-positive detergent-insoluble fraction. c, COS-7 cells were transfected with WTNgR and tested for 10 nM AP-Nogo binding. d, COS-7 cells were transfected with NgRL1 and tested for 10 nM AP-Nogo binding. Cells expressing WTNgR or NgRL1 bind similar amounts of AP-Nogo. Scale bar, 100 µm.

View larger version (62K):
[in this window]
[in a new window]
Figure 4. The GPI linkage region of NgR is not required for Nogo-mediated inhibition. a, E7 retinal explants were infected with recombinant viral preparations of PlexA1, WTNgR, or NgRL1. Explants were treated with 500 nM GSTNogo-66 for 40 min, fixed, and stained with rhodamine-phalloidin. RGCs infected with PlexA1 control virus are insensitive to Nogo, whereas those infected with WTNgR or NgRL1 collapse in response to Nogo. Scale bar, 50 µm. b, Dose-response of RGCs to GSTNogo-66 after infection with NgR viral preparations. Student's t tests comparing WTNgR or NgRL1 to PlexA1 at the indicated Nogo concentration are reported. *p = 0.01; **p < 0.01. Significance indicators (*) are coded with the appropriate infection. Means ± SEM for 6-10 experiments are reported.

NgR binds NgR

One hypothesis for the diminished signaling efficiency of NgRL1 is that NgRL1 fails to concentrate in lipid rafts, and theconsequent loss of receptor clustering leads to inefficient Nogosignaling. To consider this possibility, we determined whetherNgR was capable of interacting with itself. COS-7 cells were transfectedwith WTNgR or NgR deletion mutant plasmids and stained with AP-NgRconditioned medium (Fig. 5). Clearly, the extracellular domainof NgR has significant affinity for surface-bound NgR. Bindingsaturation was difficult to achieve reliably; however, the K_dof this interaction is estimated to be $>=$ 50 nM. Considering thatendogenous NgR molecules are likely to interact in cis withinlipid rafts, this affinity is consistent with physiological relevance.Analysis of AP-NgR binding to NgR deletion mutants reveals thatthe receptor multimerization domain, like the Nogo-66 bindingsite (Fig. 1), is localized to the LRR domains.

View larger version (59K):
[in this window]
[in a new window]
Figure 5. NgR interacts with itself. a, COS-7 cells were transfected with WTNgR or NgR deletion mutant plasmids and tested for AP or AP-NgR binding. WTNgR- and NgR $Delta$ CT-transfected COS-7 cells bind to AP-NgR. b, Quantification of AP or AP-NgR binding to COS-7 cells transfected with NgR deletion mutants. c, AP-NgR binding to COS-7 cells transfected with NgR as a function of AP-NgR concentration. Mean ± SEM for three experiments. d, COS-7 cells were transfected with WTNgR and treated with AP-NgR in the presence of 25 nM GST or GSTNogo-66 (GSTNg66). AP-NgR interaction with WTNgR is not modified by the presence of GST or GSTNogo-66. Scale bar, 100 µm. e, Quantification of AP-NgR binding to WTNgR-transfected COS-7 cells in the presence of 25 nM GST or GSTNogo-66.

Receptor multimerization does not appear to be regulated by ligand. First, the presence of Nogo has little, if any, effecton AP-NgR binding to NgR-transfected COS-7 cells (Fig. 5b). Second,when transfected HEK293T cells were treated with Nogo, the membranefractionation profile of WTNgR and NgRL1 remained unchanged (datanot shown). This suggests that Nogo does not modulate NgR localizationto lipid raft compartments in HEK293T cells. It should be notedthat both of these assays were performed in non-neuronal celllines. It is possible that Nogo affects NgR multimerization inneurons that may possess additional components required for Nogosignaling. It is also possible that ligand binding modifies thelocalization of additional unidentified signaling components withinthe lipid raft, as is the case for ephrins (Davy et al., 1999).Because the components of the NgR intracellular signaling cascadehave not been identified, the effect of Nogo on the recruitmentof signaling components to lipid rafts remains an openquestion.

Truncated NgR antagonizes Nogo and myelin-dependent inhibition

On the basis of the structure-function analysis of NgR, a truncated soluble NgR (NgREcto) was assayed for antagonism of Nogo-66signaling. NgREcto consists of residues 1 through 310, which includesthe entire binding region for Nogo-66, but lacks the NgRCT regionthat is required for NgR signaling and the GPI linkage regionof the receptor. NgREcto protein was purified from the conditionedmedium of stably transfected CHO cells. The ability of NgREctoto antagonize Nogo-NgR interactions was tested by treating WTNgR-expressingCOS-7 cells with 7 nM Nogo-AP in the presence or absence of 70nM NgREcto (Fig. 6a,b). NgREcto significantly reduces Nogo-APbinding to transfected cells. To test the effect of NgREcto onsignaling through the NgR, E13 dissociated DRGs were plated onmixed NgREcto-Nogo-66 substrates (Fig. 6c,d). Neurite outgrowthfrom E13 chick DRGs plated on GSTNogo-66 substrates without NgREctois strongly inhibited. NgREcto to a great extent reverses thisneurite outgrowth inhibition by Nogo. NgREcto is unable to overcomethe inhibitory activity of the chondroitin sulfate proteoglycanaggrecan (Seidenbecher et al., 1998), suggesting that the NgREctoreagent is acting specifically on the NgR pathway. Because boundNgREcto might alter the surface properties of the laminin-Nogosubstrate, purified NgREcto was also applied as a soluble proteinto test for its ability to antagonize Nogo inhibition (Fig. 6f).The inhibitory effect of Nogo-66 is significantly diminished inthe presence of 2 µM soluble NgREcto protein.

View larger version (68K):
[in this window]
[in a new window]
Figure 6. Soluble NgREcto antagonizes neurite outgrowth inhibition on Nogo and myelin substrates. a, AP-Nogo stain of COS-7 cells transfected with WTNgR. Cells were stained with 7 nM AP-Nogo in the presence or absence of 70 nM NgREcto. NgREcto blocks AP-Nogo binding to WTNgR. b, Quantification of AP-Nogo (7 nM) binding to WTNgR-transfected COS-7 cells in the presence or absence of 70 nM NgREcto. c, Dissociated E13 DRGs were plated on spots of PBS or 500 ng of NgREcto mixed with Nogo, myelin, or aggrecan. Nogo and myelin inhibition is partially reversed by the addition of NgREcto, whereas aggrecan inhibition is not. d, e, Dose-response of E13 DRG outgrowth on spots of PBS or 500 ng of NgREcto mixed with Nogo, myelin, or aggrecan. f, E13 DRG neurite outgrowth on Nogo or myelin substrates in the presence of 2 µM soluble purified NgREcto (Soluble NgREcto) or PBS. Neurite outgrowth is expressed as micrometers of growth per cell. Means ± SEM for four to six experiments are reported. Student's t tests comparing PBS to NgREcto at the indicated Nogo concentration are reported. *p < 0.01. Scale bar, 200 µm.

NgREcto is a specific Nogo-66 antagonist; therefore, the relative importance of Nogo-66 in inhibition of axon outgrowth byCNS myelin can be assessed. When the same protocol is used asfor GSTNogo-66, myelin strongly inhibits chick E13 DRG neuriteoutgrowth. NgREcto blocks a significant proportion of this inhibitoryactivity (Fig. 6c,e,f), consistent with the notion that NgR playsa primary role in mediating myelinaction.

  DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Previous studies have identified NgR as a highly potent, biologically active receptor for Nogo-66 (Fournier et al., 2001).By generating NgR deletion mutants and chimeric receptors, wedemonstrate that the entire LRR region of NgR is required forNogo binding to NgR and that the CT region of NgR is necessarybut not sufficient for inhibitory NgR signaling (Fig. 7). Furthermore,the GPI linkage is not critical for NgR signaling but may modulatethe efficacy of NgR-dependent inhibition. We have also identifieda soluble, truncated form of NgR that can antagonize the inhibitoryeffects of Nogo or myelin on E13 chick DRG outgrowth. This supportsa central role for NgR in myelin inhibition of axon growth.

View larger version (42K):
[in this window]
[in a new window]
Figure 7. Model of Nogo receptor-mediated signaling. This schematic illustrates the proposed role each Nogo receptor domain plays in Nogo-signal transduction. See Discussion.

Role of NgR LRR and CT domains

It is clear that the LRR domains of NgR are required for binding to Nogo. Because the NgRCT region is not sufficient to induceinhibition, it is likely that the LRR domains contribute to additionalaspects of inhibitory signaling. The LRR region can also bindto full-length NgR; therefore, this domain may regulate receptoroligomerization and/or bind to an unidentified signal-transducingreceptor subunit. The greatest sequence similarity in the NgRLRR region exists with Slit 1-3 and the acid-labile subunit ofthe insulin-like growth factor-binding protein complex. Slitsare a family of extracellular matrix proteins that are expressedat the developing CNS midline and repel axons via receptors ofthe Roundabout (Robo) family (Brose et al., 1999; Zinn and Sun,1999). The Slit LRRs have been shown recently to mediate bindingto Robo and repellent signaling (Battye et al., 2001). Thus, theSlit-Robo interaction may provide a model for NgR interactionwith a signal-transducingprotein.

The unique CT domain of the NgR is required for NgR-dependent inhibition. The most plausible model is that this domain participatesdirectly in the activation of a transmembrane signal-transducingcomponent of the NgR. However, its inability to act in a constitutivelyactive manner raises the possibility that the CT domain may facilitateNgR conformational changes that lead to axon inhibition by theLRRdomain.

Role of the NgR GPI anchor

The GPI anchor is not absolutely required for NgR inhibitory signaling, because chimeric NgRL1 mediates Nogo-66-induced growthcone collapse when expressed in RGCs. The GPI anchor site couldmodulate the efficacy of NgR signaling by concentrating NgR inlipid rafts. The importance of raft localization of receptorsis clear for the GDNF receptors GFR $alpha$ 1-GFR $alpha$ 4. GFR $alpha$ 1-GFR $alpha$ 4 are GPI-anchoredreceptors that are responsible for providing specific high-affinitybinding sites for individual GDNF family ligands (GFL). All GFRsinteract with a common receptor tyrosine kinase, RET (Tansey etal., 2000), that signals intracellularly via its cytoplasmic kinasedomain. The GPI anchor plays a critical role in the GFL signalingpathway by restricting GFR $alpha$ 1 protein to lipid rafts, where RETis recruited after GDNF family ligand binding. GFR $alpha$ 1-mediatedRET recruitment to the lipid raft is critical for efficient GFLsignaling. Lipid rafts are thought to represent specialized signalingcompartments within the plasma membrane because of the enrichmentof Src family kinases and other signaling proteins that localizeto the intracellular leaflet of lipid rafts (Anderson, 1998).The GPI anchor of the NgR could regulate the efficiency of NgRsignaling by restricting its localization within the plasma membrane.This restricted distribution might enhance NgR multimerizationand access to downstream signalingmolecules.

It is also plausible that the role of the NgR GPI linkage is to provide an NgR cleavage site. Although there is as yet noevidence that truncated soluble NgR exists in vivo, it is clearthat NgREcto is capable of antagonizing myelin inhibition. ReleasedNgR might modulate Nogo signaling by loss of surface NgR fromone axon and by diffusible blockade of NgRaction.

NgREcto reverses Nogo signaling

The NgREcto protein contains a Nogo-66 binding site and blocks Nogo-66 action. Soluble NgREcto may bind to Nogo and preventits binding to full-length active Nogo receptors on the neuronalcell surface. Alternatively, NgREcto might interact with surface-boundaxonal NgR and prevent receptor oligomerization or NgR interactionwith a signal-transducing receptor subunit (Fig. 7). The affinityof AP-Nogo is fivefold to 10-fold higher than AP-NgR for surface-boundNgR. Therefore, it is likely that NgREcto acts primarily by disruptingligand-receptorinteractions.

NgR mediates myelin inhibition

Previous work had not clarified the relative role of myelin-derived inhibitors on axon growth or the role of different Nogodomains. The ability of NgREcto to reverse a majority of myelin-dependentinhibition of axon growth demonstrates that the Nogo-66 receptoris a primary mediator of myelin action. Furthermore, the NgREctoprotein is a potential therapeutic agent to promote axon regenerationin the injured adultCNS.

  FOOTNOTES

Received Feb. 8, 2002; revised July 25, 2002; accepted Aug. 1, 2002.

This work was supported by grants to S.M.S. from the National Institutes of Health, the McKnight Foundation for Neuroscience,the Institute for the Study of Aging, and Biogen Inc. S.M.S. isan Investigator of the Patrick and Catherine Weldon Donaghue MedicalResearch Foundation. Purified NgREcto protein was a generous giftfrom Biogen Inc. (Cambridge,MA).

Correspondence should be addressed to Stephen M. Strittmatter, Department of Neurology, Yale University School of Medicine,P.O. Box 208018, New Haven, CT 06510. E-mail: stephen.strittmatter{at}yale.edu.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Anderson RG (1998) The caveolae membrane system. Annu Rev Biochem 67:199-225[ISI][Medline].
Battye R, Stevens A, Perry RL, Jacobs JR (2001) Repellent signaling by Slit requires the leucine-rich repeats. J Neurosci 21:4290-4298[Abstract/Free Full Text].
Brose K, Bland KS, Wang KH, Arnott D, Henzel W, Goodman CS, Tessier-Lavigne M, Kidd T (1999) Slit proteins bind Robo receptors and have an evolutionarily conserved role in repulsive axon guidance. Cell 96:795-806[ISI][Medline].
Brown DA, London E (1998) Functions of lipid rafts in biological membranes. Annu Rev Cell Dev Biol 14:111-136[ISI][Medline].
Brown DA, Rose JK (1992) Sorting of GPI-anchored proteins to glycolipid-enriched membrane subdomains during transport to the apical cell surface. Cell 68:533-544[ISI][Medline].
Buchanan SG, Gay NJ (1996) Structural and functional diversity in the leucine-rich repeat family of proteins. Prog Biophys Mol Biol 65:1-44[ISI][Medline].
Caroni P, Schwab ME (1988a) Two membrane protein fractions from rat central myelin with inhibitory properties for neurite growth and fibroblast spreading. J Cell Biol 106:1281-1288[Abstract/Free Full Text].
Caroni P, Schwab ME (1988b) Antibody against myelin-associated inhibitor of neurite growth neutralizes nonpermissive substrate properties of CNS white matter. Neuron 1:85-96[ISI][Medline].
Chen MS, Huber AB, van der Haar ME, Frank M, Schnell L, Spillmann AA, Christ F, Schwab ME (2000) Nogo-A is a myelin-associated neurite outgrowth inhibitor and an antigen for monoclonal antibody IN-1. Nature 403:434-439[Medline].
Davy A, Gale NW, Murray EW, Klinghoffer RA, Soriano P, Feuerstein C, Robbins SM (1999) Compartmentalized signaling by GPI-anchored ephrin-A5 requires the Fyn tyrosine kinase to regulate cellular adhesion. Genes Dev 13:3125-3135[Abstract/Free Full Text].
Fournier AE, Kalb RG, Strittmatter SM (2000a) Rho GTPases and axonal growth cone collapse. Methods Enzymol 325:473-482[Medline].
Fournier AE, Nakamura F, Kawamoto S, Goshima Y, Kalb RG, Strittmatter SM (2000b) Semaphorin3A enhances endocytosis at sites of receptor-F-actin colocalization during growth cone collapse. J Cell Biol 149:411-422[Abstract/Free Full Text].
Fournier AE, GrandPre T, Strittmatter SM (2001) Identification of a receptor mediating Nogo-66 inhibition of axonal regeneration. Nature 409:341-346[Medline].
GrandPre T, Nakamura F, Vartanian T, Strittmatter SM (2000) Identification of the Nogo inhibitor of axon regeneration as a reticulon protein. Nature 403:439-444[Medline].
Luo Y, Raible D, Raper JA (1993) Collapsin: a protein in brain that induces the collapse and paralysis of neuronal growth cones. Cell 75:217-227[ISI][Medline].
McKerracher L, David S, Jackson DL, Kottis V, Dunn RJ, Braun PE (1994) Identification of myelin-associated glycoprotein as a major myelin-derived inhibitor of neurite growth. Neuron 13:805-811[ISI][Medline].
Mukhopadhyay G, Doherty P, Walsh FS, Crocker PR, Filbin MT (1994) A novel role for myelin-associated glycoprotein as an inhibitor of axonal regeneration. Neuron 13:757-767[ISI][Medline].
Nakamura F, Tanaka M, Takahashi T, Kalb RG, Strittmatter SM (1998) Neuropilin-1 extracellular domains mediate semaphorin D/III-induced growth cone collapse. Neuron 21:1093-1100[ISI][Medline].
Niederost BP, Zimmermann DR, Schwab ME, Bandtlow CE (1999) Bovine CNS myelin contains neurite growth-inhibitory activity associated with chondroitin sulfate proteoglycans. J Neurosci 19:8979-8989[Abstract/Free Full Text].
Nieke J, Schachner M (1985) Expression of the neural cell adhesion molecules L1 and N-CAM and their common carbohydrate epitope L2/HNK-1 during development and after transection of the mouse sciatic nerve. Differentiation 30:141-151[ISI][Medline].
Prinjha R, Moore SE, Vinson M, Blake S, Morrow R, Christie G, Michalovich D, Simmons DL, Walsh FS (2000) Inhibitor of neurite outgrowth in humans. Nature 403:383-384[Medline].
Schnell L, Schwab ME (1990) Axonal regeneration in the rat spinal cord produced by an antibody against myelin-associated neurite growth inhibitors. Nature 343:269-272[Medline].
Seidenbecher CI, Gundelfinger ED, Bockers TM, Trotter J, Kreutz MR (1998) Transcripts for secreted and GPI-anchored brevican are differentially distributed in rat brain. Eur J Neurosci 10:1621-1630[ISI][Medline].
Simons K, Ikonen E (1997) Functional rafts in cell membranes. Nature 387:569-572[Medline].
Song YS, Ji I, Beauchamp J, Isaacs NW, Ji TH (2001a) Hormone interactions to Leu-rich repeats in the gonadotropin receptors. I. Analysis of Leu-rich repeats of human luteinizing hormone/chorionic gonadotropin receptor and follicle-stimulating hormone receptor. J Biol Chem 276:3426-3435[Abstract/Free Full Text].
Song YS, Ji I, Beauchamp J, Isaacs NW, Ji TH (2001b) Hormone interactions to Leu-rich repeats in the gonadotropin receptors. II. Analysis of Leu-rich repeat 4 of human luteinizing hormone/chorionic gonadotropin receptor. J Biol Chem 276:3436-3442[Abstract/Free Full Text].
Takahashi T, Nakamura F, Jin Z, Kalb RG, Strittmatter SM (1998) Semaphorins A and E act as antagonists of neuropilin-1 and agonists of neuropilin-2 receptors. Nat Neurosci 1:487-493[ISI][Medline].
Takahashi T, Fournier A, Nakamura F, Wang LH, Murakami Y, Kalb RG, Fujisawa H, Strittmatter SM (1999) Plexin-neuropilin-1 complexes form functional semaphorin-3A receptors. Cell 99:59-69[ISI][Medline].
Tansey MG, Baloh RH, Milbrandt J, Johnson Jr EM (2000) GFRalpha-mediated localization of RET to lipid rafts is required for effective downstream signaling, differentiation, and neuronal survival. Neuron 25:611-623[ISI][Medline].
Zinn K, Sun Q (1999) Slit branches out: a secreted protein mediates both attractive and repulsive axon guidance. Cell 97:1-4[ISI][Medline].

Copyright © 2002 Society for Neuroscience 0270-6474/02/22208876-08$05.00/0

This article has been cited by other articles:

J. K. Atwal, J. Pinkston-Gosse, J. Syken, S. Stawicki, Y. Wu, C. Shatz, and M. Tessier-Lavigne
PirB is a Functional Receptor for Myelin Inhibitors of Axonal Regeneration
Science, November 7, 2008; 322(5903): 967 - 970.
[Abstract] [Full Text] [PDF]

G. K. Seabold, P. Y. Wang, K. Chang, C.-Y. Wang, Y.-X. Wang, R. S. Petralia, and R. J. Wenthold
The SALM Family of Adhesion-like Molecules Forms Heteromeric and Homomeric Complexes
J. Biol. Chem., March 28, 2008; 283(13): 8395 - 8405.
[Abstract] [Full Text] [PDF]

L. Dupuis, M. Pehar, P. Cassina, F. Rene, R. Castellanos, C. Rouaux, M. Gandelman, L. Dimou, M. E. Schwab, J.-P. Loeffler, et al.
Nogo receptor antagonizes p75NTR-dependent motor neuron death
PNAS, January 15, 2008; 105(2): 740 - 745.
[Abstract] [Full Text] [PDF]

G. B. Ferraro
Refining Our Understanding of NgR1 Function during Myelin Inhibition
J. Neurosci., October 24, 2007; 27(43): 11451 - 11452.
[Full Text] [PDF]

O. Chivatakarn, S. Kaneko, Z. He, M. Tessier-Lavigne, and R. J. Giger
The Nogo-66 Receptor NgR1 Is Required Only for the Acute Growth Cone-Collapsing But Not the Chronic Growth-Inhibitory Actions of Myelin Inhibitors
J. Neurosci., July 4, 2007; 27(27): 7117 - 7124.
[Abstract] [Full Text] [PDF]

W. B. J. Cafferty, S.-H. Yang, P. J. Duffy, S. Li, and S. M. Strittmatter
Functional Axonal Regeneration through Astrocytic Scar Genetically Modified to Digest Chondroitin Sulfate Proteoglycans
J. Neurosci., February 28, 2007; 27(9): 2176 - 2185.
[Abstract] [Full Text] [PDF]

J. Lauren, F. Hu, J. Chin, J. Liao, M. S. Airaksinen, and S. M. Strittmatter
Characterization of Myelin Ligand Complexes with Neuronal Nogo-66 Receptor Family Members
J. Biol. Chem., February 23, 2007; 282(8): 5715 - 5725.
[Abstract] [Full Text] [PDF]

L. Dimou, L. Schnell, L. Montani, C. Duncan, M. Simonen, R. Schneider, T. Liebscher, M. Gullo, and M. E. Schwab
Nogo-A-Deficient Mice Reveal Strain-Dependent Differences in Axonal Regeneration
J. Neurosci., May 24, 2006; 26(21): 5591 - 5603.
[Abstract] [Full Text] [PDF]

J. H. Park, D. A. Gimbel, T. GrandPre, J.-K. Lee, J.-E. Kim, W. Li, D. H. S. Lee, and S. M. Strittmatter
Alzheimer Precursor Protein Interaction with the Nogo-66 Receptor Reduces Amyloid-beta Plaque Deposition
J. Neurosci., February 1, 2006; 26(5): 1386 - 1395.
[Abstract] [Full Text] [PDF]

E. M. Frohman, O. Stuve, E. Havrdova, J. Corboy, A. Achiron, R. Zivadinov, P. S. Sorensen, J. T. Phillips, B. Weinshenker, K. Hawker, et al.
Therapeutic Considerations for Disease Progression in Multiple Sclerosis: Evidence, Experience, and Future Expectations
Arch Neurol, October 1, 2005; 62(10): 1519 - 1530.
[Abstract] [Full Text] [PDF]

F. Hu, B. P. Liu, S. Budel, J. Liao, J. Chin, A. Fournier, and S. M. Strittmatter
Nogo-A Interacts with the Nogo-66 Receptor through Multiple Sites to Create an Isoform-Selective Subnanomolar Agonist
J. Neurosci., June 1, 2005; 25(22): 5298 - 5304.
[Abstract] [Full Text] [PDF]

B. Schimmele, N. Grafe, and A. Pluckthun
Ribosome display of mammalian receptor domains
Protein Eng. Des. Sel., June 1, 2005; 18(6): 285 - 294.
[Abstract] [Full Text] [PDF]

D. A. Dodd, B. Niederoest, S. Bloechlinger, L. Dupuis, J.-P. Loeffler, and M. E. Schwab
Nogo-A, -B, and -C Are Found on the Cell Surface and Interact Together in Many Different Cell Types
J. Biol. Chem., April 1, 2005; 280(13): 12494 - 12502.
[Abstract] [Full Text] [PDF]

K. Venkatesh, O. Chivatakarn, H. Lee, P. S. Joshi, D. B. Kantor, B. A. Newman, R. Mage, C. Rader, and R. J. Giger
The Nogo-66 Receptor Homolog NgR2 Is a Sialic Acid-Dependent Receptor Selective for Myelin-Associated Glycoprotein
J. Neurosci., January 26, 2005; 25(4): 808 - 822.
[Abstract] [Full Text] [PDF]

B. Zheng, J. Atwal, C. Ho, L. Case, X.-l. He, K. C. Garcia, O. Steward, and M. Tessier-Lavigne
From the Cover: Genetic deletion of the Nogo receptor does not reduce neurite inhibition in vitro or promote corticospinal tract regeneration in vivo
PNAS, January 25, 2005; 102(4): 1205 - 1210.
[Abstract] [Full Text] [PDF]

P. Fontoura, P. P. Ho, J. DeVoss, B. Zheng, B. J. Lee, B. A. Kidd, H. Garren, R. A. Sobel, W. H. Robinson, M. Tessier-Lavigne, et al.
Immunity to the Extracellular Domain of Nogo-A Modulates Experimental Autoimmune Encephalomyelitis
J. Immunol., December 1, 2004; 173(11): 6981 - 6992.
[Abstract] [Full Text] [PDF]

S. Li, B. P. Liu, S. Budel, M. Li, B. Ji, L. Walus, W. Li, A. Jirik, S. Rabacchi, E. Choi, et al.
Blockade of Nogo-66, Myelin-Associated Glycoprotein, and Oligodendrocyte Myelin Glycoprotein by Soluble Nogo-66 Receptor Promotes Axonal Sprouting and Recovery after Spinal Injury
J. Neurosci., November 17, 2004; 24(46): 10511 - 10520.
[Abstract] [Full Text] [PDF]

W. Li, L. Walus, S. A. Rabacchi, A. Jirik, E. Chang, J. Schauer, B. H. Zheng, N. J. Benedetti, B. P. Liu, E. Choi, et al.
A Neutralizing Anti-Nogo66 Receptor Monoclonal Antibody Reverses Inhibition of Neurite Outgrowth by Central Nervous System Myelin
J. Biol. Chem., October 15, 2004; 279(42): 43780 - 43788.
[Abstract] [Full Text] [PDF]