The Membrane-anchoring Domain of Epidermal Growth Factor Receptor Ligands Dictates Their Ability to Operate in Juxtacrine Mode

Jianying Dong^*, Lee K. Opresko, William Chrisler, Galya Orr, Ryan D. Quesenberry, Douglas A. Lauffenburger, and H. Steven Wiley

^* Department of Pathology, Division of Cell Biology and Immunology, University of Utah, Salt Lake City, UT 84133; Biological Sciences Division, Pacific Northwest National Laboratory, Richland, WA 99352; and Biological Engineering Division, Massachusetts Institute of Technology, Cambridge, MA 02139

Submitted November 16, 2004; Revised March 30, 2005; Accepted March 31, 2005
Monitoring Editor: Carl-Henrik Heldin

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

All ligands of the epidermal growth factor (EGF) receptor (EGFR)are synthesized as membrane-anchored precursors. Previous workhas suggested that some ligands, such as EGF, must be proteolyticallyreleased to be active, whereas others, such as heparin-bindingEGF-like growth factor (HB-EGF) can function while still anchoredto the membrane (i.e., juxtacrine signaling). To explore thestructural basis for these differences in ligand activity, weengineered a series of membrane-anchored ligands in which thecore, receptor-binding domain of EGF was combined with differentdomains of both EGF and HB-EGF. We found that ligands havingthe N-terminal extension of EGF could not bind to the EGFR,even when released from the membrane. Ligands lacking an N-terminalextension, but possessing the membrane-anchoring domain of EGF,still required proteolytic release for activity, whereas ligandswith the membrane-anchoring domain of HB-EGF could elicit fullbiological activity while still membrane anchored. Ligands containingthe HB-EGF membrane anchor, but lacking an N-terminal extension,activated EGFR during their transit through the Golgi apparatus.However, cell-mixing experiments and fluorescence resonanceenergy transfer studies showed that juxtacrine signaling typicallyoccurred in trans at the cell surface, at points of cell-cellcontact. Our data suggest that the membrane-anchoring domainof ligands selectively controls their ability to participatein juxtacrine signaling and thus, only a subclass of EGFR ligandscan act in a juxtacrine mode.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Epidermal growth factor (EGF) receptor (EGFR) signaling pathwaysplay important roles in a variety of cellular functions, includingproliferation, differentiation, migration, and apoptosis (Wells,1999). EGFR signaling is initiated by the binding of one ofat least seven ligands, including EGF (Carpenter and Cohen,1990), transforming growth factor- ${alpha}$ (TGF ${alpha}$ ) (Derynck, 1992), heparin-bindingEGF-like growth factor (HB-EGF) (Higashiyama et al., 1991),amphiregulin (Shoyab et al., 1989), betacellulin (Shing et al.,1993) epiregulin (Toyoda et al., 1995), and epigen (Strachanet al., 2001). Soluble EGFR ligands are produced through extracellularcleavage of integral membrane precursor proteins, which consistof an EGF motif flanked by an N-terminal extension and a C-terminalmembrane-anchoring domain (Massague and Pandiella, 1993; Harriset al., 2003). There is no obvious homology in the predictedcleavage sites among the different EGFR ligands, although manystudies have shown that metalloprotease activity is requiredfor their release (Arribas et al., 1996; Brown et al., 1998;Dempsey et al., 1997; Sunnarborg et al., 2002; Hinkle et al.,2004).

TNF alpha converting enzyme (TACE), also known as ADAM 17, isprobably responsible for cleaving TGF ${alpha}$ , because TACE -/- cellsshowed a 95% reduction in TGF ${alpha}$ release (Black et al., 1997; Peschonet al., 1998). TACE also has been implicated in the cleavageof amphiregulin and HB-EGF (Sunnarborg et al., 2002). ADAM 10and ADAM 12 also have been implicated in HB-EGF shedding fromcells (Asakura et al., 2002; Yan et al., 2002). Substantialevidence indicates that proteolytic release of EGFR ligandsis a regulated process, which can be influenced by protein kinaseC (PKC) activity (Brown et al., 1998; Pandiella and Massague,1991a; Raab et al., 1994), calcium influx, and phosphatase activity(Pandiella and Massague, 1991b; Dethlefsen et al., 1998; Vecchiet al., 1998).

Release of EGFR ligands seems to be an important regulatorystep in activating the receptor. Mice lacking TACE showed aphenotype similar to that of EGFR -/- mice, probably becauseof defective processing of TGF ${alpha}$ and other EGFR ligands (Peschonet al., 1998). Blocking EGF and TGF ${alpha}$ release also inhibits growthand migration of EGFR-dependent cell lines (Dong et al., 1999).In addition, processing of Spitz, a Drosophila TGF ${alpha}$ homologue,is a limiting step in the activation of the Drosophila EGFR(Sibilia and Wagner, 1995; Hansen et al., 1997). Transactivationof the EGFR by a variety of different factors, such as insulin-likegrowth factor 1 and tumor necrosis factor- ${alpha}$ , also seem to dependon the proteolytic release of ligands such as amphiregulin,TGF ${alpha}$ , and HB-EGF (Gschwind et al., 2003; Chen et al., 2004; El-Shewyet al., 2004). These data suggest that EGFR ligands are onlybiologically active when they are released. However, a few studieshave shown that TGF ${alpha}$ , HB-EGF, amphiregulin, and betacellulincan act as juxtacrine factors (Wong et al., 1989; Anklesariaet al., 1990; Higashiyama et al., 1995; Inui et al., 1997; Tadaet al., 1999) and can induce tyrosine phosphorylation of EGFRexpressed on juxtaposed cells without the release of detectableligand. The reason for these disparate results is currentlyunresolved.

There could be numerous reasons why different laboratories havereached divergent opinions regarding the requirement for proteolyticrelease for ligand activation. One reason could be that theactivity of soluble versus juxtacrine ligands differs in theirmagnitude. Studies comparing the potencies of isolated solubleand membrane-bound forms of HB-EGF have shown that the precursorform has $~$ 10–25% of the activity of the secreted form instimulating cell proliferation (Ono et al., 1994). Thus, whenlow levels of ligand are expressed by cells, only soluble signalingmight be observed. The HB-EGF precursor, however, seems to havedistinct activities with regard to cell growth and apoptosis(Takemura et al., 1997; Iwamoto et al., 1999; Singh et al.,2004). This suggests that membrane-anchored ligands activatedifferent sets of signaling pathways in cells and argues againstthere only being a simple qualitative difference between thetwo signaling modes.

Another possible reason for the different results on the requirementfor ligand shedding might be the need for coexpression of accessoryproteins, such as CD9. These molecules seem to be crucial forthe juxtacrine activity of HB-EGF and TGF ${alpha}$ (Goishi et al., 1995;Higashiyama et al., 1995; Nakamura et al., 1995; Miyoshi etal., 1997; Shi et al., 2000). Accessory proteins could be requiredto remove a steric constraint imposed by another structuralfeature of the ligand, such as the heparin-binding domain (Takazakiet al., 2004). Alternatively, the accessory protein could berequired to "present" the ligand to the receptor by formingpart of a multiprotein complex, analogous to the formation ofantigen–major histocompatibility complex (MHC) complexeswith the T-cell receptor in lymphocytes (Cambier, 1992). Ifthis is the case, then the ability to form a juxtacrine complexcould be highly cell type dependent, requiring the expressionof a discrete set of proteins in either the ligand-expressingor receptor-bearing cell.

We have previously shown that the biological activity of membrane-anchoredEGF constructs has an absolute requirement for proteolytic release(Dong et al., 1999). These constructs consisted of the corereceptor binding and the membrane-anchoring domains of EGF,but lacked the amino-terminal extension of the native ligand.The absence of juxtacrine signaling by these engineered ligandscould have been due to the absence of an amino-terminal extensionthat would facilitate formation of a juxtacrine complex. Alternatively,the membrane-anchoring domain of EGF might have prevented juxtacrinesignaling. Although the core EGF structure of different EGFRligands is very homologous and induces almost identical biochemicalresponses, the membrane-anchoring domain is distinct. Mutationalstudies with TGF ${alpha}$ , HB-EGF and betacellulin suggest that the juxtamembranestructure dictates the cleavage process and that the cytoplasmictail regulates ligand trafficking (Dempsey and Coffey, 1994;Arribas et al., 1997; Briley et al., 1997; Dethlefsen et al.,1998; Hinkle et al., 2004). It seemed possible that the membraneanchor also could restrict a ligand's ability to act in a juxtacrinemanner.

To determine whether specific structural domains of EGFR ligandsdictate their ability to act in a juxtacrine mode, we createda series of artificial ligand chimeras and expressed them inEGF-responsive cells. We found that the biological activityof EGF required both the removal of its amino-terminal extensionand its proteolytic release from the cell surface. However,when EGF was tethered on the cell surface by the membrane-anchoringdomain of HB-EGF, it was able to participate in efficient juxtacrinesignaling. This indicates that the membrane-anchoring domainof EGFR ligands controls their ability to act as either solubleor juxtacrine ligands.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Reagents and Antibodies
Batimastat was kindly provided by British Biotech Pharmaceuticals(Oxford, United Kingdom). All fluorescently labeled antibodieswere from Molecular Probes (Eugene, OR). Anti-EGFR 225 monoclonalantibody (mAb) was isolated from a hybridoma cell line obtainedfrom the American Type Culture Collection (Manassas, VA). Anti-EGFR13A9 mAb was a gift from Genentech (South San Francisco, CA).Anti-phosphotyrosine (RC-20) horseradish peroxidase conjugate,anti-EGFR antibody (C-13), and goat anti-mouse IgG horseradishperoxidase conjugate were from BD Biosciences (San Jose, CA).Sheep antibodies were generated against a phosphopeptide correspondingto the major tyrosine-phosphorylation site of the EGFR (anti-EGFR-1173P)as described previously (Burke et al., 2001). Anti-FLAG mAbM2 was purchased from Sigma-Aldrich (St. Louis, MO). Monoclonalantibodies directed against human EGF (HA, LB, and LC) wereisolated from hybridoma cell lines (Yoshitake and Nishikawa,1988). The HA mAb was directly labeled with Alexa dye 594 accordingto the manufacturer's instructions (Molecular Probes). Fab fragmentsof LC and 13A9 were generated using immobilized papain (PierceChemical, Rockford. IL) and separated from undigested wholeIgG and Fc by using a protein A column. The Fab fragments werelabeled with Alexa dye 546 and Alexa dye 647, for LC and 13A9,respectively. The degree of labeling was 1.6–2.0 mol/molFab. Endoglycosidase H (Endo H) was purchased from Roche Diagnostics(Indianapolis, IN), and neuraminidase was from Calbiochem-Novabiochem(La Jolla, CA).

Construction of Cell Lines and Ligand Chimeras
The B82L cell line expressing the first plasmid (pUHD 15.1.neo)of the two-plasmid tetracycline-controlled (Tet-off) mammalianexpression system has been described previously (Will et al.,1995). They were selected and grown in DMEM containing 10% dialyzedcalf serum, 1 µM methotrexate, and 600 µg/ml G418(Geneticin). Construction and expression of sEGF and EGF-ctin the second plasmid of the Tet-off system (pUHD 13-3) alsohas been described previously (Will et al., 1995; Wiley et al.,1998).

The full-length EGF precursor in vector pCB6-pEGF was obtainedfrom Barbara Mroczkowski (Agouron Pharmaceutics, San Diego,CA). The pEGF was excised with SmaI and ClaI and subcloned intopBluescript KS cut with HincII and ClaI. The pEGF was excisedfrom pBluescript by cutting with XhoI, endfilling, and cuttingwith SacII. This fragment was then inserted into pUHD 13-3,which was first digested with BamHI and endfilled before cuttingwith SacII. The secreted form of the EGF precursor (At-EGF)was made by inserting a stop codon following Arg¹⁰²³ of theprecursor. This corresponds to the carboxy terminus of the matureEGF peptide. The stop codon was generated by PCR mutagenesis.This construct was inserted into pUHD 13-3 as described abovefor pEGF. Ligands EGF-ctF (EGF with the membrane-anchoring regionfrom EGF and FLAG epitope) and EGF-hcF (EGF with the membrane-anchoringregion from HB-EGF and FLAG epitope) were constructed as describedpreviously (Dong and Wiley, 2000). These constructs are shownschematically in Figure 1.

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Figure 1. Natural and artificial EGFR ligands. Shown at the top is native epidermal growth factor (pEGF) followed by the different EGF molecules used in this study. TM includes the transmembrane and juxtamembrane regions, whereas the membrane-anchoring domain includes both the TM region and the cytoplasmic domain. Note that EGF-hcF and EGF-hc contain the membrane-anchoring domain of HB-EGF (shown at the bottom) but have the same receptor-binding core and signal sequence of EGF-ctF.

The human mammary epithelial cell (HMEC) lines HB2 (Berdichevskyet al., 1994

) and 184A1 (Stampfer and Yaswen, 1993

) were obtainedfrom Joyce Taylor-Papadimitriou (Imperial Cancer Research, London,United Kingdom) and Martha Stampfer (Lawrence Berkley NationalLaboratory, University of California, Berkeley, Berkeley, CA),respectively. HB2 clones expressing EGF-ctF and EGF-hcF wereisolated as described previously (Dong and Wiley, 2000

). 184A1clones expressing EGF-ctF and EGF-hcF were derived in the sameway using a retrovirus-based strategy. HB2 clones were culturedDMEM supplemented with 10% cosmic calf serum (Hyclone Laboratories,Logan, UT), 5 µg/ml insulin, and 5 µg/ml dexamethasone.A1 clones were maintained in DFCI-1 medium (Band and Sager,1989

). All experiments were performed using clones before passage30.

B82L mouse cell lines expressing EGF-ctF and EGF-hcF also weremade using the retrovirus-based strategy described previously(Dong and Wiley, 2000). They were maintained in DMEM containing10% calf serum. The B82L clonal lines expressing EGFR were grownin DMEM containing 10% dialyzed calf serum and 1 µM methotrexate.

Wild-type Chinese hamster ovary (CHO) cells (R-) and cells expressingthe EGFR (R+) were a kind gift of Dr. Gordon Gill (Universityof California, San Diego) and were used to express both EGF-ctand EGF-hc. The cells were grown in ${alpha}$ -minimal essential medium:Ham's F-12 containing 5% fetal bovine serum and 5% defined supplementedcalf serum (Hyclone Laboratories). The cells were transfectedwith LipofectAMINE reagent (Invitrogen, Carlsbad, CA) at a rateof 5 µl reagent/2 µg DNA/35-mm plate of cells. Thetransfection was carried out for 3 h after which time the cellswere propagated for 2 d. The cells were split 1:20 and placedinto selective medium containing 10 µg/ml puromycin. Individualclones were isolated through limiting dilution and were periodicallysubjected to fluorescence-activated cell sorting analysis. Cellpopulations were sorted when the level of expression droppedbelow 70%. All transfected cells were maintained in selectivemedium.

EGFR Phosphorylation Analysis
Confluent cells were extracted using RIPA buffer (1% NP-40,0.5% sodium deoxycholate, 0.1% SDS, 50 mM Tris, pH 7.2, 150mM NaCl, and 0.02% sodium azide). Equal amounts of protein fromeach sample were separated on a 7.5% SDS polyacrylamide geland subsequently transferred to a nitrocellulose membrane (Bio-Rad,Hercules, CA). Phosphotyrosine and EGFR levels were determinedon Western blots by using horseradish peroxidase directly labeledanti-phosphotyrosine RC-20, or anti-EGFR mAb C-13 followed bygoat anti-mouse IgG horseradish peroxidase conjugate, respectively.

EGF Immunoprecipitations
To identify the different forms of EGF, cells were grown toconfluence in 60-mm dishes in the absence of tetracycline tofully induce ligand expression. Cells were changed to cysteineand methionine-free medium for 30 min and then changed to thesame medium containing 0.5 mCi/ml Tran³⁵ S-Label (MP Biomedicals,Irvine, CA) for 2 h at 37°C. The cells were rinsed and lysedand scraped from plates in 1 ml of 25 mM Tris, pH 8.0, 0.5%NP-40, 0.5% sodium deoxycholate, and 150 mM NaCl. Debris wasremoved by centrifugation at 15,000 x g for 10 min. Anti-EGFmAb HA (6 µg) was added to each tube followed by an overnightincubation at 4°C. Immunoprecipitates were isolated usinganti-mouse rabbit IgG and protein A-Sepharose. Samples wereboiled in SDS and run on 5–15% gradient SDS polyacrylamidegels, transferred to nitrocellulose, and exposed to film.

For the coimmunoprecipitation studies, proteins were isolatedin extraction buffer (1% Triton X-100, 50 mM HEPES, pH 7.0,150 mM NaCl, 10% glycerol, 1 mM EGTA, and 0.02% sodium azide).Equal amounts of protein from each sample were immunoprecipitatedwith 5 µg/ml M2 anti-FLAG mAb for 0.5 h and then with10 µg/ml rabbit anti-mouse IgG and 50 µl/ml 50%protein A-Sepharose for 1.5 h. Immunoprecipitates were washedtwice with the extraction buffer, separated on a 7.5% SDS polyacrylamidegel, and transferred to a nitrocellulose membrane. The membranewas probed with horseradish peroxidase (HRP)-conjugated anti-phosphotyrosineRC-20 antibody followed by chemiluminescence detection. Afterincubating with the stripping buffer (2% SDS, 100 mM 2-mercaptoethanol,and 6.25 mM Tris-HCl, pH 6.8) for 30 min at 50°C, the blotswere reprobed with anti-EGFR C-13 antibody, followed by HRP-labeledgoat anti-mouse IgG. Blots again were developed by the enhancedchemiluminescence reaction.

Immunofluorescence
Cells were plated on fibronectin-coated coverslips for 48 hin media lacking EGF. They were rinsed in ice-cold saline andfixed with 3.6% paraformaldehyde and 0.024% saponin, freshlyprepared in phosphate-buffered saline (PBS) as described previously(Wiley et al., 1998). Cells were incubated with 3.5 µg/mlaffinity-purified sheep anti-EGFR-1173P antibody for 1 h followedby staining with 1 µg/ml Alexa 594-labeled mAb HA, 5 µg/mlAlexa 488-labeled affinity-purified donkey anti-sheep IgG for45 min. After rinsing, the coverslips were mounted in 40 µlof Prolong mounting medium (Molecular Probes). Images were capturedseparately at 520 nm (Alexa 488) and 610 nm (Alexa 594) andcorrected for background. Composite images were assembled inAdobe Photoshop. The lack of cross-reactivity of the Alexa 488-labeledaffinity-purified donkey anti-sheep IgG for HA mAb was verifiedexperimentally.

For confocal microscopy, cells were grown on coverslips andtreated with 10 µM AG 1517 for 1 h to block activity ofthe EGFR and to prevent receptor desensitization. The cellswere then rinsed and incubated with fresh medium at 37°Cand incubated a further 15 min before fixation as describedabove. Activated EGFR were imaged using affinity-purified sheepanti-1173P (see above), and the ligand chimera was visualizedusing anti-FLAG antibody M2 directly labeled with Alexa 488.We have previously shown that anti-EGF and anti-FLAG antibodiesshow identical staining patterns in chimera-expressing cells(Dong and Wiley, 2000). Samples were analyzed using a LeicaDMIRE2 confocal microscope using a 100x Plan Apo oil immersionobjective. Control cells that did not express the ligand chimeraswere used to verify that there was no significant staining ofeither activated EGFR or the FLAG epitope tag.

Fluorescence Resonance Energy Transfer (FRET)
Cells were incubated simultaneously with 20–40 nM labeledFabs for 10 min at room temperature. Alexa 546 (LC), servingas the donor, and Alexa 647 (13A9), serving as the acceptorof energy, were excited by 532-nm laser (Nd:YAG Verdi V-10,Coherent, Santa Clara, CA), and 632 nm laser (dye laser CR-599;Coherent), respectively, by using a dual-dichroic mirror (ChromaTechnology, Brattleboro, VT). Donor and acceptor emissions weresent simultaneously onto two defined areas on a charge-coupleddevice (CCD) camera, while toggling between the two lasers.The green and red emissions were separated using a dichroicwedge mirror (Chroma Technology). FRET was detected by Alexa647 indirect excitation with 532 nm, as the energy was transferredfrom the excited Alexa 546.

The intensities in the acceptor and FRET channels were usedto define a cut-off value, and signals that overlapped in thetwo channels were further pursued for analysis. The bleed throughof the donor (10%) and the acceptor (7%) into the FRET (red)channel was determined empirically and was subtracted pixelby pixel, to obtain the true FRET signal (Fc):

(1)
where FRET, DONOR, and ACCEPTOR are the fluorescence intensitiesin the corresponding channels. FRET efficiency (E) was thencalculated pixel by pixel according to equation 2, where ${gamma}$ isthe acceptor to donor ratio of the quantum yields of the fluorophores,the objective, and the CCD camera, and equals 0.82.

(2)

Proliferation Assays
Cells were split at 1:10 into 12-well plates. The next day,cells were changed to control growth medium or medium containing10 µg/ml 225, 10 µM batimastat, 2.7 µM LBmAb, or 4.7 µM LC mAb. Medium was changed every otherday. Cells were counted using a Coulter counter.

Glycosidase Treatments
EGF-ctF and EGF-hcF cells were lysed in RIPA buffer, and theEGFR was immunoprecipitated from the cell lysates with anti-EGFRmAb 225, rabbit anti-mouse IgG, and protein A-Sepharose. Immunoprecipitateswere suspended in 50 µl of Endo H buffer (3.6 mM Na₂HPO₄/NaH₂PO₄buffer, pH 5.5, 0.05% SDS, 4 µg/ml phenylmethylsulfonylfluoride, and 70 mM ${beta}$ -mercaptoethanol) and boiled for 5 min.After centrifugation at 3000 rpm for 3 min, the supernatantwas incubated with 5 mU Endo H for 4 h at 37°C. For neuraminidasetreatment, the immunoprecipitates were incubated with 50 µlof neuraminidase (1 U/ml) for 30 min at 37°C.

Juxtacrine Activity Assay
B82 cells transfected with or without the gene for human EGFRwere transduced either with or without retrovirus containingthe EGF-hcF gene. This yielded cells expressing EGFR alone (R+),ligand alone (L+), or both ligand and receptor (R+L+). Beforethe experiment, cells were first evaluated for receptor numberand rate of ligand production. Pure populations of cells (R+or R+L+) or mixtures of cells (R+/L+) were plated into 100-mmplates such that the number of EGFR (cells x receptors per cell)on each plate was equal. The numbers of ligand producing cellsin the mixed cell population were adjusted to equal ligand productionby the R+L+ cells. Thus, each plate contained equal numbersof EGFR and ligand production despite varying cell number. However,cell number was always within a factor of 2. Two hours afterplating, the medium was replaced with medium containing no additives(control), 10 µg/ml 225 mAb, 50 ng/ml EGF, or 10 µMbatimastat; incubated for an additional 16 h; and washed withPBS. Cells were then extracted with 1 ml of RIPA buffer containing10 mM NaF, 1 mM sodium orthovanadate, and 1 µg/ml eachof pepstatin, chymostatin, aprotinin, and leupeptin. After centrifugation,the EGFR was immunoprecipitated from the clarified supernatantas described above, and the relative amount of activated receptorwas determined by Western blot analysis.

When using mixtures of CHO cells, equal numbers of receptor-positiveand chimera-expressing cells were plated onto 60-mm dishes andallowed to attach for 4 h. The medium was then changed to mediumcontaining 3 nM AG 1517 (Calbiochem-Novabiochem) and either10 µM batimastat, 10 µg/ml 225 antibody, or 20 µg/mlLC antibody. The cells were incubated overnight and brieflyrinsed before the addition of the identical media lacking AG1517.Samples were collected after 2 h by lysing the cells in 1% NP-40buffer containing 1 mM sodium orthovanadate and then placingsamples containing equal amounts of protein on 4–12% gradientbis-Tris polyacrylamide gels. After electrophoresis and Westernblotting, the nitrocellulose membranes were probed with anti-phospho1173 EGFR antibody and then stripped and probed for total receptormass by using anti-EGFR ab SC-03 (Santa Cruz Biotechnology,Santa Cruz, CA).

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

The N-terminal Domain of EGF Inhibits Its Activity
We have previously shown that membrane-anchored EGF-ct mustbe proteolytically released to have biological activity (Donget al., 1999). Additional studies have suggested that otherEGFR ligands also must be released to be active (Peschon etal., 1998; Prenzel et al., 1999). Studies by some investigators,however, have indicated that ligands such as HB-EGF can be biologicallyactive while still membrane associated (Goishi et al., 1995;Inui et al., 1997; Takemura et al., 1997, 1999). A major differencebetween our studies and those of other investigators was thatwe were using ligands that lack the domain N terminal of thecore receptor binding domain. To determine whether the N-terminaldomain of EGF could facilitate its ability to act in a juxtacrinemode, we expressed the full-length EGF precursor (pEGF) as wellas three different "preprocessed'' forms of EGF in B82 cellsunder control of the tetracycline-repressible expression system.As shown in Figure 1, At-EGF (Amino-terminus EGF) lacks themembrane-anchoring domain and corresponds to the high-molecular-weightform of EGF isolated from human breast milk and urine (Mroczkowskiand Reich, 1993); EGF-ct (EGF with carboxy terminus) lacks theentire prepro region of At-EGF, as does the mature EGF peptide,but it retains the membrane-anchoring domain; sEGF (secretedEGF) corresponds to the mature EGF peptide with the additionof a signal peptide to allow export from cells. All four formsof EGF were expressed in B82 cells that also were stably transfectedwith human EGFR so that the activity of these constructs couldbe evaluated.

EGF was immunoprecipitated from cells expressing the differentconstructs after induction and metabolic labeling. As shownin Figure 2A, the At-EGF and pEGF forms expressed by cells were $~$ 160–180 kDa, indicating that they were fully glycosylated.Only a single, high-molecular-weight product was observed incells expressing pEGF. Immunoprecipitation of the conditionedmedium showed that cells expressing sEGF and EGF-ct produceda very similar 7-kDa product, whereas cells producing eitherpEGF or At-EGF secreted the same 160-kDa product (our unpublisheddata). Thus, B82 cells are very efficient in cleaving EGF atthe juxtamembrane site, but they seem to be unable to processthe N-terminal domain of the molecule.

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Figure 2. Expression and activity of different forms of epidermal growth factor. (A) B82 cells expressing the indicated constructs were incubated with Tran³⁵ S label for 2 h and rinsed and lysed as described in Materials and Methods. After immunoprecipitation, the EGFs were separated on a 5–15% gradient denaturing gel. After transfer of the proteins to nitrocellulose, they were visualized by autoradiography. The sample in each lane was normalized to the amount of protein in the original cell extract. (B) B82 cells expressing both the human EGFR and the indicated construct in a Tet-off vector were induced by withdrawal of tetracycline overnight. The parental cells (lacking a ligand vector) were incubated with 25 nM EGF overnight. Cells were extracted and the relative amount of phosphotyrosine associated with the EGFR was determined by a ratiometric ELISA as described in Materials and Methods. All samples were done in triplicate and diluted to keep the ELISA readings within the linear range. Expression of the ligand constructs was verified by nuclease protection assays of parallel plates.

To determine the biological activity of the different EGF constructs,we evaluated EGFR activation after induction of ligand expressionby using a ratiometric tyrosine phosphorylation assay (Schoolerand Wiley, 2000

). As shown in Figure 2B, addition of EGF tothe parental (ligand negative) cells resulted in a large increasein the Tyr(P):EGFR ratio. A similar increase was observed afterinduction of sEGF or EGF-ct expression. The lower absolute levelof tyrosine phosphorylation in cells expressing sEGF or EGF-ctis probably due to chronic stimulation of the cell caused bya low level of ligand production even in the Tet-off state (Willet al., 1995

). Significantly, we failed to observe any EGFRactivation after induction of either At-EGF or pEGF expression.This was not due to low ligand expression in the induced statebecause the amount of pEGF and At-EGF in the medium was 240and 500 ng/ml, respectively, as determined by enzyme-linkedimmunosorbent assay (ELISA). This corresponds to 8 and 16 ng/mlmature EGF. Although this is somewhat less than the amount producedby cells expressing sEGF or EGF-ct, it is $~$ 10-fold higher thanthe K_d of the EGF receptor. We also examined four separate clonesof cells expressing At-EGF. We were unable to detect any significantchange in either EGFR phosphorylation or down-regulation afterAt-EGF induction (our unpublished data). This indicates thatrather than facilitating the ability of EGF to interact withits receptor, the N-terminal domain inhibits receptor binding.

Role of the Membrane-anchoring Domain in Regulating Ligand–Receptor Interactions
The inability of membrane-anchored pEGF to stimulate EGFR activationis very similar to the lack of EGF-ct activity observed whenits cleavage is blocked by batimastat (Dong et al., 1999). Thus,in contrast to HB-EGF, it seems that all membrane-anchored formsof EGF are incapable of juxtacrine signaling. One possible explanationfor the lack of observable juxtacrine activity for EGF-ct isthat its membrane-anchoring domain restricts its ability toengage in this signaling mode. The membrane-anchoring domainsof EGF-like ligands are structurally diverse and have alreadybeen shown to control the rate of regulated proteolysis (Hinkleet al., 2004). Thus, it seemed reasonable that this domain alsocould dictate the interactions of membrane-anchored ligandswith the EGFR. To explore this idea, we created an EGF chimerathat was tethered to the cell surface by the membrane-anchoringdomain of HB-EGF, a ligand that has been shown to engage injuxtacrine signaling (Nakamura, 1995). Cells were engineeredto express either of two chimeric ligands: EGF-ctF or EGF-hcF.These ligands have the receptor-binding domain of EGF and themembrane-anchoring domains from EGF and HB-EGF, respectively.They also have a FLAG epitope fused to the carboxy terminusof the ligand (Figure 1). We have previously characterized theseligands and found that their distribution and shedding ratesmimicked the ligand parent that contributed the membrane-anchoringdomain (Dong and Wiley, 2000).

We first examined the expression and rate of release of EGF-ctFand EGF-hcF in HMECs. This cell type was used because of itsrobust biological response to EGFR activation (Stampfer et al.,1993). As shown in Figure 3A, the constitutive release of EGFfrom cells expressing EGF-ctF was significantly higher thanfrom cells expressing EGF-hcF. The metalloprotease inhibitorbatimastat inhibited the release of both ligands. These dataare consistent with previously published reports (Dempsey etal., 1997; Dong and Wiley, 2000).

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Figure 3. Expression and activity of EGF-hcF and EGF-ctF in mammary epithelial cells. (A) Cells expressing the indicated construct were solubilized, and EGF levels were determined by ELISA. To measure released EGF, cells were incubated with mAb 225 (133 nM) in combination with or without 10 µM batimastat (Bat) for 24 h before medium was harvested and assayed. Error bars represent SD of ELISA data. (B) Cells were split 1:10 into 12-well dishes. Eighteen hours later, cells were changed to medium containing 67 mM mAb 225 or 10 µM batimastat. Medium was changed every 2 d, and cells were counted on the indicated days. Data are average of duplicate plates of cells. The data are representative of those obtained from at least three separate clonal cell lines expressing the ligand chimeras.

As shown in Figure 3B, growth of cells expressing EGF-ctF wasstrongly inhibited by either blocking the EGFR with the antagonisticantibody 225 or by inhibiting ligand shedding with batimastat.This shows that proliferation of HMECs is dependent on the activationof the EGFR and shedding of either EGF-ctF or their endogenousligands. In cells expressing the EGF-hcF chimera (Figure 3C),blocking the EGFR with 225 antibody also blocked cell proliferation,showing that these cells retained their dependence on EGFR activation.However, batimastat treatment did not block proliferation ofthese cells. Its minor effect was consistent with its previouslydemonstrated effect on EGF-induced HMEC growth (Dong et al.,1999

). Because batimastat totally blocked release of EGF-hcF(Figure 3A), these data suggest that EGF-hcF could activatethe EGFR while still anchored to the membrane (i.e., througha juxtacrine mechanism).

To directly demonstrate the ability of membrane-anchored EGF-hcFto activate the EGFR, we examined EGFR phosphorylation by usingWestern blots. In addition, we used two distinct HMEC strains(184A1L5 and HB2) expressing EGF-hcF and EGF-ctF to make surethat the results were independent of cell type. Cells were treatedwith 225 antibody or batimastat for 24 h, and the EGFR was immunoprecipitatedand then analyzed on Western blots for phosphotyrosine content.As shown in Figure 4A, treating cells expressing either EGF-hcFor EGF-ctF with 225 antibody efficiently blocked EGFR phosphorylation.Significantly, batimastat strongly inhibited EGFR phosphorylationonly in cells expressing EGF-ctF, but it had little effect oncells expressing EGF-hcF, demonstrating that proteolytic releaseof EGF-hcF is not required for its activity.

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Figure 4. Differential inhibition of EGFR phosphorylation in EGF-hcF and EGF-ctF cells by batimastat. (A) Both 184A1 and HB2 clones expressing the indicated construct were analyzed. Cells were treated with 67 nM mAb 225 or 10 µM batimastat for 22 h. EGFR was immunoprecipitated and analyzed by Western blots by using an anti-phosphotyrosine HRP conjugate (RC20-HRP) or anti-EGFR antibody (C-13), followed by HRP-labeled goat anti-mouse IgG. (B) 184A1 cells expressing full-length HB-EGF or EGF-hcF were treated as described in A. The separating gel was a 4–12% gradient.

Although EGF-hcF contains the membrane-anchoring domain of HB-EGF,it lacks its N-terminal glycosylaminoglycan binding domains.To determine whether the juxtacrine activity of EGF-hcF wassimilar to native HB-EGF, we expressed full-length HB-EGF inHMEC 184 A1L5 cells by using retroviral transduction. Phosphorylationof the EGFR was evaluated in the presence or absence of either225 antibody or batimastat. As shown in Figure 4B, 225 antibodyblocked EGFR phosphorylation in cells expressing either HB-EGFor EGF-hc. Batimastat had a similar, minor effect on EGFR phosphorylationin cells expressing either ligand. This result suggests thatnative HB-EGF and the chimera have similar potential for juxtacrineactivity in HMEC and thus the N-terminal extension of HB-EGFis not a requirement.

If membrane-anchored EGF-hcF was directly binding to the EGFR,we should be able to coprecipitate the EGFR with anti-ligandantibodies. Because both EGF-ctF and EGF-hcF have a FLAG epitopeat their carboxy terminus, we used anti-FLAG antibodies in anattempt to isolate ligand–receptor complexes. Extractsof cells expressing either EGF-hcF or EGF-ctF were incubatedwith anti-FLAG antibody M2 or an anti-EGFR mAb. The immunoprecipitateswere separated on a 7.5% SDS polyacrylamide gel and immunoblottedfor phosphotyrosine and EGFR. As shown in Figure 5, phosphorylatedEGFR was effectively coimmunoprecipitated with anti-FLAG antibodyonly in the case of cells expressing EGF-hcF, although a faintband was sometimes observed in the case of EGF-ctF.

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Figure 5. Activated EGFR can be coimmunoprecipitated with full-length EGF-hcF. HB2 parental cells and cells expressing EGF-hcF or EGF-ctF were grown in 100-mm dishes to confluence and extracted in 1% Triton X-100 lysis buffer. Cell extracts were immunoprecipitated with anti-FLAG M2 (right three lanes) or anti-EGFR 13A9 mAb (left three lanes). The immunoprecipitates were analyzed on Western blots for phosphotyrosine (top) and then stripped and reprobed for the EGFR (middle). Alternately, the cells were first treated with the cross-linking agent disuccinimidyl suberate before extraction (bottom). In this case, only one-third of the anti-EGFR 13A9 mAb sample was loaded to facilitate band visualization.

The low efficiency of the coprecipitation indicated that theligand–receptor complexes were rare or unstable. Alternately,it seemed possible that the complexes between the receptor andthe ligands formed after cell solubilization. To explore thesedifferent hypotheses, we incubated cells with a cross-linkingagent before they were solubilized. Chemical cross-linkers onlywork efficiently on preformed protein complexes (Sorkin andCarpenter, 1991

). As shown in Figure 5 (bottom), the cross-linkersubstantially increased the amount of coprecipitated EGFR onlyin the case of EGF-hcF, demonstrating that this chimera formeda complex with the EGFR in intact cells. Because the amountof complexes between EGF-ctF and the EGFR were not enhancedby a cross-linker, they probably formed after cell solubilization.

Intracellular Binding and Activation of EGFR by EGF-hcF
During our studies of EGFR phosphorylation, we noticed thatthe molecular weight of EGFR in some cells expressing EGF-hcFwas significantly lower than that observed either in the parentalcells or in cells expressing EGF-ctF (Figure 5). This lowermolecular weight receptor was especially evident in the anti-Tyr(P)blots by using single-percentage gels (i.e., 7.5% acrylamide)and was independent of cell type (Figure 4A). In an attemptto determine the reason for the lower molecular weight form,we probed blots with antibodies against individual phosphorylationsites of the EGFR. No differences were seen between receptorsactivated by exogenous EGF, EGF-ctF, or EGF-hcF (our unpublisheddata). Likewise, anti-phosphoserine and anti-phosphothreonineantibodies did not reveal any differences (our unpublished data).The distribution of EGFR between the cell surface and intracellularcompartments also was indistinguishable between cells expressingthe different ligands. However, EGFR cells expressing EGF-hcFdisplayed sensitivity to endoglycosidase H treatment (Figure 6A),indicating that they were incompletely glycosylated.

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Figure 6. Differential glycosylation of EGFR in cells expressing EGF-ctF versus EGF-hcF. (A) The EGFR was immunoprecipitated from lysates of cells expressing either EGF-hcF (left three lanes) or EGF-ctF (right three lanes). The immunoprecipitates were treated with either endoglycosidase H or neuraminidase as described in Materials and Methods and analyzed by Western blots by using polyclonal anti-EGFR antibody SC-003. (B) Cells expressing the indicated ligand constructs were grown on coverslips, fixed, permeabilized, and stained with anti-EGF mAb (left) or affinity-purified antibodies against the major phosphorylation site in the EGFR (right) as described in Materials and Methods. Arrows indicate colocalization.

Terminal glycosylation of the EGFR takes place in the Golgiapparatus. The ability of the EGFR to bind to ligands, however,is gained before processing of the core oligosaccharides (Sliekerand Lane, 1985

). This suggested to us the possibility that EGF-hcF was binding to the immature EGFR in the Golgi apparatus,thus interfering with the synthesis of complex carbohydratechains. If this were the case, then we would expect to see activatedEGFR colocalized in the perinuclear region with EGF-hcF.

Cells expressing either EGF-ctF or EGF-hcF were fixed, and thedistribution of ligands was determined using an anti-EGF antibody.The distribution of activated EGFR was determined using an affinity-purifiedsheep antibody against the major phosphorylation site of theEGFR (Burke et al., 2001). As shown in Figure 6B, EGF-ctF wasdiffusely distributed on the cell surface and in small vesicles.Activated EGFR displayed a weak, diffuse pattern in those cells.In contrast, EGF-hcF was found in intracellular vesicles, aswe have described previously (Dong and Wiley, 2000). ActivatedEGFRs also were found concentrated in small vesicles in theperinuclear region of the cell (Figure 6B, arrows). Most ofthe intracellular, ligand-containing vesicles, however, didnot contain activated EGFR. These data indicate that EGF-hcFis able to form direct complexes with the receptor in some,but not all, intracellular vesicles. These data are also consistentwith EGF-hcF binding to the EGFR before its exit from the Golgiapparatus.

The images shown in Figure 6B were taken at a focal plane throughthe midpoint of the cell, to better image ligand–receptorcomplexes in the perinuclear region. When the focal plane waschanged to visualize the area of cell-cell contact, we noticedthat most activated receptors were not intracellular, but insteadcould be found at the plasma membrane at areas of contact (Figure 7,top). This was specific for the cells expressing EGF-hcF,but it did not correspond to an area of high receptor density.Confocal microscopy of cells expressing EGF-hcF confirmed thatareas of cell-cell contact generally displayed increased levelsof phosphorylated EGFR (Figure 7, bottom), suggesting that muchof the juxtacrine signaling at the cell surface occurred betweenopposing cells. In the case of cells expressing EGF-ctF, nosignificant anti-phosphotyrosine staining was observed at pointsof cell-cell contact (our unpublished data).

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Figure 7. Activated EGFR in cells expressing EGF-hcF are found at points of cell-cell contact. (A) Cells expressing EGF-hcF were fixed, permeabilized, and stained for both EGF (top) and tyrosine-phosphorylated EGFR as described in the legend for Figure 6B. The focal plane was adjusted to optimally visualize the area of cell-cell contact. (B) Cells were treated as described in A, but the immunofluorescence was by confocal microscopy. Shown is a group of four cells imaged through their midplane.

Juxtacrine Signaling Primarily Operates in Trans
The observed concentration of activated EGFR at areas of cell-cellcontact suggests that juxtacrine signaling operates as a mechanismto signal between cells in trans. The ability of EGF-hcF toform complexes within the Golgi apparatus suggests that juxtacrinesignaling could potentially operate within a cell in cis. Itis important to determine whether juxtacrine signaling normallyoperates in cis or trans because it defines the flow of informationwithin the system (either between cells or within a single cell).To investigate this issue, we expressed either EGF-ct or EGF-hcin Chinese hamster ovary (CHO) cells, which lack EGFR. We thenmixed these with CHO cells in which the EGFR was expressed asa transgene. As shown in Figure 8A, the EGFR was activated inthe mixed cell population and blocking the EGFR with 225 antibodyinhibited this activation. Interestingly, adding the anti-EGFantibody LC had little effect on receptor activation, indicatingthat this antibody does not interfere with receptor binding.Batimastat blocked signaling mediated by EGF-ct, but not EGF-hc,indicating that EGF-hc participated in efficient juxtacrinesignaling in this mixed cell system. Because the receptors andligands were on different cells, juxtacrine signaling seemsto operate in trans.

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Figure 8. Juxtacrine activation primarily operates in trans. (A) CHO cells expressing either EGF-ct (left) or the EGF-hc chimera (right) were mixed with an equal number of cells expressing the EGFR and allowed to plate for 2 h. The cells were then changed to fresh medium (Con) or together with 10 µM batimastat (Bat), 10 µg/ml 225 mAb (225), or 10 µg/ml LC mAb (LC). After 18 h, the cells were extracted, and the EGFR was immunoprecipitated and analyzed for phosphotyrosine (top) or EGFR content (bottom) as described in Materials and Methods. (B) Mouse B82L cells expressing either human EGFR alone (R+) or both receptor and EGF-hcF (R+L+) were plated alone. Alternately, R+ cells were mixed together with cells expressing EGF-hcF alone (R+/L+). The number of cells on each plate was adjusted so that the net receptor number and ligand production was the same. Two hours after plating, the medium was replaced with that containing 10 µg/ml 225 mAb or 10 µM batimastat. After 18 h, the cells were processed as described in A. Numbers under the Tyr(P) bands are their relative intensities (in arbitrary densitometric units). This blot is representative of three replicated experiments.

We confirmed these results by using B82 cells transfected eitherwith or without the human EGFR gene, yielding R+ and R-cells,respectively. These cells were then transduced with retroviruscontaining the ligand genes. As shown in Figure 8B, receptoractivation in cells expressing both receptors and ligands (R+L+)was essentially the same as observed in the mixed cell population(R+/L+). This is consistent with trans-juxtacrine signaling.Blocking the EGFR with mAb 225 inhibited ligand-induced receptoractivation in all cases. Adding batimastat increased receptoractivation, suggesting that the membrane-anchored growth factorwas the active species. These results suggest that althoughEGF-hc can form intracellular cis-juxtacrine complexes, themajority of receptor signaling is due to its action as a trans-juxtacrinegrowth factor.

The purpose of the experiment shown in Figure 8B was to comparecells expressing both ligand and receptors (R+L+) to those expressingeither ligands or receptors (R+/L+). To accomplish this, weadjusted the number of ligand-expressing cells in the R+/L+group to be equivalent to the R+L+ group. An intrinsic consequenceof this experimental design was nonequivalency in cell densitybecause the receptors and ligands were now on different cells.However, we found that varying cell density in the R+/L+ groupby a factor of five had little effect on the level of observedjuxtacrine signaling. To explore this puzzling observation,we visualized the interactions of the two cell types to determinewhether cell-cell contacts were proportional to cell density.Mixtures of live R+ and L+ cells were incubated with low levelsof fluorescently labeled mAb 13A9 and mAb LC to identify theR+ and L+ cells, respectively. We found that the presence ofL+ cells resulted in R+ cells forming extensive protrusionsand contacts with the L+ cells (Figure 9). Extensions from theR+ cells seemed to be attached to the surface of L+ cells, particularlyin the space between the cells and the culture dish (Figure 9F).In contrast, cells expressing both EGF-hcF and the EGFR(R+L+ cells) were more rounded and uniform in appearance (ourunpublished data; also see Figures 6B and 7). Thus, juxtacrinesignaling does not seem to be a passive process simply dependenton cell density but is instead a facilitated process in whichR+ cells make numerous contacts with the ligand-producing cells.

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Figure 9. Cells involved in juxtacrine signaling display extensive intercellular contacts. B82 cells expressing either the EGFR or EGF-hcF were mixed and incubated overnight in a Bioptechs coverslip dish for live cell imaging. Cells were incubated for 1 h at 37°C with 1 µg/ml anti-EGFR mAb 13A9 labeled with Alexa 488 (B, green, C and D) or anti-EGF mAb LC labeled with Alexa 594 (A, red, C and D). Arrows show areas of contact between R+ and L+ cells. Shown in E is a differential interference contrast image of D. (F) Outlined composite image of D.

The extensive contacts we observed between cells expressingEGF-hcF and EGFR suggest that juxtacrine complexes form betweenopposing cell surfaces. To directly test this idea, we usedfluorescence resonance energy transfer (FRET). By labeling mAbLC with Alexa 546 and the non-antagonistic anti-EGFR antibody13A9 with Alexa 647, complexes between membrane-anchored EGFand the EGFR should be indicated by a FRET signal. Neither LCnor 13A9 interferes with juxtacrine signaling (our unpublishedobservations; also see Figure 8A). We used Fab fragments ofboth antibodies to prevent antibody-induced aggregation andto reduce the potential of steric hindrance by bulky, full-sizedantibodies. Cells expressing either EGF-ct or EGF-hc were used.As shown in Figure 10, we did not observe any significant FRETsignal in cells expressing EGF-ct. In contrast, cells expressingEGF-hc displayed a robust FRET signal at points of cell-cellcontact. These results demonstrate that the membrane-anchoringdomain of HB-EGF, but not EGF, allows the formation of juxtacrinecomplexes between cells in trans.

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Figure 10. FRET between ligands and the EGFR in juxtacrine complexes. Cells expressing EGF-hcF chimeras show substantial FRET signals along cell-cell contacts, indicating molecular interactions between the chimera and EGFR. Typical images of donor, acceptor and FRET efficiency, taken from cells expressing EGF-ctF (top row) and EGF-hcF (bottom row) chimeras, are shown. The right column shows images of the chimeras, tagged with labeled antibodies against the extracellular domain of EGF. The center column shows images of EGFR, tagged with the antibody against the receptor. The left column shows images of FRET efficiency, calculated pixel by pixel (see Materials and Methods).

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

One of the most important aspects of receptor regulation iscontrol of receptor activation. Most studies have focused ondownstream signaling events, but few have focused on the controlof ligand availability, which is rate limiting for EGFR activation.This has been demonstrated by studies in which inhibition ofligand binding blocks most of the endogenous activity of EGFR(Stampfer et al., 1993; Dong et al., 1999). Although ligand-independentmechanisms of EGFR activation have been reported (reviewed inGschwind et al., 2001; Yan et al., 2002; Bill et al., 2004),the magnitude of their effect seems minor, at least in mammaryepithelium at steady state.

What regulates ligand availability? A series of recent reportssuggests that proteolytic processing is the primary regulatorfor a number of EGFR ligands (Peschon et al., 1998; Dong etal., 1999; Prenzel et al., 1999; Sunnarborg et al., 2002; Hinkleet al., 2004). However, there is strong evidence that HB-EGFdoes not require proteolytic release for activity. Instead,its ability to form a complex with accessory proteins, suchas CD9, seems to be crucial for its activity (Goishi et al.,1995; Higashiyama et al., 1995; Nakamura et al., 1995; Miyoshiet al., 1997). Accessory proteins could be required to removea steric constraint imposed by another structural feature ofthe ligand, such as the heparin-binding domain. Alternatively,the accessory protein could be required to "present" the ligandto the receptor by forming part of a multiprotein complex, analogousto the formation of antigen–MHC complexes with the T-cellreceptor in lymphocytes (Cambier, 1992).

By expressing EGF constructs that contained or lacked the preproextension in an inducible expression system, we found that removalof this domain was required for ligand activity. The lack ofactivity of 160-kDa EGF contradicts previous work by Parrieset al. (1995), but is consistent with results published by Dempseyet al. (1997). The difference between these studies is thatthe Parries study used purified 160-kDa EGF, whereas the Dempseystudy (and the current study) examined native 160-kDa EGF producedby cultured cells. It seems possible that the conditions usedto purify EGF from large quantities of urine could have resultedin partial denaturation of the precursor, leading to its abilityto bind to the EGFR. We could find no evidence that the 160-kDaEGF produced by cultured cells could bind or activate EGFR,and so removal of the prepro extension is probably necessaryfor its biological activity in situ.

It has previously been shown that membrane-anchored EGF or TGF ${alpha}$ also must be proteolytically released to have biological activity(Dong et al., 1999; Borrell-Pages et al., 2003). Our currentstudies confirm that EGF must be released to be active becausemembrane-anchored EGF could neither bind nor activate the EGFR.Our results are in contrast with previous studies with EGF andTGF ${alpha}$ (Brachmann et al., 1989; Mroczkowski et al., 1989). However,the endogenous metalloprotease activity of cells was not inhibitedin those studies. Instead, they used ligand mutants that werebelieved to be noncleavable (Brachmann et al., 1989; Wong etal., 1989). More recent evidence indicates that the cleavageof these mutants proceeds at a low but significant rate andthat assays to detect ligand release in the presence of EGFR-bearingcells are inaccurate unless the EGFR is blocked (Dempsey andCoffey, 1994; Dong et al., 1999). Thus, the observed EGFR activationcould have arisen from a small amount of released ligand.

In contrast to the results obtained with EGF or TGF ${alpha}$ , we foundthat a chimera between the membrane-anchoring domain of HB-EGFand the receptor-binding domain of EGF resulted in a moleculethat was fully active as a juxtacrine factor. Protease inhibitorscould no longer inhibit EGFR activation. Our ability to isolatea complex of EGFR and EGF-hcF directly demonstrates the formationof juxtacrine complexes by the chimera. Imaging studies usingfluorescently labeled Fab fragments against EGF and the receptordemonstrated FRET at points of cell-cell contact only in thecase of the HB-EGF chimera. Although full-length HB-EGF expressedin our cells also displayed juxtacrine activity, the activityof the chimera in the presence of metalloprotease inhibitorswas similar. Because the chimera lacks the domains of HB-EGFrequired for binding to accessory proteins such as CD9, themembrane-anchoring domain seems to be the critical juxtacrinedeterminant. Recent reports suggest that the heparin-bindingdomain of HB-EGF functions as a negative regulator of its activity(Takazaki et al., 2004). Our results cannot address this pointdirectly because the cells used to express native HB-EGF containhigh levels of CD9 and other cell surface proteins that havebeen reported to relieve the inhibitory activity of that domain(our unpublished observations).

It is not clear how the membrane-anchoring region of EGFR ligandsrestricts receptor access. The "stem" (juxtamembrane) domainbetween the last critical leucine in EGF (L47) and the membrane-spanningdomain of the ligand consist of only 18 and 15 hydrophilic residuesfor EGF-ctF and EGF-hcF, respectively. Both stems are predictedto assume bend configurations, but display no other obviousstructural motifs. However, the anchoring domain could positionthe core EGF domain in an appropriate orientation for bindingin the cleft between EGFR domains I and III or could directlyassociate with the receptor itself (Garrett et al., 2002). Themembrane-spanning domains also could affect the conformationof the stem. Alternately, ligand trafficking and localizationcould be determined by their membrane-anchoring domain (Dempseyand Coffey, 1994; Brown et al., 2001), and the chimeric ligandmay be localized to a compartment or domain of the cell surfacewhere the EGFR is accessible (Dong and Wiley, 2000). Finally,there may be accessory molecules associating with the two differentmembrane-anchoring domains that stabilize the association ofEGFR with EGF-hcF and/or prevent the association of EGFR withthe membrane-bound EGF-ctF. Further studies will be requiredto discriminate between these possibilities.

We noticed that when the EGFR was expressed in the same cellas the EGF-hcF chimera, it migrated at a lower molecular weighton denaturing gels, apparently because of incomplete glycosylation.The simplest explanation for this observation is that EGF-hcFligand binds to the EGFR during its transit through the Golgiapparatus, thereby interfering with processing of its complexcarbohydrates. Consistent with this explanation, we observedthat EGF-hcF and activated EGFR were colocalized in the perinuclearregion of cells. The incomplete glycosylation indicates thatmost if not all of the EGFR is interacting with EGF-hcF beforeit exits from the Golgi. What is not clear is the amount ofsignaling that arises from this interaction and its stability.The number and distribution of EGFR found in cells expressingEGF-hcF is not substantially different from that found in cellsexpressing EGF-ctF, suggesting that the "intracrine" interactionsdo not result in down-regulation of the receptor. In addition,we only see significant numbers of juxtacrine complexes at pointsof cell-cell contact. The simplest explanation for these observationsis that juxtacrine interactions require the receptor and membrane-anchoredligand be juxtaposed on facing membrane surfaces. Such a situationexists at both points of cell-cell contact and in the stacksof membranes found in the Golgi apparatus. When the receptorand ligand enter vesicles for transport to the cell surface,the juxtacrine complex could dissemble because of steric considerations.After delivery to cell surface, new juxtacrine complexes couldonly form at points of cell-cell contact.

The "intracrine signaling" we observe due to EGF-hcF expressionis probably due to the lack of a prepro domain in the ligandchimera. Indeed, we have never seen underglycosylation of theEGFR in cells expressing high levels of native HB-EGF (our unpublishedobservations). Under normal circumstances, prepro domains ofligands are removed, probably at the cell surface. Significantly,it has been shown that removing the prepro region of amphiregulinprevents its transport to the cell surface (Thorne and Plowman,1994). In addition, the normal removal of the prepro domainof HB-EGF has been shown to significantly enhance its juxtacrineactivity (Nakagawa et al., 1996). We therefore propose thatan important role of the prepro domain of EGFR ligands is toprevent binding of the ligands to receptors during their transportto the cell surface. The regulated removal of the prepro domainat the cell surface could restrict receptor activation to thatcompartment.

It seems that juxtacrine complexes can function as points ofcell adhesion. When we mixed cells expressing only EGFR withcells expressing only EGF-hcF, we observed the formation ofnumerous contacts between the two cell types. The presence ofcells expressing EGF-hcF induced the formation of extensiveprotrusions and ruffling in cells expressing EGFR (Figure 9),probably due to the constitutive release of small amounts ofEGF from the cells expressing EGF-hcF (Dong and Wiley, 2000).The contacts between the two cell types are probably due tothe formation of stable juxtacrine complexes because we wereable to detect FRET between ligand and receptors at these points(Figure 10). It has previously been shown that HB-EGF can actas a cell adhesion factor (Singh et al., 2004), but it is hasbeen unclear whether this was mediated by the heparin-bindingor receptor-binding domains of the molecule. Our results indicatethat the receptor binding domain itself can mediate cell adhesions.

Our data are consistent with a model in which there are twodistinct steps that regulate ligand access to the EGFR. Thefirst step involves the maintenance of the prepro domain duringligand transport to the cell surface. The retention of thisstructural element is probably necessary to prevent intracrinesignaling and unregulated cell proliferation (Wiley et al.,1998). The second step involves either the proteolytic releaseof the membrane-anchored ligand or the formation of a juxtacrinecomplex with neighboring cells. The ability of any given ligandto form a juxtacrine complex would require the appropriate membrane-anchoringdomain and the presence of auxiliary proteins, such as the tetraspaninCD9. In this model, ligand activation is a highly regulatedprocess that depends on the involvement of a number of distinctmolecules and processing events. The multiple steps requiredfor activation probably serve as important control points ofregulation for cell proliferation and differentiation. Furtherinvestigation into the coordination of these processes shouldreveal important new insights into how the activity of the EGFRsystem is regulated.

ACKNOWLEDGMENTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

We thank Margaret Woolf for excellent technical assistance,Birgit Will for help with the metabolic labeling studies, SerdarOzcelik and Haluk Resat for assistance with the FRET analysis,and Yoshino Yoshitake and Katsuzo Nishikawa for the anti-EGFhybridomas. This research was in part sponsored by LaboratoryDirected Research and Development funds from the U.S. Departmentof Energy and by National Institutes of Health Grant GM-62575.

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E04-11-0994)on April 13, 2005.

Present address: Abgenix, 6701 Kaiser Dr., Fremont, CA 94555.

Address correspondence to: H. Steven Wiley (steven.wiley{at}pnl.gov).

REFERENCES

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

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Arribas, J., Coodly, L., Vollmer, P., Kishimoto, T. K., Rose-John, S., and Massague, J. ((1996). ). Diverse cell surface protein ectodomains are shed by a system sensitive to metalloprotease inhibitors. J. Biol. Chem. 271, , 11376-11382.[Abstract/Free Full Text]

Arribas, J., Lopez-Casillas, F., and Massague, J. ((1997). ). Role of the juxtamembrane domains of the transforming growth factor- ${alpha}$ precursor and the beta-amyloid precursor protein in regulated ectodomain shedding. J. Biol. Chem. 272, , 17160-17165.[Abstract/Free Full Text]

Asakura, M., et al. ((2002). ). Cardiac hypertrophy is inhibited by antagonism of ADAM12 processing of HB-EGF: metalloproteinase inhibitors as a new therapy. Nat. Med. 8, , 35-40.[CrossRef][Medline]

Band, V., and Sager, R. ((1989). ). Distinctive traits of normal and tumor-derived human mammary epithelial cells expressed in a medium that supports long-term growth of both cell types. Proc. Natl. Acad. Sci. USA 86, , 1249-1253.[Abstract/Free Full Text]

Berdichevsky, F., Alford, D., D'Souza, B., and Taylor-Papadimitriou, J. ((1994). ). Branching morphogenesis of human mammary epithelial cells in collagen gels. J. Cell Sci. 107, , 3557-3568.