Eps15 Is Recruited to the Plasma Membrane upon Epidermal Growth Factor Receptor Activation and Localizes to Components of the Endocytic Pathway during Receptor Internalization

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Vol. 10, Issue 2, 417-434, February 1999

Eps15 Is Recruited to the Plasma Membrane upon Epidermal Growth Factor Receptor Activation and Localizes to Components of the Endocytic Pathway during Receptor Internalization

Maria Rosaria Torrisi,^* Lavinia Vittoria Lotti,^*^§ Francesca Belleudi,^* Roberto Gradini,^* Anna Elisabetta Salcini, Stefano Confalonieri, Pier Giuseppe Pelicci,^¶ and Pier Paolo Di Fiore^#

^*Dipartimento di Medicina Sperimentale e Patologia, University of Roma "La Sapienza," Rome 00161, Italy; Istituto San Gellicano, Rome, Italy; ^§Istituto Nazionale Ricerca sul Cancro di Genova, Sezione di Biotecnologie, Rome, Italy; Department of Experimental Oncology, European Institute of Oncology, 20141 Milan, Italy; ^¶Istituto di Patologia Speciale Medica, University of Parma, Italy; and ^#Istituto di Microbiologia, University of Bari, Italy

Submitted June 5, 1998; Accepted December 7, 1998
Monitoring Editor: Juan Bonifacino

	ABSTRACT

Top Abstract Introduction Materials and methods Results Discussion References

Eps15 is a substrate for the tyrosine kinase of the epidermal growth factor receptor (EGFR) and is characterized by the presenceof a novel protein:protein interaction domain, the EH domain.Eps15 also stably binds the clathrin adaptor protein complex AP-2.Previous work demonstrated an essential role for eps15 in receptor-mediatedendocytosis. In this study we show that, upon activation of theEGFR kinase, eps15 undergoes dramatic relocalization consistingof 1) initial relocalization to the plasma membrane and 2) subsequentcolocalization with the EGFR in various intracellular compartmentsof the endocytic pathway, with the notable exclusion of coatedvesicles. Relocalization of eps15 is independent of its bindingto the EGFR or of binding of the receptor to AP-2. Furthermore,eps15 appears to undergo tyrosine phosphorylation both at theplasma membrane and in a nocodazole-sensitive compartment, suggestingsustained phosphorylation in endocytic compartments. Our resultsare consistent with a model in which eps15 undergoes cycles ofassociation:dissociation with membranes and suggest multiple rolesfor this protein in the endocyticpathway.

	INTRODUCTION

Top Abstract Introduction Materials and methods Results Discussion References

Receptor tyrosine kinases (RTKs) are rapidly internalized, through clathrin-coated pits, following binding to the cognateligand and activation of their intrinsic kinase activity (reviewedin Sorkin and Waters, 1993). After internalization, RTKs are sortedthrough vesicular structures into intracellular endosomal compartmentswhere decisions are made regarding whether to recycle the receptorto the cell surface or target it to lysosomes for degradation(Sorkin and Waters, 1993). The epidermal growth factor (EGF) receptor(EGFR) represents one of the best characterized systems. In itsintracellular domain, three regions have been defined that containendocytic codes, i.e., amino acid sequences capable by themselvesof sustaining EGFR internalization (Chang et al., 1993). Endocyticcodes are thought to be cryptic in the unstimulated EGFR and tobe unmasked by conformational changes that follow receptor activationand autophosphorylation (Nesterov et al., 1995a). In other typesof receptors, such as cargo receptors, endocytic codes are probablycontinuously exposed, thus determining constitutive internalization.In many cases endocytic codes contain a critical tyrosine residue,thus being known as "tyrosine-based" signals (reviewed in Mellman,1996; Marks et al., 1997), and are interchangeable among receptors(Chang et al., 1993). There is ample evidence that tyrosine-basedsignals, in the EGFR and in other receptors, bind directly tothe clathrin adaptor protein complex AP-2 (Glickman et al., 1989;Nesterov et al., 1995b; Sorkin et al., 1996).

AP-2 is a heterotetrameric protein complex that couples the process of coated pit assembly to that of recruitment of membranereceptors, through its ability to bind to receptor endocytic codes,on the one hand, and to clathrin, on the other (reviewed in Robinsons,1992, 1994; Kirchhausen, 1993). It is unknown whether AP-2 isdirected to the plasma membrane solely because of its interactionwith receptor endocytic codes; however, this possibility is unlikely,because receptors are present also in compartments to which adaptorcomplexes are not normally recruited (reviewed in Kirchhausenet al., 1997). In addition, removal of the tyrosine-based signal,responsible for AP-2 binding, in the EGFR did not appreciablyaffect internalization kinetics (Nesterov et al., 1995b), at leastat low levels of receptor expression (Sorkin et al., 1996). Finally,there is evidence of specificity in the endocytic machinery asshown by the findings that EGFRs compete with themselves but notwith transferrin receptor (TfR) for endocytosis (Dickson et al.,1983; Hanover et al., 1985; Wiley, 1988; Wiley et al., 1991).Thus, recruitment of AP-2 to the plasma membrane might requirea docking apparatus other than the receptors themselves (reviewedin Kirchhausen et al., 1997). One might speculate further thatdifferent docking machineries are responsible for endocyticspecificity.

A recently discovered family of RTK substrates, comprising the related eps15 and eps15R proteins, is also involved in receptor-mediatedendocytosis. Eps15 (Fazioli et al., 1993; Wong et al., 1994) andeps15R (Schumacher et al., 1995; Wong et al., 1995; Coda et al.,1998) are characterized by the presence of three copies of a novelprotein:protein interaction domain, the EH domain (Wong et al.,1995; Di Fiore et al., 1997). A number of observations have recentlylinked eps15, eps15R, and other EH-containing proteins to coatedpits-mediated internalization. 1) eps15 (Tebar et al., 1996; VanDelft et al., 1997b) and eps15R (Coda et al., 1998) colocalizewith markers of the plasma membrane clathrin-coated pits and vesicles;2) by electron microscopy, eps15 is found at the rim of buddingcoated vesicles (Tebar et al., 1996); 3) eps15 and eps15R areconstitutively associated with the clathrin adaptor protein complexAP-2 (Benmerah et al., 1995, 1996; Iannolo et al., 1997; Van Delftet al., 1997b; Coda et al., 1998); 4) a putative 160-kDa EH-containingprotein is associated with the $gamma$ -subunit of the Golgi adaptorcomplex AP-1 (Robinsons and Page, 1996); 5) End3p, an EH-containingyeast protein, is essential for endocytosis of the $alpha$ -factor receptor(Benedetti et al., 1994); 6) mutations in the EH domains of anotheryeast protein, Pan1p, impair endocytosis (Wendland et al., 1996;Tang et al., 1997); in addition, Pan1p functions as an adaptorprotein involved in the assembly of protein:protein interactionsessential for endocytosis (Wendland and Emr, 1998); 7) the aminoacid motif NPF (Asn-ProPhe) is a ligand for the EH domain (Salciniet al., 1997) and functions as an internalization motif in yeast(Tan et al., 1996); 8) microinjection of anti-eps15 or anti-eps15Rantibodies inhibits endocytosis of EGF and TfR (Carbone et al.,1997, Benmerah et al., 1998); and 9) overexpression of a dominantnegative mutant of eps15, comprising only its AP-2 binding region,is also able to inhibit EGFR internalization (Carbone et al.,1997).

In this study we analyzed the intracellular distribution of eps15 and its association with organelles of the endocytic pathwayduring internalization of the EGFR. Our observations, viewed inthe context of existing knowledge, are compatible with a modelin which eps15 might serve, at least in the case of EGFR internalization,as a docking molecule responsible for AP-2 recruitment to theplasma membrane. In addition, we show that eps15 colocalizes withthe EGFR, and is phosphorylated by it, in various compartmentsof the endocytic pathway, raising the possibility of its additionalinvolvement in late steps of the endocyticprocess.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and methods Results Discussion References

Cell lines

NIH-EGFR transfectants have been described previously (Di Fiore et al., 1987). B82 cells, transfected with normal EGFR wildtype (WT), mutant kinase-inactive EGFR (Chen et al., 1989), andmutant EGFR lacking the sequence for AP-2 binding (Nesterov etal., 1995b), were kindly provided by Dr. G. N. Gill (Universityof California, San Diego, CA). All cells were cultured in DMEMsupplemented with 10% fetal calf serum and antibiotics. In B82cell cultures, 2 mM methotrexate was added to the medium

For morphological experiments, cells were serum-starved for 12 h and incubated with EGF (100 ng/ml) (Gibco, Grand Island,NY) and anti-EGFR 108.1 monoclonal antibody (1:100 in PBS) orwith PDGF (20 ng/ml) (Upstate Biotechnology, Waltham, MA) at 4°Cfor 1 h and then warmed to 37°C for an additional 10 or 30 minor kept at 4°C before fixation. Treatment with nocodazole (20µg/ml) to depolymerize microtubules was performed in NIH-EGFRcells for 1 h at 37°C before EGF addition and prolonged duringincubations with EGF as above. To label early endosomes, cellsdepleted of serum for 12 h were incubated in medium containing18 nm BSA-colloidal gold particles for 10 min at 37°C to allowtheir internalization in early endocytic compartment beforefixation.

Immunofluorescence and Confocal Microscopy

Cells, grown on coverslips, were fixed in methanol at $-$ 20°C for 4 min. After washing in PBS, cells were incubated for 1 hat 25°C with an anti-eps15 affinity-purified polyclonal antibody(1 µg/ml in PBS, described below). The bound antibodies were visualizedwith anti-rabbit IgG FITC (1:100 in PBS, 30 min at 25°C) (CappelResearch Products, Durham, NC). For microtubule staining, cellswere successively incubated with anti-tubulin monoclonal antibody(1:100 in PBS, 1 h at 25°C) (Sigma, St. Louis, MO) and visualizedwith anti-mouse IgG TRITC (1:10 in PBS, 1 h at 25°C) (Cappel)after appropriate washing in PBS. For Golgi apparatus identificationin immunofluorescence, NIH-EGFR cells were incubated with thelectin HPA-FITC (1:10 in PBS, 1 h at 25°C) (Sigma). For AP-2 staining,cells were incubated with anti-AP-2 monoclonal antibody (mAb)(1:100 in PBS, 1 h at 25°C) (AP.6 mAb, kindly provided by Dr.Alexander Sorkin, University of Colorado). For double immunofluorescence,the anti-eps15 affinity-purified polyclonal antibody was visualizedwith anti-rabbit IgG Texas Red (1:50 in PBS) (Jackson ImmunoResearch,West Grove, PA) and anti-EGFR monoclonal antibody or anti-AP-2monoclonal antibody was detected with anti-mouse IgG FITC (1:10in PBS, 30 min at 25°C) (Cappel). Colocalization of the two fluorescencesignals was analyzed by a Zeiss Invert Laser Scan Microscope (Zeiss,Oberkochen, Germany). To follow the internalization of PDGFR,NIH-EGFR cells were treated with PDGF and fixed as described aboveand incubated with anti-PDGFR-A C20 polyclonal antibody (1:50in PBS, 1 h at 25°C) (Santa Cruz Biotechnology, Santa Cruz, CA),and the bound antibodies were visualized with anti-rabbit IgGFITC (1:100 in PBS, 1 h at 25°C)(Cappel).

The anti-eps15 antibody used in this study was raised against the full-length murine eps15, recombinantly produced as a GST-fusionprotein (GST/eps15-2-907; the numbers refer to the amino acidpositions of the eps15 moiety present in the GST fusion), by immunizingNew Zealand rabbits. The total serum was immunopurified by a two-stepprocedure involving first depletion of the anti-GST componentby three cycles of affinity chromatography on agarose-immobilizedGST and then by affinity purification onto agarose-immobilizedGST/eps15-2-907. The anti-eps15 serum was described in Coda etal. (1998) and shown not to cross-react with eps15R, the othermember of the eps15 family ofproteins.

Immunoelectron Microscopy

Cells untreated or treated with EGF as above, and cells incubated with BSA-gold (18 nm), were processed for postembeddingimmunocytochemistry. Briefly, cells were fixed with 0.5% glutaraldehydein PBS for 1 h at 25°C, partially dehydrated in ethanol, and embeddedin LR White resin. Thin sections were collected on nickel gridsand immunolabeled with the anti-eps15 affinity-purified antibodyantibodies (10 µg/ml in Tris, for 1 h at 25°C) followed by proteinA colloidal gold (18 nm) prepared by the citrate method (Slotand Geuze, 1981). In double-labeling experiments, the sectionswere first incubated alternatively with anticathepsin D polyclonalantibodies (1:100 in Tris, for 1 h at 25°C) (kindly provided byDr. Ciro Isidoro, University of Torino, Torino, Italy), with anti- $alpha$ Csubunit of AP-2, Ab31 polyclonal antibodies (1:5 in Tris, 1 hat 25°C) (kindly provided by Dr. Alexander Sorkin, Universityof Colorado, Denver, CO) or with anti-EGFR 528 monoclonal antibody(1:5 in Tris, 1 h at 25°C) (Santa Cruz Biotechnology), followedby 10 nm protein-A colloidal gold conjugates (British BioCellInternational, Cardiff, UK) and then with the anti-eps15 affinity-purifiedantibody followed by 18 nm protein A gold particles. Control experimentswere performed 1) by omission of the primary antibody or 2) byincubation of the sections with anti-eps15 polyclonal antibodypreviously adsorbed with the full-length eps15 protein (for 1h at 25°C). All sections were finally stained with uranyl acetateand leadhydroxide.

In preembedding experiments, B82 cells, treated as described above with EGF and anti-EGFR monoclonal antibody for 1 h at 4°Cand fixed or warmed to 37°C for 5 min before fixation in 0.5%glutaraldehyde (for 30 min at 4°C), were incubated with goat anti-mouseIgG (1:10 in PBS, for 1 h at 4°C) (Cappel), and finally labeledwith 18 nm protein-A gold particles. Cells were then processedfor conventional thin sections electron microscopy (post-fixedin 1% osmium tetroxide, stained with uranyl acetate 5 mg/ml, dehydratedin acetone, and finally embedded in Epon812).

Density of the immunogold labeling, determined as gold particles/micrometer of membrane length, and the statistical analysiswere evaluated using a Sigma Scan Measurement System (Jandel Scientific,Corte Madera,CA).

Protein Studies

Immunoprecipitation, immunoblotting, and coimmunoprecipitations were performed as described previously (Fazioli et al., 1993;Coda et al., 1998). Typically, we used 50-100 µg of total cellularproteins for direct immunoblot analysis and 3-5 mg of total cellularproteins for immunoprecipitation/immunoblotting experiments. Immunoblotswere decorated with the appropriate primary antibody (see below)and detection was with horseradish peroxidase conjugated withspecific secondary antisera followed by enhanced chemiluminescencereaction.

For coimmunoprecipitation studies, cells were lysed with a buffer containing 1% Triton X-100 (Pierce, Rockford, IL), 50 mMHEPES, pH 7.5, 150 mM NaCl, 10% glycerol, 1.5 mM MgCl₂, 5 mM EGTA,protease inhibitors (4 mM phenyl methylsulfonylfluoride and 100mg/ml aprotinin), and phosphatase inhibitors (10 mM sodium orthovanadateand 20 mM sodium pyrophosphate); cell lysates were used immediately,without freeze/thawing. Immunoprecipitations and coimmunoprecipitationswere performed for 1 h, and immune complexes were recovered byadsorption to Gamma Bind G-agarose (Pharmacia, Piscataway,NJ).

Antibodies used were 1) the described affinity-purified anti-eps15 antibody (Coda et al., 1998), 2) a commercial antiphosphotyrosinemonoclonal antibody (Upstate Biotech.), 3) a monoclonal anti- $alpha$ -adaptinrecognizing both $alpha$ A and $alpha$ C adaptins (Sigma), 4) commercial anti-shcantibodies (Santa Cruz Biotechnology), and 5) the E7 anti-EGFRpeptide serum (Di Fiore et al., 1990).

	RESULTS

Top Abstract Introduction Materials and methods Results Discussion References

Intracellular Localization of Eps15

As a preliminary step, we analyzed the intracellular localization of eps15 in different cell lines. Because one of the researchgoals was to investigate modifications of the distribution ofeps15 upon RTK activation, we focused our attention on cell linesexpressing EGFR, which is able to phosphorylate eps15 efficiently(Fazioli et al., 1993). In particular, two models of rodent fibroblasts,NIH-EGFR (Di Fiore et al., 1987) and B82-EGFR (Chen et al., 1989)cells, were used. These lines were genetically engineered to expresselevated levels of the EGFR, in the order of 0.5-1.0 × 10⁶ receptors/cell.

The intracellular localization of eps15 protein was analyzed by indirect immunofluorescence in NIH-EGFR cells, using a polyclonalantibody directed against the full-length eps15 protein. In logarithmicallygrowing NIH-EGFRs, the signal appeared punctate and dispersedthroughout the cell. Signals were present at the cell peripheryand along cell projections (Figure 1a, arrowheads) or concentratedin the perinuclear Golgi region (Figure 1a, arrows). Nocodazoletreatment, which induces dispersion and fragmentation of the Golgiapparatus by microtubule depolymerization, also induced a dispersionof the eps15 perinuclear concentration (Figure 1b). Similar resultswere obtained in B82-EGFR (Figure 3a₁) and in A172 glioblastoma,HeLa cervical carcinoma, and CV1 monkey kidney cell lines (ourunpublished results).

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Figure 1. Immunofluorescence analysis of the intracellular localization of eps15 in NIH-EGFR transfectants. (a) The pattern of staining with anti-eps15 antibody is punctate and the small dots are localized either at the cell periphery and along cell projections (arrowheads) or concentrated in the perinuclear Golgi area (arrows). (b) After treatment with nocodazole, resulting in microtubule depolymerization and subsequent Golgi fragmentation, the dots appear dispersed from the perinuclear cluster. The disrupting effect of nocodazole on microtubules was established by double staining with anti-tubulin antibodies. Bar, 5 µm. The anti-eps15 staining in this and all subsequent experiments was obtained with the described affinity-purified anti-eps15 antibody. In addition, comparable results were obtained using anti-eps15 monoclonal antibodies).

To identify the intracellular sites and structures of eps15 localization, we performed immunoelectron microscopy with anti-eps15antibodies and protein A-colloidal golds on thin sections of resin-embeddedNIH-EGFR cells. In logarithmically growing cells, immunolabelingwas mostly present on small vesicles (50-60 nm in diameter, measuredusing both the magnification scale bar and the 18 nm gold particlesas an internal size marker) (Figure 2, arrows) distributed eitherat the cell periphery and in close proximity to the plasma membrane(Figure 2b), or in the Golgi perinuclear area (Figure 2, a andc), juxtaposed to Golgi cisternae. Eps15 appeared also associatedwith clathrin-coated pits at the cell plasma membrane, as shownpreviously (Tebar et al., 1996). Double labeling with anti- $alpha$ -adaptinantibodies indicated colocalization of eps15 and $alpha$ -adaptin, asreported (Tebar et al., 1996; Van Delft et al., 1997b) (Figure2b, inset). Labeled vesicles were also frequently observed nearendosomal structures (Figure 2, c and d, arrows), identified asearly endosomes by the presence inside their lumen of internalizedBSA-gold particles (15 min of internalization at 37°C) (Figure2d, arrowheads). Immunolabeling of eps15 was not observed on theplasma membranes (Figure 2, a, b, and d), on Golgi cisternae (Figure2, a and c) and on endosomal or lysosomal membranes (Figure 2,c and d). In control experiments, gold immunolabeling was drasticallyreduced by incubation of the cell sections with anti-eps15 antibodyin the presence of the competing full-length eps15 protein (100µg/ml). Thus, eps15 appears mostly associated with the membranesof small vesicles located in peripheral as well as perinuclearregions. The intracellular distribution of these vesicles, frequentlyobserved in the proximity of plasma membranes, Golgi cisternae,and endosomes, suggests that they may represent transport carriersof the endocytic pathway.

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Figure 2. Immunoelectron microscopic analysis of eps15 localization. NIH-EGFR cells were resin-embedded, and thin sections were immunolabeled with anti-eps15 antibody and protein A-gold. (a-c) Gold particles (18 nm) are associated with small vesicles located either at the cell periphery and close to the plasma membrane (b, arrows) or in proximity to Golgi complexes (a and c, arrows) and to endosomal and lysosomal structures (c). Immunolabeling for eps15 appears also present at the cell surface in clathrin-coated pits, identified by double labeling with antibody to the $alpha$ subunit of AP-2 (detail in b, eps15: large golds; AP-2: small golds). (d) Immunogold particles corresponding to eps15 (arrows point to small golds) are frequently seen on vesicles located close to early endosomes identified by internalized BSA-gold (arrowheads point to large golds). er, Endoplasmic reticulum; M, mitochondrion; PM, plasma membrane; G, Golgi complex; cp, clathrin-coated pit; E, endosome; Ly, lysosome; EE, early endosome. Bars, 0.2 µm.

Eps15 is redistributed during EGFR and PDGFR endocytosis: redistribution depends on kinase activity of the receptors and is controlled by microtubules

Eps15 is a substrate for activated RTKs, including EGFR; however, the subcellular localization of eps15 is not modified byEGF treatment (Tebar et al., 1996; Van Delft et al., 1997b; ourunpublished results), even when receptor-saturating doses (100ng/ml, equivalent to 17 nM) of the ligand are used. This resultsomehow conflicts with the postulated role of eps15 in receptor-mediatedendocytosis (Carbone et al., 1997; Benmerah et al., 1998): a dynamicprocess involving rapid and progressive sorting of molecules invarious cellular compartments. One possible explanation is thatthe various pools of eps15 (coated pits-associated, small vesicle-associated,trans-Golgi network-associated) evidenced in immunoelectron microscopy(Figure 2) are in a dynamic equilibrium, possibly controlled byrapidly reversible posttranslational modifications of eps15. Ifthis were the case, redistribution of eps15 should become evidentupon induction of a synchronous wave of receptor-mediated endocytosis.In an attempt to achieve this, we treated NIH-EGFR or B82-EGFRcells with receptor-saturating doses of EGF (100 ng/ml) at 4°C,a temperature that is nonpermissive for EGFR internalization,albeit allowing its catalytic activation. After receptor loading,cells were shifted to 37°C for different time points to permitendocytosis. Under these various conditions we analyzed, by doubleimmunofluorescence, the localization of eps15 and EGFR. To selectivelyfollow internalizing receptors, cells were incubated simultaneouslywith EGF and a monoclonal antibody directed against the EGFR extracellularportion, which does not compete for EGF binding and does not inducereceptor cross-linking andinternalization.

Figure 3 shows a confocal analysis of B82-EGFR cells under various conditions. In logarithmically growing cells, as expected,the eps15 signal (red) appeared punctate and distributed throughoutthe cell, with only marginal enrichment at the cell periphery(Figure 3a₁). The EGFR signal (green) appeared mostly associatedwith the plasma membrane (Figure 3a₂), and only a modest amountof colocalization was visible by superimposition of the red andgreen signals in the three-dimensional reconstruction (colocalizedeps15 and EGFR appear in yellow) (Figure 3a₃). Treatment withEGF for 1 h at 4°C dramatically induced recruitment of eps15 tothe plasma membrane and substantially increased colocalizationof eps15 and EGFR at the cell surfaces (Figure 3b). Subsequentwarming to 37°C for 10 min induced redistribution of eps15 towardcentral areas of the cells (Figure 3c₁), where the eps15 punctatesignal colocalized with dots corresponding to internalized EGFR(Figure 3c₂). After 30 min of warming, both eps15 (Figure 3d₁)and EGFR (Figure 3d₂) signals appeared concentrated in the perinucleararea. Thus activation of the EGFR kinase induced recruitment ofeps15 at the plasma membrane, and synchronous triggering of endocytosisprovoked redistribution of eps15 to the perinuclear area. In bothcases eps15 signals colocalized with those of EGFR, indicatingthe presence of eps15 in the intracellular sites of traffickingof the receptor. Of note, redistribution and colocalization ofeps15 with the EGFR involved a sizable fraction of the eps15 pool,but not its totality.

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Figure 3. Confocal microscopic analysis of the distribution of eps15 (red: rhodamine staining) and EGFR (green: fluorescein staining) in B82 cells expressing EGFR WT. (a) Untreated cells; (b) cells treated with EGF for 1 h at 4°C; (c) cells treated with EGF for 1 h at 4°C and warmed to 37°C for 10 min; (d) cells treated with EGF for 1 h at 4°C and warmed to 37°C for 30 min. The extent of colocalization, assessed by superimposing red and green signals, is shown in yellow (panels labeled 3). Bar, 10 µm.

Parallel confocal analysis of B82-EGFR cells treated with EGF as above and double-labeled with anti- $alpha$ -adaptin (green signal)and anti-eps15 (red signal) antibodies indicated colocalizationof eps15 and $alpha$ -adaptin (yellow signal) mostly at the cell plasmamembrane after treatment with EGF for 1 h at 4°C (Figure 4a_1-3)and in the perinuclear area after an additional 30 min of warmingat 37°C (Figure 4b_1-3). Similarly coimmunoprecipitationbetween $alpha$ -adaptin and eps15 was not affected by treatment withEGF (Figure 4C). Thus, colocalization and physical associationof eps15 and AP-2, which has been already demonstrated in EGFuntreated cells (Tebar et al., 1996; Van Delft et al., 1997b),persists during redistribution of eps15 toward the plasma membraneat 4°C of EGF treatment and toward the perinuclear area afterEGFR internalization.

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Figure 4. Association between eps15 and AP-2 in various conditions of EGF treatment. (a, b) Confocal microscopic analysis of the distribution of eps15 (red: rhodamine staining) and AP-2 (green: fluorescein staining) in B82 cells expressing EGFR WT. (a) Cells treated with EGF for 1 h at 4°C; (b) cells treated with EGF for 1 h at 4°C and warmed to 37°C for 30 min. Colocalization of the two signals is shown in yellow (panels labeled 3). Bar, 10 µm. (c) Coimmunoprecipitation of eps15 and $alpha$ -adaptin. B82 cells expressing wild-type EGFR were serum-starved for 24 hours and then treated with EGF (100 ng/ml) for 1 h at 4°C (lane labeled 1h 4°C). Cells were then shifted to 37°C for the indicated lengths of time (lanes labeled 4°C $right-arrow$ 37°C). Total cellular lysates (4 mg) were immunoprecipitated with anti-eps15 antibody and subjected to immunoblots with anti-eps15 (top) or anti- $alpha$ -adaptin (bottom). The lanes labeled Lys were loaded with 100 µg of total lysates to serve as a reference. Positions of eps15 and $alpha$ -adaptin are indicated by arrows. The shift in mobility of eps15, upon EGF treatment, visible in the top panel, has been described and is probably caused by monoubiquitination.

Redistribution of eps15 during endocytosis was totally dependent on kinase activity of the EGFR. We used a kinase-defectiveEGFR mutant, which does not internalize in response to the ligand(Chen et al., 1989; Wiley et al., 1991). The results revealed1) no redistribution of eps15 after treatment with EGF eitherat 4°C or during subsequent warming to 37°C, 2) unperturbed distributionof EGFR kinase-defective mutant, as expected (Wiley et al., 1991),and 3) low levels of colocalization of eps15 and EGFR kinase-defectivemutant at all timepoints.

Similar results were obtained in NIH-EGFR cells that were subjected to the same protocol of treatment with either EGF or PDGF(our unpublished results). In addition, treatment with nocodazolefor 1 h at 37°C before EGF binding and warming to 37°C for 30min prevented eps15 (Figure 5c) and EGFR (Figure 5d) redistributiontoward the juxtanuclear region of the cell. Because depolymerizationof microtubules prevents late steps of EGFR endocytosis (Gruenbergand Maxfield, 1995), it appears that eps15 colocalizes with EGFRalong the entire pathway of receptor internalization.

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Figure 5. Immunofluorescence analysis of the redistribution of eps15 during EGFR endocytosis in NIH-EGFR cells treated with nocodazole. Double staining of eps15 (left panels) and of EGFR (right panels) on NIH-EGFR cells treated with EGF and anti-EGFR mAb for 1 h at 4°C and then warmed for 30 min at 37°C, in the absence (a and b) or presence (c and d) of nocodazole. Treatment with EGF at 4°C followed by incubation for 30 min at 37°C induces concentration of the eps15 and EGFR signals in the perinuclear area (a and b, respectively). Treatment with nocodazole blocks the redistribution of both eps15 and EGFR toward the central portion of the cell, keeping the signals at the cell periphery (c and d). Bar, 5 µm.

Eps15 is localized first on early and then on late endosomes during EGFR endocytosis

To identify the intracellular structures involved in eps15 redistribution during EGFR endocytosis, we performed immunolabelingwith anti-eps15 monoclonal antibody (mAb) and protein A-colloidalgold conjugates of thin sections of NIH-EGFR resin-embedded cellsincubated with EGF at 4°C and fixed or warmed to 37°C for 10 or30 min, to allow receptor internalization before fixation. Doubleimmunolabeling of EGFR and eps15 was also performed. After treatmentwith EGF at 4°C, immunogold labeling of eps15 appeared to be presentmostly on small vesicles closely apposed to the plasma membraneor associated with surface pits, as expected (Table 1). Warmingto 37°C for 10 min induced immunogold association with endosomalstructures (Figure 6a, arrows, and Table 1) and with vesiclesmostly located close to the Golgi complex (Figure 6a). Colocalizationof eps15 (large golds) and EGFR (small golds) was observed onclathrin-coated pits at the cell surface (Figure 6a, left inset),on small noncoated vesicles, and on early endosomes (our unpublishedresults). Interestingly, clathrin-coated vesicles juxtaposed tothe plasma membrane were positively labeled only for EGFR, appearingnegative for eps15 (Figure 6a, right inset). After 30 min of warming,gold labeling of eps15 appeared confined to the perinuclear area(Figure 6b), frequently associated with the membranes of endosomes(Table 1) identified as late endosomes by morphological criteria(Figure 6b), and in double-labeling experiments by positive reactionto cathepsin D, a marker of late endosomes and lysosomes (Figure6c). At the 30-min time point of warming, endosomes and vesiclesat the cell periphery appeared unlabeled (Figure 6b). Similarresults were obtained in B82-EGFR cells. Thus, eps15 appears toassociate with endosomal membranes after EGFR endocytosis anddown-regulation.

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Table 1. Quantitation of eps 15 gold immunolabeling associated with the plasma membrane and endosomal membranes in NIH-EGFR cells after EGF binding and internalization

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Figure 6. Immunoelectron microscopic analysis of eps15 redistribution during EGFR endocytosis. NIH-EGFR cells were treated with EGF for 1 h at 4°C and warmed to 37°C for 10 min (a) or 30 min (b and c). After 10 min of warming, gold immunolabeling appears associated with endosomal membranes (a, arrows) and vesicles mostly localized in proximity to Golgi cisternae (a). Colocalization of eps15 (large golds) and EGFR (small golds) is observed on clathrin-coated pits at the cell surface (Figure 5a, left inset; eps15: arrow, EGFR: arrowhead), whereas clathrin-coated vesicles juxtaposed to the plasma membrane appear positively labeled only for EGFR (Figure 5a, right inset, arrowhead). At 30 min of warming, gold particles are present in the central perinuclear region of the cell (b and c), close to Golgi complexes (c), and around late endosomes (b and c) positive for cathepsin D (small golds in c). In b, the arrow points to a vesicle positively labeled for eps15 in the process of fusion with a late endosome. Nu, Nucleus; LE, late endosome; cv, clathrin-coated vesicle. Bars, 0.2 µm; insets in a, 0.1 µm.

Biochemical Events Involved in Eps15 Redistribution and Colocalization with EGFR during Endocytosis

A simple mechanism to account for recruitment of eps15 to the plasma membrane upon EGFR activation is binding to the activatedEGFR. There is discordance in the literature as to whether eps15can associate, directly or indirectly, with the EGFR in vivo (Fazioliet al., 1993; Van Delft et al., 1997b). In B82-EGFR (Figure 7A)or in NIH-EGFR cells (our unpublished results), we were consistentlyunable to evidence coimmunoprecipitation of the EGFR with eps15.This was true also in the case in which cells were treated with100 ng/ml EGF for 2 h at 4°C (Figure 7A), a condition that maximizesassociation of eps15 with the plasma membrane (Figure 3b₁). Ofnote, under the same conditions of coimmunoprecipitation, EGF-dependentassociation of the $alpha$ subunit of the AP-2 clathrin adaptor complexprotein with EGFR was readily detectable (Figure 7A). EGFR/AP-2association was evident when stimulation with EGF was performedat 37°C, but not at 4°C, as reported previously (Sorkin and Carpenter,1993), because this latter condition prevents recruitment of activatedEGFR into coated pits, where interaction with AP-2 takes place.In addition, under the same conditions of coimmunoprecipitation,we could readily detect association of eps15 with several bindingpartners, such as AP-2, NUMB, and RAB/Rip (Iannolo et al., 1997;Salcini et al., 1997; Coda et al., 1998). Thus we favor the hypothesisthat recruitment of eps15 to the plasma membrane is not causedby a stable detergent-resistant association between eps15 andthe EGFR.

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Figure 7. Association of AP-2 or eps15 with EGFR WT or a mutant deficient in AP-2 binding (EGFR $Delta$ AP-2). B82 cells expressing wild-type EGFR (A) or the AP-2-binding mutant EGFR (B) were serum-starved for 24 hours (SF) and then treated with EGF (100 ng/ml) for the indicated times. In some case, as indicated, EGF treatment was performed at 4°C after 24 h of serum starvation at 37°C, followed by 2 h of serum starvation at 4°C. Total cellular lysates were then immunoprecipitated with the anti-EGFR antibody E7 and subjected to immunoblots with (from top to bottom): anti-eps15 (5 mg of lysates), anti- $alpha$ -adaptin (5 mg of lysates), anti-pTyr (1 mg of lysate), anti-EGFR (1 mg of lysate). The lanes labeled Lys were loaded with 50 µg of total lysates to serve as a reference. The positions of eps15, $alpha$ -adaptin, and EGFR are indicated by arrows.

A hypothetical association between EGFR and eps15, however, could be indirect and mediated by adaptor molecule(s). Under thisscenario it might also be more difficult to detect significantcoimmunoprecipitation between EGFR and eps15. The best candidatefor such an adaptor role is AP-2. Eps15 is constitutively associatedwith AP-2 (Benmerah et al., 1995, 1996; Iannolo et al., 1997;Van Delft et al., 1997b). AP-2 in turn binds to EGFR upon EGF-inducedactivation of the receptor (Sorkin and Carpenter, 1993). To investigatethe role of the constitutive interaction of eps15 with AP-2 indetermining redistribution of eps15 and colocalization of eps15with EGFR during receptor internalization, we used B82 cells expressinga mutant form of EGFR deficient in AP-2 binding (Nesterov et al.,1995b). This mutant (EGFR958f993-1186, henceforth referred toas EGFR $Delta$ AP-2) bears an interstitial deletion between amino acids959 and 992 that removes the binding site for AP-2 and does notcoimmunoprecipitate with AP-2 (Nesterov et al., 1995b) (Figure6B).

Double immunofluorescence and confocal analysis were performed to evaluate eps15 redistribution and colocalization with theEGFR $Delta$ AP-2 mutant. A remarkably similar behavior of eps15 redistributionand EGFR internalization, as well as extent of colocalization,was observed in the cells expressing WT (Figure 3) or mutant (Figure8) receptors. In the absence of EGF treatment, the signal correspondingto eps15 in B82-EGFR $Delta$ AP-2 cells (Figure 8a₁) revealed the sameintracellular localization described for untreated B82-EGFR cells(Figure 3a₁), and the EGFR $Delta$ AP-2 appeared localized to the plasmamembranes as expected (Figure 8a₂). Treatment with EGF for 1 hat 4°C induced recruitment of eps15 to the plasma membranes andincreased colocalization of eps15 and EGFR $Delta$ AP-2 at the cell surfaces(Figure 8b_1-3). Warming to 37°C for 10 min (Figure 8c) orfor 30 min (Figure 8d) resulted in eps15 redistribution and EGFR $Delta$ AP-2endocytosis, as described above for B82-EGFR cells (Figure 3).At both time points of warming, high levels of colocalizationof the two signals were evident in correspondence of the intracellularsites of trafficking of EGFR (Figure 8, c₃ and d₃). Therefore,eps15 colocalization with EGFR is not dependent on AP-2 bindingto the receptors.

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Figure 8. Confocal microscopy of B82 cells expressing a mutant EGFR deficient in AP-2 binding (EGFR $Delta$ AP-2). Legend as in Figure 3.

To ascertain whether the observed EGFR internalization process was occurring through clathrin-coated pits, also in the absenceof AP-2 interaction with the receptors, we performed immunoelectronmicroscopy on B82 cells expressing EGFR WT or mutant EGFR $Delta$ AP-2.Cells were treated with EGF and anti-EGFR mAb at 4°C as aboveand then warmed to 37°C for 5 min to allow receptor clusteringinto coated pits at the plasma membrane. In cells expressing bothtypes of receptors, immunogold labeling of EGFR appeared localizedin clathrin-coated pits upon warming to 37°C (Figure 9 and Table2). This observation implies that EGFR may enter into clathrin-coatedpits independently on AP-2 binding and suggest that eps15, whichcolocalizes with EGFR also independently on AP-2, may play a rolein this first step of internalization. Interestingly the EGFR $Delta$ AP-2is competent for eps15 tyrosine phosphorylation, with a kineticsvirtually indistinguishable from wild-type EGFR (Figure 10A), indicatingthat a hypothetical recruitment of eps15 to the EGFR through AP-2is not necessary for eps15 to serve efficiently as a kinase substrate.

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Figure 9. Surface immunogold labeling with anti-EGFR mAb of B82 cells expressing EGFR WT (a-c) or EGFR $Delta$ AP-2 mutant (d). After incubation with EGF for 1 h at 4°C (a), EGFRs are distributed over the cell plasma membranes, preferentially associated with the microvilli, and excluded by clathrin-coated pits (a, arrowhead). After warming to 37°C for 5 min, either WT EGFRs (b and c) or mutant EGFRs (d) appear clustered over the nonvillous portions of the plasma membrane (b) and inside clathrin-coated pits (c and d, arrowheads). Bars, 0.5 µm.

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Table 2. Quantitative distribution of EGFR immunogold labeling on the surface of B82 cells expressing EGFR and EGFR $Delta$ AP-2 after EGF binding and internalization

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Figure 10. Tyrosine phosphorylation of eps15 by EGFR WT or by EGFR $Delta$ AP-2. (A) B82 cells expressing wild-type EGFR (top) or the AP-2-binding mutant EGFR (bottom) were serum-starved for 24 h and then treated with EGF (100 ng/ml) for the indicated times. Total cellular lysates (2 mg) were then immunoprecipitated with the anti-eps15 antibody and subjected to immunoblots with anti-pTyr. The position of eps15 is indicated by arrows. (B) Time kinetics of eps15 tyrosine phosphorylation in B82-EGFR cells treated with various concentrations of EGF. pTyr-containing eps15 was assessed by immunoprecipitation/blotting experiments, as in A. Densitometric scans of the blot were obtained, and results are reported after correction for the amount of eps15 immunoprecipitated revealed by stripping of the blots and decoration with an anti-eps15 antibody.

Tyrosine Phosphorylation of Eps15 during Receptor Internalization

The observation that eps15 colocalizes with the EGFR at various steps in the internalization route raises the question ofwhether eps15 can be phosphorylated by the receptor at locationsother than the plasma membrane. This possibility is indirectlysupported by the fact that the time-dependent kinetics of eps15tyrosine phosphorylation by EGFR (Figure 10B) shows frequentlya biphasic behavior with two peaks of phosphorylation, one around5 min and a second between 20 and 30 min of EGF addition. Thisbehavior is even more pronounced if EGF is added at nonreceptorsaturating doses (10 ng/ml equal to 1.7 nM) (Figure 10B). Thusthe apparent biphasic time kinetics could be the result of prolongedphosphorylation occurring in some endosomalcompartment.

To gain insight into this issue we analyzed the phosphotyrosine (pTyr) content of eps15 in cells stimulated with EGF in thepresence or absence of nocodazole. In parallel, under the sameconditions, we analyzed the pTyr content of shc, an EGFR substratewhose phosphorylation is likely to occur exclusively at the plasmamembrane, because its localization is not altered under conditionsdesigned to inhibit EGFR endocytosis (Lotti et al., 1996). Asshown in Figure 11, a and b, nocodazole treatment did not affectthe initial phases of eps15 phosphorylation (1 min) but severelydecreased the pTyr content at 5 and 30 min. As expected, shc tyrosinephosphorylation was unaffected by nocodazole treatment at alltime points (Figures 11, d and e). A simple model to explain theseresults is that eps15 is subjected to a first wave of phosphorylationby the EGFR concomitantly to its recruitment to the plasma membrane,a step that should be nocodazole-insensitive. Subsequently, eps15might be subject to further phosphorylation by the receptors,even in the late phases of the endocytic process, which are nocodazole-sensitive.

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Figure 11. Tyrosine phosphorylation of eps15 and shc under various conditions of EGF treatment. B82-EGFR cells were serum-starved for 24 hours (0) and then treated with EGF (100 ng/ml) for the indicated times. In A and D, cells were treated at 37°C after serum starvation at 37°C; in B and E, cells were treated at 37°C after serum starvation at 37°C and treatment in the presence of nocodazole (20 µg/ml for 1 h; nocodazole was kept also during EGF stimulation). In C and F, cells were serum-starved at 37°C and for an additional 2 h at 4°C, followed by treatment with EGF at 4°C. Total cellular lysates (2 mg) were immunoprecipitated with either an anti-eps15 (A-C) or an anti-shc (D-F) antibody and then immunoblotted with anti-pTyr. The positions of eps15 and shc are indicated by arrows.

Interestingly, when EGF treatment was performed at 4°C, eps15 was still tyrosine-phosphorylated (Figure 11C), albeit with adelayed kinetics, with respect to shc (Figure 11D). A quantitativeassessment of these latter results is impossible, because toomany variables are unaccounted for, including kinase efficiencyof the EGFR and phosphatase(s) activity in vivo at 4°C versus37°C; however, it appears as if phosphorylation of eps15 by theEGFR at the plasma membrane does not require recruitment of thereceptor into coated pits, this phenomenon being inhibited at4°C.

	DISCUSSION

Top Abstract Introduction Materials and methods Results Discussion References

The endocytic pathway followed by RTKs, and in particular by EGFR, has been widely studied (reviewed in Sorkin and Waters,1993). Upon ligand binding, EGFR enters clathrin-coated pits atthe cell surfaces, is internalized by clathrin-coated vesicles,and reaches early endosomes where sorting occurs to the plasmamembrane for receptor recycling or to late endosomes and lysosomesfor down-regulation. Several lines of evidence (reviewed in DiFiore et al., 1997) suggest that eps15 plays a role in the controlof endocytosis, a possibility that is antagonized, however, bythe observation that eps15 distribution does not change appreciablyupon ligand-induced endocytosis of the EGFR (Tebar et al., 1996;Van Delft et al., 1997b). We were conversely able to show thatthe eps15 undergoes dramatic relocalization during EGFR endocytosis,by first being recruited to the plasma membrane and then colocalizingwith the EGFR in early and lateendosomes.

In our opinion, the initial relocalization of eps15 to the plasma membrane deserves particular attention. Two major modelsfor RTK-mediated internalization have been proposed. In the first,ligand-bound receptors enter coated pits simply by virtue of theirrandom lateral mobility in the plasma membrane. Once they reachthe pit, they are retained by specific components of the pit machinery.The best candidate for such a role is the clathrin adaptor complexprotein AP-2. In the EGFR system, AP-2 binds in a ligand-dependentmanner (Sorkin and Carpenter, 1993) to a tyrosine-based signal,which is part of one of the three endocytic codes present in theC-terminal portion of the EGFR. Binding of AP-2 to the EGFR requiresactivation of the receptor kinase activity, autophosphorylation,and conformational changes that probably unmask the binding site;however, endocytosis of EGFR is a second-order saturable process,likely involving competition among EGFRs for a downstream componentof the endocytic machinery (Lund et al., 1990). Quantitative considerations(reviewed in Nesterov et al., 1995b) militate against AP-2 beingsuch a component. In addition, AP-2-binding mutants of the EGFRdisplay unperturbed internalization kinetics (Nesterov et al.,1995b), at least at low levels of receptor expression (Sorkinet al., 1996). In addition, evidence has been provided that atyrosine kinase substrate, different from EGFR itself, is neededfor efficient recruitment into coated pits of ligand-activatedEGFR (Lamaze and Schmid, 1995).

In a second model, a membrane-bound docking apparatus (or several receptor-specific apparatuses) might exist that facilitatestargeting of receptors to coated pits. The docking molecule (ora component of the docking apparatus) might coincide with theaforementioned tyrosine kinase substrate, other than the EGFR.Eps15 possesses several of the characteristics that fit this role:1) it is an EGFR substrate (Fazioli et al., 1993); 2) it is anessential component of the endocytic pathway (Carbone et al.,1997); 3) it localizes to the plasma membrane and colocalizeswith the EGFR after ligand stimulation (this study); and 4) itis constitutively bound to AP-2 (Benmerah et al., 1995). One mightthus postulate that constitutive nonplasma membrane-bound eps15/AP-2complexes are recruited to the plasma membrane by EGFR-inducedposttranslational modifications of eps15. Tyrosine phosphorylationis the most obvious candidate for such a modification, albeitother modifications, such as the recently shown monoubiquitinationof eps15 (Van Delft et al., 1997a), cannot be excluded at thisstage. The relocalization of AP-2 to the plasma membrane can thentrigger assembly of the clathrin lattice and receptor retentioninto the pit through various mechanisms (reviewed in Kirchhausenet al., 1997). At this stage eps15 might dissociate from AP-2,as indicated by recent findings of Cupers et al. (1998).

The above model would predict that plasma membrane relocalization and tyrosine phosphorylation of eps15 are independent ofbinding of AP-2 to the receptor: a prediction that was experimentallyvalidated in this study. In addition, this model would easilyaccommodate experimental findings such as the preferential localizationof eps15 at the rims of the coated pits (Tebar et al., 1996).As originally pointed out by Tebar et al. (1996), the localizationof eps15 at the rims of coated pits is surprising, because AP-2,the binding partner, is localized throughout the coat profile.This observation led Kirchhausen et al. (1997) to postulate thateps15 might undergo cycles of binding to and release from AP-2during coat assembly. In our proposed model, the location of eps15at the rim, which is likely the growing part of a forming pit,would be self-explanatory, if eps15 were to function as a docking/recruitingmolecule.

Recruitment of eps15 to the plasma membrane does not require a stable detergent-resistant physical interaction (direct orindirect) between eps15 and the EGFR (this study). In addition,a stoichiometrically significant interaction between eps15 andEGFR could not be immediately reconciled with the absence of eps15from the deeper parts of coated pits (Tebar et al., 1996) whereEGFR and AP-2 are abundant. Indeed, there is discordance in theliterature as to whether eps15 is complexed to the EGFR in vivo(Fazioli et al., 1993; Van Delft et al., 1997b; this study). Partof the differences can be cell-specific because in a survey ofseveral cell lines expressing the EGFR we identified some celllines in which eps15 and EGFR can indeed be coimmunoprecipitated(our unpublished results), albeit with rather low stoichiometry:<1% of the eps15 pool. The lack of universality of the phenomenonand its quantitative limitedness appear to militate against itsrelevance; however, one can envision a transitory, unstable interactionbetween eps15 and EGFR at the recruiting edge of the pit, whichmight account for all of the aboveobservations.

An interesting finding is that in addition to the expected association with coated pits at the cell surface, eps15 is localizedon intracellular vesicles not only peripheral, but also perinuclear.EGFR activation and endocytosis determines first a recruitmentof eps15 at the cell surface and later a redistribution towardthe central area of the cell. This phenomenon, although not involvingthe total eps15 pool, clearly reflects the behavior of a largeamount of eps15 molecules. In addition, eps15 colocalizes withthe EGFR during endocytosis. Thus, our findings pose the questionas to whether eps15 is "trafficked" with the EGFR from the plasmamembrane to the endosomes or whether it is "targeted" to endosomalmembranes. We note that although we were able to readily detectassociation of eps15 with coated pits and early and late endosomes,we could not detect its presence in clathrin-coated vesicles.This result is consistent with those reported by Cupers et al.(1998), who showed that purified coated vesicles contain negligibleamounts of eps15 and that eps15 is lost during coat assembly invitro. Thus, we favor the possibility that multiple cycles ofassociation:dissociation of eps15 with membranes occur as theEGFR moves forward in the endocytic pathway. The molecular determinantsinvolved in the "retargeting" of eps15 to endosomes are unknown;however, the kinetics of eps15 tyrosine phosphorylation correlateswith its reassociation to endosomes. A late peak of eps15 tyrosinephosphorylation occurs, in fact, in a nocodazole-sensitive compartment.Thus, in analogy with what we propose for eps15 recruitment tothe plasma membrane, the EGFR might be able to phosphorylate eps15in the endosomal compartment, thereby determining its associationwith endosomalmembranes.

Also somewhat surprising is our finding that eps15 colocalizes with $alpha$ -adaptin not only at the plasma membrane, in cells treatedwith EGF at 4°C, but also in perinuclear structures after warmingat 37°C. We do not know whether these structures also containinternalized EGFR, thus representing bona fide early or late endosomes.On the basis of current knowledge, this possibility appears unlikely.These structures, however, might represent intermediate carriervesicles, other than endosomes, involved in the receptor transportand/or sorting along the endocyticpathway.

The retargeting of eps15 to endosomes, after its dissociation from coated vesicles, strongly suggests that eps15 plays a rolein the late steps of endocytosis, different from that exertedat the plasma membrane level in the formation of coated pits.Indeed some molecular evidence already exists that these two putativefunctions of eps15 can be dissociated. We have shown previouslythat microinjection of anti-eps15 antibodies efficiently inhibitsinternalization of EGFR (Carbone et al., 1997). In addition, overexpressionof a dominant negative mutant comprising only the AP-2 bindingregion of eps15 (L2 region) inhibited internalization of EGFRand establishment of successful infection by Sindbis virus, whichis known to require coated pits-mediated internalization of thevirus (reviewed in Marsh and Helenius, 1989). Surprisingly, aneps15 mutant encompassing only its three EH domains had no effecton EGFR internalization but completely inhibited Sindbis infection(Carbone et al., 1997; our unpublished observations). One possibleexplanation for this discrepancy is that the inhibition by EHdomains is exerted at a step in the endocytic pathway other thaninternalization, as for example in the transport from early endosomesto the more acidic late endosomes, a step required for viral fusionand infection (Marsh and Helenius, 1989). If this were true, itwould direct the attention regarding a possible role of eps15in late endocytosis to the protein:protein interaction abilitiesof the EH domain, an intriguing possibility that warrants furtherinvestigation.

	ACKNOWLEDGMENTS

We are very grateful to Dr. Gordon N. Gill for providing B82 cells expressing EGFR WT and mutants. We thank Dr. Maria Gianmatteofor help in the confocal analysis, Mr. Ilio Piras for excellentphotographic work, and Mr. Giuseppe Lucania and Ms. Lucia Cutinifor excellent technical assistance. This work was partially supportedby grants from Ministero Università Ricerca Scientifica Tecnologica,from Associazione Italiana per la Ricerca sul Cancro (AIRC), fromConsiglio Nazionale delle Ricerche (Target Project on "Biotechnology"),from the European Community (BIOMED-2 Program), from the Armenise-HarvardFoundation, and from the FondazioneFerrero.

	FOOTNOTES

Corresponding author. E-mail address: torrisi{at}axrma.uniroma1.it.

REFERENCES

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

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				K. G. Bache, C. Raiborg, A. Mehlum, and H. Stenmark STAM and Hrs Are Subunits of a Multivalent Ubiquitin-binding Complex on Early Endosomes J. Biol. Chem., March 28, 2003; 278(14): 12513 - 12521. [Abstract] [Full Text] [PDF]

				E. Klapisz, I. Sorokina, S. Lemeer, M. Pijnenburg, A. J. Verkleij, and P. M. P. van Bergen en Henegouwen A Ubiquitin-interacting Motif (UIM) Is Essential for Eps15 and Eps15R Ubiquitination J. Biol. Chem., August 16, 2002; 277(34): 30746 - 30753. [Abstract] [Full Text] [PDF]

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				T. Ringerike, F. D. Blystad, F. O. Levy, I. H. Madshus, and E. Stang Cholesterol is important in control of EGF receptor kinase activity but EGF receptors are not concentrated in caveolae J. Cell Sci., March 15, 2002; 115(6): 1331 - 1340. [Abstract] [Full Text] [PDF]

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				H.-J. Kuo, N. T. Tran, S. A. Clary, N. P. Morris, and R. W. Glanville Characterization of EHD4, an EH Domain-containing Protein Expressed in the Extracellular Matrix J. Biol. Chem., November 9, 2001; 276(46): 43103 - 43110. [Abstract] [Full Text] [PDF]

				G. Wang, J. M. McCaffery, B. Wendland, S. Dupré, R. Haguenauer-Tsapis, and J. M. Huibregtse Localization of the Rsp5p Ubiquitin-Protein Ligase at Multiple Sites within the Endocytic Pathway Mol. Cell. Biol., May 15, 2001; 21(10): 3564 - 3575. [Abstract] [Full Text]

				E. Santolini, C. Puri, A. E. Salcini, M. C. Gagliani, P. G. Pelicci, C. Tacchetti, and P. P. Di Fiore Numb Is an Endocytic Protein J. Cell Biol., December 11, 2000; 151(6): 1345 - 1352. [Abstract] [Full Text] [PDF]

				M. Barbieri, R. Roberts, Gumusboga, Highfield, Alvarez-Dominguez, Wells, and P. Stahl Epidermal Growth Factor and Membrane Trafficking: EGF Receptor Activation of Endocytosis Requires Rab5a J. Cell Biol., October 30, 2000; 151(3): 539 - 550. [Abstract] [Full Text] [PDF]

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				A. J. Bean, S. Davanger, M. F. Chou, B. Gerhardt, S. Tsujimoto, and Y. Chang Hrs-2 Regulates Receptor-mediated Endocytosis via Interactions with Eps15 J. Biol. Chem., May 12, 2000; 275(20): 15271 - 15278. [Abstract] [Full Text] [PDF]

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