Localization of Autocrine Motility Factor Receptor to Caveolae and Clathrin-independent Internalization of Its Ligand to Smooth Endoplasmic Reticulum

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Vol. 9, Issue 7, 1773-1786, July 1998

Localization of Autocrine Motility Factor Receptor to Caveolae and Clathrin-independent Internalization of Its Ligand to Smooth Endoplasmic Reticulum

Naciba Benlimame, Phuong U. Le, and Ivan R. Nabi^*

Département de Pathologie et Biologie Cellulaire, Université de Montréal, Montréal, Québec, Canada H3C 3J7

Submitted February 20, 1998; Accepted April 15, 1998
Monitoring Editor: W. James Nelson

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Autocrine motility factor receptor (AMF-R) is a cell surface receptor that is also localized to a smooth subdomain of theendoplasmic reticulum, the AMF-R tubule. By postembedding immunoelectronmicroscopy, AMF-R concentrates within smooth plasmalemmal vesiclesor caveolae in both NIH-3T3 fibroblasts and HeLa cells. By confocalmicroscopy, cell surface AMF-R labeled by the addition of anti-AMF-Rantibody to viable cells at 4°C exhibits partial colocalizationwith caveolin, confirming the localization of cell surface AMF-Rto caveolae. Labeling of cell surface AMF-R by either anti-AMF-Rantibody or biotinylated AMF (bAMF) exhibits extensive colocalizationand after a pulse of 1-2 h at 37°C, bAMF accumulates in denselylabeled perinuclear structures as well as fainter tubular structuresthat colocalize with AMF-R tubules. After a subsequent 2- to 4-hchase, bAMF is localized predominantly to AMF-R tubules. Cytoplasmicacidification, blocking clathrin-mediated endocytosis, resultsin the essentially exclusive distribution of internalized bAMFto AMF-R tubules. By confocal microscopy, the tubular structureslabeled by internalized bAMF show complete colocalization withAMF-R tubules. bAMF internalized in the presence of a 10-foldexcess of unlabeled AMF labels perinuclear punctate structures,which are therefore the product of fluid phase endocytosis, butdoes not label AMF-R tubules, demonstrating that bAMF targetingto AMF-R tubules occurs via a receptor-mediated pathway. By electronmicroscopy, bAMF internalized for 10 min is located to cell surfacecaveolae and after 30 min is present within smooth and rough endoplasmicreticulum tubules. AMF-R is therefore internalized via a receptor-mediatedclathrin-independent pathway to smooth ER. The steady state localizationof AMF-R to caveolae implicates these cell surface invaginationsin AMF-R endocytosis.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Expression of autocrine motility factor receptor (AMF-R) is associated with the acquisition of motile and metastatic propertiesby tumor cells (for review see Silletti and Raz, 1996). AMF-Rexpression correlates with the malignancy of human bladder, colon,and gastric tumors (Nakamori et al., 1994; Otto et al., 1994;Hirono et al., 1996). In cultured cells, AMF-R expression is decreasedin contact-inhibited A31-3T3 fibroblasts (Silletti and Raz, 1993)and increased after viral transformation of MDCK epithelial cells(Simard and Nabi, 1996). AMF-R is a cell surface receptor thatmediates motility stimulation by its 55-kDa polypeptide ligand,AMF, recently shown to be homologous to phosphohexose isomerase(Liotta et al., 1986; Watanabe et al., 1996). AMF is selectivelysecreted after transformation of NIH-3T3 cells, and the presenceof AMF activity in the urine of cancer patients correlates withtumor malignancy (Liotta et al., 1986; Guirguis et al., 1990).

Transduction of the AMF motility signal occurs via receptor phosphorylation, a pertussis toxin-sensitive G-protein, inositolphosphate production, tyrosine kinase and PKC activation, andproduction of the lipoxygenase metabolite 12-HETE (Silletti andRaz, 1996). AMF-R is localized not only to the plasma membranebut also to an intracellular tubular organelle, the AMF-R tubule(Nabi et al., 1992; Benlimame et al., 1995). AMF-R tubules aredistinct from endosomes and lysosomes; by postembedding immunoelectronmicroscopy AMF-R is present primarily in smooth tubules that extendfrom ribosome-studded cisternae; however, AMF-R tubules do notcolocalize with ERGIC-53, a marker for the ER-Golgi intermediatecompartment (Benlimame et al., 1995; Wang et al., 1997). Aftertreatment with ilimaquinone, which induces vesiculation of theGolgi apparatus (Takizawa et al., 1993), AMF-R tubules acquirea fenestrated morphology typical of smooth ER, suggesting thatthe AMF-R tubule is a distinct smooth subdomain of the ER (Wanget al., 1997). The intracellular distribution of this cell surfacereceptor to smooth ER implicates AMF-R recycling in its functionin cell motility and tumor cell metastasis.

Actin cytoskeleton reorganization at the leading edge and de novo establishment of cell-substrate contacts results in lamellipodialextension and the consequent polarization of the motile cell (Rinnerthaleret al., 1988; Condeelis, 1993; Stossel, 1993). The role of intracellularvesicular traffic in the establishment and maintenance of epithelialand neuronal polarity is well-established (Rodriguez-Boulan andPowell, 1992; Drubin and Nelson, 1996; Keller and Simons, 1997)and strongly supports a role for intracellular membrane trafficin the polarization of the motile cell and formation of a distinctplasma membrane domain, the leading lamella (Singer and Kupfer,1986; Nabi et al., 1992; Bretscher, 1996). Influenza hemagglutininand vesicular stomatitis virus G proteins, polarized apicallyand basolaterally in epithelial cells and axonally and dendriticallyin neurons (Rodriguez-Boulan and Sabatini, 1978; Dotti and Simons,1990), also follow distinct pathways to the cell surface in "unpolarized"fibroblasts (Yoshimoro et al., 1996). Newly synthesized VSV Gprotein is targeted to the leading edge and cellular protrusionsof motile fibroblasts, and the directionality of its deliverywas shown to be microtubule-dependent (Bergmann et al., 1983;Rogalski et al., 1984; Peränen et al., 1996). Membrane recyclingvia coated pits has long been suggested to be implicated in cellspreading and cell motility (Bretscher, 1984). We show here thatAMF-R is concentrated at the cell surface within smooth plasmalemmalvesicles or caveolae and that AMF is internalized via a nonclathrinpathway to intracellular smooth ER tubules. Our results implicatecaveolae in transduction of the AMF motility signal as well asin the internalization of its receptor.

	MATERIALS AND METHODS

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Cells and Cell Culture

NIH-3T3 fibroblasts obtained from the ATCC were cloned, and a highly spread clone was used for these studies. HeLa and NIH-3T3cells were grown in an air-5% CO₂ incubator at constant humidityin DMEM containing nonessential amino acids, vitamins, glutamine,and a penicillin-streptomycin antibiotic mixture (Life Technologies,Burlington, Ontario, Canada) supplemented with 5% FCS (Immunocorp,Montreal, Quebec, Canada) for HeLa or 10% calf serum (Life Technologies)for NIH-3T3 cells.

Antibodies and Chemicals

Monoclonal antibody against AMF-R was used in the form of concentrated hybridoma supernatant (Nabi et al., 1990). Rabbit anti-caveolinpolyclonal antibody was purchased from Transduction Laboratories(Lexington, KY), rabbit anti-biotin antibody was purchased fromSigma (St. Louis, MO), and rat anti-LAMP-1 was purchased fromthe Developmental Studies Hybridoma Bank (University of Iowa,Iowa City, IA). Secondary antibodies conjugated to either fluorescein,Texas Red, or 12-nm gold particles and streptavidin conjugatedto fluorescein or Texas Red were purchased from Jackson ImmunoresearchLaboratories (West Grove, PA). Texas Red-conjugated human diferrictransferrin was kindly provided by Dr. Tim McGraw (Columbia University,New York, NY). Streptavidin conjugated to 10-nm gold particleswas purchased from Sigma. The secondary antibodies were designedfor use in multiple labeling studies, and no interspecies cross-reactivitywas detected. To detect antibodies to AMF-R, secondary antibodiesspecific for the µ chain of rat immunoglobulin M (IgM) were used.

Rabbit phosphohexose isomerase was purchased from Sigma and biotinylated with NHS-LC-biotin (Pierce, Rockford, IL) accordingto the manufacturer's instructions. To assess its purity, biotinylatedphosphohexose isomerase was separated by SDS-PAGE, transferredto nitrocellulose, probed with HRP-conjugated streptavidin (JacksonImmunoresearch Laboratories) and revealed by chemiluminescence.

Immunofluorescence

Cells were plated on glass cover slips 2 d before each experiment at a concentration of 30,000 cells/35-mm dish. For AMF-Rsurface labeling, the cells were incubated in DMEM minus bicarbonatesupplemented with 25 mM HEPES, pH 7.2, and 2.5% serum for 15 minat 4°C before labeling with anti-AMF-R primary antibody or biotinylatedAMF (bAMF) at 4°C for 30 min. The cells were washed at 4°C andthen fixed with 3% paraformaldehyde in PBS (pH 7.4) supplementedwith 0.1 mM Ca⁺⁺ and 1 mM Mg⁺⁺ (PBS/CM) for 15 min at room temperature. For caveolin labeling,after AMF-R surface labeling at 4°C and fixation as above, thecells were permeabilized with 0.2% Triton X-100 for 10 min, andthen extensively washed with PBS/CM containing 1% BSA. The cellswere incubated with rabbit anti-caveolin polyclonal antibodies,washed, and then incubated with FITC goat anti-rat IgM to revealanti-AMF-R and Texas Red donkey anti-rabbit IgG to reveal anti-caveolin.Cell surface labeling with bAMF was revealed with rabbit anti-biotinantibody and fluorescent anti-rabbit secondary antibody.

For the AMF internalization studies, NIH-3T3 cells were pulsed with bAMF (~250-500 µg/ml) and chased at 37°C for the indicatedperiods of time before fixation by the addition of precooled ( $-$ 80°C)methanol/acetone directly to the cells. After fixation, internalizedbAMF was revealed with Texas Red streptavidin and lysosomes andAMF-R tubules by anti-LAMP-1 and anti-AMF-R antibodies, respectively,followed by the corresponding FITC-conjugated secondary antibodies.Disruption of clathrin-coated pits and vesicles by cytoplasmicacidification was performed essentially as previously described(Heuser, 1989). NIH-3T3 cells were pretreated with acidificationmedium (DMEM containing 5% calf serum and 50 mM 2-(N-morpholino)ethanesulfonicacid, pH 5.5) for 15 min at 37°C before addition of bAMF in acidificationmedium for 1 h at 37°C. To ensure that cellular acidificationblocked clathrin-mediated endocytosis, Texas Red transferrin (50µg/ml) was added to cells in regular or acidification medium for30 min at 37°C, after which the cells were fixed with 3% paraformaldehyde.

After labeling, the coverslips were mounted in Airvol (Air Products and Chemicals, Allentown, PA) and viewed in a Zeiss Axioskopfluorescent microscope (Carl Zeiss, Thornwood, NY) equipped witha 63× Plan Apochromat objective and selective filters. Confocalmicroscopy was performed with the 60× Nikon Plan Apochromat (Nikon,Garden City, NY) objective of a dual channel Bio-Rad MRC600 laserscanning confocal microscope (Bio-Rad, Richmond, CA) equippedwith a krypton/argon laser and the corresponding dichroic reflectorsto distinguish fluorescein and Texas Red labeling. Confocal imageswere printed using a Polaroid TX 1500 video printer.

Electron Microscopy

Postembedding immunolabeling for AMF-R was performed as previously described (Benlimame et al., 1995). Cells grown on Petridishes were rinsed and incubated at 37°C in Ringer's solutionfor 15 min before being fixed in Ringer's solution containing2% paraformaldehyde and 0.2% glutaraldehyde for 30 min at 37°C.The fixed cells were rinsed in PBS/CM, scraped from the Petridish, and collected by centrifugation. The cell pellet was postfixedfor 30 min with 1% osmium tetroxide in PBS/CM containing 1.5%potassium ferrocyanide (reduced osmium), dehydrated, and embeddedin LR-White resin. Ultrathin sections (80 nm) were blocked with2% BSA, 0.2% gelatin in PBS/CM for 1 h, and then incubated atroom temperature with anti-AMF-R antibody for 1 h followed by12 nm gold-conjugated goat anti-rat antibodies for 1 h. The sectionswere then stained with 5% uranyl acetate and examined in a Philips300 electron microscope. The numerical density of gold particlesassociated with plasma membrane, caveolae, clathrin-coated pitsand vesicles, smooth tubules and vesicles, and rough ER was determined.The length of the limiting membrane of the indicated organelleswas measured using a Sigma-Scan measurement system, and the goldparticles associated with these organelles were counted. RoughER was defined by the presence of a linear array of membrane-associatedribosomes. Smooth vesicles attached to the plasma membrane orwithin 100 nm of the plasma membrane were considered to be caveolae.Control labeling with nonimmune rat IgM antibodies was analyzedsimilarly.

To follow the endocytic pathway of AMF by electron microscopy, bAMF was internalized as described for the fluorescence studiesand detected by postembedding labeling with streptavidin conjugatedto 10 nm gold as described above. No labeling was observed inthe absence of bAMF.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Localization of AMF-R to Cell Surface Caveolae

By postembedding immunoelectron microscopy in NIH-3T3 and HeLa cells, AMF-R is primarily localized to smooth intracellularmembranous tubules (Figure 1, A and D), similar in morphologyto those previously described in MDCK cells (Benlimame et al.,1995). At the cell surface, AMF-R label localizes to smooth invaginationsof the plasma membrane morphologically equivalent to caveolae(Figure 1, B, C, E, and F). Quantification of the labeling revealedthat the predominant AMF-R label is localized to smooth tubulesand vesicles, flat regions of the plasma membrane, and caveolae(Table 1). While specific label was previously detected in therough ER of MDCK cells (Benlimame et al., 1995), the density oflabeling of rough ER tubules in NIH-3T3 and HeLa cells is reducedand at control levels. The density of AMF-R labeling of caveolaeis equal to that of intracellular smooth tubules and vesiclesin NIH-3T3 cells and greater than that of intracellular smoothtubules and vesicles in HeLa cells, and essentially no AMF-R labelis found within clathrin-coated pits and vesicles. The densityof AMF-R labeling in caveolae is increased relative to flat regionsof the plasma membrane. However, based on the total number ofgold particles at the plasma membrane, only 13% of cell surfaceAMF-R in NIH-3T3 and 26% in HeLa cells is found within caveolae.

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Figure 1. Electron microscopic localization of AMF-R in NIH-3T3 fibroblasts and HeLa cells. HeLa (A, B, and C) and NIH-3T3 (D, E, and F) cells were postembedding immunolabeled with anti-AMF-R and 12-nm gold-conjugated anti-rat IgM secondary antibodies. Typical AMF-R labeling of smooth tubules (A and D, arrows) and cell surface caveolae (B, C, E, F, arrowheads) is shown. PM, Plasma membrane. Bar, 0.2 µm.

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Table 1. Localization of AMF-R in HeLa and NIH-3T3 cells by immunoelectron microscopy

To assess whether cell surface AMF-R colocalizes with caveolin, viable NIH-3T3 cells were surface labeled for AMF-R by theaddition of anti-AMF-R antibodies to the cells at 4°C (Nabi etal., 1992) and then double immunofluorescently labeled after fixationand permeabilization with antibodies to caveolin (Figure 2). Whilethe punctate AMF-R surface label (Figure 2A) did not completelycolocalize with the finer caveolin labeling (Figure 2B), confocalmicroscopy clearly revealed distinct points and patterns labeledfor both cell surface AMF-R and caveolin (Figure 2C, yellow).Peripheral regions densely labeled for both AMF-R and caveolinwere frequently observed. The partial colocalization of cell surfaceAMF-R with caveolin is consistent with the fact that, based onthe electron microscopic data, only 13% of cell surface AMF-Rwas localized within the caveolae of NIH-3T3 cells.

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Figure 2. Colocalization of AMF-R and caveolin by confocal microscopy. Viable NIH-3T3 cells were labeled for cell surface AMF-R at 4°C (A) and for caveolin after fixation and permeabilization (B). To demonstrate the colocalization of AMF-R and caveolin, confocal images from both fluorescent channels were superimposed (panel C; AMF-R in green and caveolin in red) and colocalization appears in yellow. Bar, 20 µm.

Internalization of AMF

The ligand for AMF-R, AMF, is homologous to phosphohexose isomerase (Watanabe et al., 1996). Phosphohexose isomerase (referredto here as AMF) was biotinylated and after separation by SDS-PAGErevealed a single major band after revelation of the blots withstreptavidin-HRP (Figure 3A). Cell surface labeling of NIH-3T3cells by the addition of both bAMF (Figure 3B) and anti-AMF-Rat 4°C (Figure 3C) revealed a high degree of colocalization (Figure3D, yellow), demonstrating that AMF and antibodies to AMF-R recognizethe same receptor. The presence of spots labeled exclusively witheither bAMF or anti-AMF-R may be due to the fact that the twowere added together and may compete for the same site. Indeed,the addition of excess cold AMF before cell surface labeling withanti-AMF-R significantly reduced binding of the antibody (ourunpublished observations), as previously demonstrated by immunoblot(Nabi et al., 1990).

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Figure 3. bAMF and anti-AMF-R mAb colocalize on the cell surface. bAMF migrated as a single band in protein blots revealed with HRP-streptavidin (A). Confocal imaging of cell surface labeling of viable NIH-3T3 cells at 4°C with bAMF (B) or anti-AMF-R antibody (C). Confocal images from both fluorescent channels were superimposed (panel D; bAMF in green and AMF-R in red) and revealed a significant degree of colocalization in yellow. Bar, 20 µm.

Pulse labeling of NIH-3T3 cells with bAMF for 1 or 2 h resulted in the ability to detect both punctate structures as wellas fainter tubular structures that colocalized with AMF-R tubules(Figure 4, A and B). Under these conditions, the extent of punctateand tubular labeling varied between cells. Fibrillar labelingof bAMF was also observed and has been determined to be localizedto the cell surface (our unpublished results). An extended chaseof 2 or 4 h after a 2-h pulse resulted in decreased punctate labelingand the accumulation of bAMF labeling in tubular structures thatcolocalized with AMF-R tubules (Figure 4, C and D). The vast majorityof the cells exhibited predominantly intracellular tubular labelingas well as cell surface fibrillar labeling. After treatment ofcells with acidified medium (pH 5.5) and disruption of clathrin-coatedpits and vesicles (Heuser, 1989), bAMF internalized for 1 h islocalized to intracellular AMF-R tubules (Figure 4, E and F).In the acidified medium, internalized transferrin did not clusterin the perinuclear recycling compartment, demonstrating that theacidification procedure did indeed disrupt clathrin-mediated endocytosis(Figure 4, G and H). bAMF is therefore internalized via a clathrin-independentendocytic pathway to the smooth ER.

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Figure 4. Internalization of bAMF to AMF-R tubules. NIH-3T3 cells were pulse labeled with bAMF at 37°C for 1 h (A and B), for 2 h and chased for 4 h (C and D), or for 1 h in medium acidified to pH 5.5 to disrupt clathrin-mediated endocytosis (E and F). After fixation with methanol/acetone, cells were double labeled with Texas Red-streptavidin to reveal bAMF (A, C, and E) and anti-AMF-R mAb and FITC-conjugated anti-rat secondary antibody to reveal AMF-R labeling (B, D, and F). To ensure that cellular acidification disrupted clathrin-mediated endocytosis of transferrin receptor, NIH-3T3 cells were incubated at 37°C with Texas Red transferrin for 30 min in regular medium (G) or in medium acidified to pH 5.5 (H). Bar, 20 µm.

The colocalization of bAMF-labeled tubules with AMF-R tubules was confirmed by confocal microscopy (Figure 5). After a 1-hbAMF internalization, internalized bAMF is localized to tubularstructures that colocalize with AMF-R tubules (Figure 5, A-C)as well as to punctate structures that exhibit partial colocalizationwith LAMP-1-positive lysosomes (Figure 5, D-F). As seen here,the intense punctate labeling can hide the fainter tubular labelingof bAMF in some cells (Figures 4A and 5D). In acidification medium,the vast majority of bAMF labeling, aside from cell surface fibrils,is localized to tubules that colocalize with AMF-R tubules (Figure5, G-I). bAMF internalized for 1 h in the presence of a 10-foldexcess of unlabeled AMF is localized only to punctate structures,and no labeling of AMF-R tubules can be detected (Figure 5, J-L).While the extent of tubular labeling of bAMF varies between cellsunder control conditions (Figure 5, A and D), in the presenceof excess unlabeled AMF the localization of bAMF to AMF-R tubulesis never observed (Figure 5, J-L). bAMF internalization to intracellularAMF-R tubules therefore occurs via a receptor-mediated process.The inability of excess AMF to block bAMF internalization to punctateperinuclear structures, which exhibit partial colocalization withLAMP-1-labeled lysosomes (our unpublished observations), demonstratesthat this labeling is not saturable and corresponds to nonspecificfluid phase uptake. The disappearance of lysosomal labeling afterextended chase times (Figure 4, C and D) is therefore most likelydue to lysosomal degradation of fluid phase-internalized bAMF.

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Figure 5. Localization of internalized bAMF to AMF-R tubules by confocal microscopy. NIH-3T3 cells were pulse labeled with bAMF at 37°C for 1 h in regular medium (A-F) for 1 h in medium acidified to pH 5.5 to disrupt clathrin-mediated endocytosis (G-I), or in regular medium in the presence of 10-fold excess unlabeled AMF (J-L) before fixation with methanol/acetone. bAMF was revealed with Texas Red-streptavidin (A, D, G, and J) and AMF-R (B, H, and K) or LAMP-1 (E) labeled with the appropriate primary antibodies and FITC-conjugated secondary antibodies. Confocal images from both fluorescent channels were superimposed (panels C, I, and L, bAMF in red and AMF-R in green; panel F, bAMF in red and LAMP-1 in green) and colocalization appears in yellow. Bar, 10 µm.

The location of bAMF internalized at 37°C was determined by postembedding electron microscopy with streptavidin-10 nm gold.After a 10-min pulse bAMF could be detected in caveolae (Figure6, A and B). After a 30-min pulse, both caveolae and intracellularsmooth and rough ER elements were labeled (Figure 6, C-G). Densestructures morphologically equivalent to lysosomes are also labeledand presumably correspond to the perinuclear structures denselylabeled for internalized bAMF by immunofluorescence (Figure 6,H and I).

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Figure 6. Electron microscopy of the internalization pathway of bAMF. NIH-3T3 cells were pulsed with bAMF at 37°C for 10 (A, B, and H) or 30 min (C, D, E, F, G, and I). The localization of bAMF was revealed by postembedding labeling with 10-nm gold-conjugated streptavidin. After 10 min, bAMF is localized to cell surface caveolae (A and B). After a 30-min pulse, bAMF is localized to caveolae and smooth vesicles (C and D) and also appears in intracellular membranous tubules (E, F, and G) including distinctive smooth (E) and rough (F) ER elements. bAMF labeling of dense lysosomal structures is also detected (H and I). Bar, 0.1 µm.

	DISCUSSION

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AMF-R Localization to Caveolae

Caveolae are smooth plasmalemmal vesicles whose cytoplasmic surface presents a spiral coat containing the 21-kDa caveolae-specificphosphoprotein caveolin (Rothberg et al., 1992). By postembeddingimmunoelectron microscopy, AMF-R is localized to morphologicallyidentifiable caveolae as well as to smooth ER tubules (Figure1 and Table 1). In contrast to polarized epithelial MDCK cells(Benlimame et al., 1995), labeling of rough ER tubules was notabove background in either NIH-3T3 or HeLa cells, indicating thatAMF-R is a specific marker for smooth ER in these two cell types.The localization of AMF-R to caveolae was confirmed by the colocalizationof cell surface AMF-R, labeled by the addition of anti-AMF-R toviable cells at 4°C, with caveolin by confocal fluorescence microscopy(Figure 2). By both postembedding immunoelectron microscopy andconfocal double labeling with caveolin, only a minor portion ofcell surface AMF-R actually is distributed to caveolae identifiedeither morphologically or by the presence of caveolin. Whetherflat plasma membrane regions to which AMF-R is localized are equivalentto cholesterol-rich Triton X-100-insoluble glycolipid rafts (Brownand Rose, 1992; Sargiacomo et al., 1993; Chang et al., 1994) isdifficult to assess due to the large quantity of AMF-R localizedto intracellular tubules (61% in NIH-3T3 and 74% in HeLa; seeTable 1). Based on the labeling of AMF-R by immunoelectron microscopy,only ~5% of total cellular AMF-R is actually localized to caveolae(Table 1).

Transduction of the AMF motility signal is mediated by a pertussis toxin-sensitive G protein, phosphorylation of AMF-R, andboth PKC and tyrosine kinase activities (Stracke et al., 1987;Nabi et al., 1990; Watanabe et al., 1991; Timar et al., 1993;Kanbe et al., 1994). Heterotrimeric G proteins, including thepertussis toxin-sensitive G_i2 protein, have been shown toassociate with caveolar domains (Sargiacomo et al., 1993; Changet al., 1994; Schnitzer et al., 1995) although results from anotherstudy indicate that heterotrimeric G proteins do not associatewith an immunoisolated caveolae fraction (Stan et al., 1997).The AMF-R sequence codes for a putative type 1 membrane proteinand contains within its cytoplasmic domain a consensus sequencefor a G protein activator motif (Watanabe et al., 1991; Okamotoand Nishimoto, 1992; Silletti et al., 1996). The association ofAMF-R with caveolae could serve to facilitate its interactionwith heterotrimeric G proteins after receptor activation. Caveolinwas originally identified as a phosphorylated substrate of Roussarcoma virus tyrosine kinase, and tyrosine kinase activitieshave been localized to caveolae (Glenney, 1989; Sargiacomo etal., 1993; Shenoy-Scaria et al., 1994; Robbins et al., 1995; Liuet al., 1997). The flattening of caveolae at the plasma membraneis stimulated by the PKC stimulator, phorbol 12-myristate 13-acetate,and the okadaic acid-mediated internalization of caveolae is blockedby the kinase inhibitor staurosporine, suggesting that PKC activitymay be associated with caveolae (Smart et al., 1993; Parton etal., 1994). The involvement of heterotrimeric G proteins as wellas tyrosine kinase and PKC activities in transduction of the AMFmotility signal is consistent with the localization of AMF-R tocell surface caveolae.

Clathrin-independent Internalization of AMF-R to Smooth ER Tubules

The presence of AMF-R both at the cell surface and within an intracellular ER-associated organelle suggested that the receptorrecycles between these two cellular sites (Nabi et al., 1992;Benlimame et al., 1995). Caveolae have been implicated in transcytosisin endothelial cells (Palade et al., 1979; Ghitescu et al., 1986;Schnitzer et al., 1994), and interaction between caveolae andsmooth ER has been proposed for the vascular endothelium (Bundgaard,1991). The inositol triphosphate receptor-like protein has beenlocalized to caveolae, and this protein is expressed not onlyat the plasma membrane but also within the ER (Fujimoto et al.,1992; Sharp et al., 1992). The fact that the density of AMF-Rlabeling within caveolae is equivalent to (NIH-3T3) or greaterthan (HeLa) that of smooth vesicles and tubules is consistentwith the concentration of AMF-R within caveolae before vesiclebudding and fusion with AMF-R tubules (Table 1).

AMF exhibits sequence identity to phosphohexose isomerase (Watanabe et al., 1996). Biotinylated phosphohexose isomerase orbAMF colocalizes with cell surface AMF-R labeled with antibodiesto AMF-R at 4°C and is endocytosed by cells at 37°C to tubulesthat colocalize with smooth ER AMF-R tubules by confocal microscopyand to morphologically identifiable ER tubules by electron microscopy.bAMF internalization to smooth ER tubules is a receptor-mediatedprocess as it can be blocked by the presence of excess unlabeledAMF. Cellular acidification, which specifically blocks clathrin-mediatedendocytosis, disrupts the internalization of transferrin, butnot that of bAMF to AMF-R tubules, demonstrating that AMF-R isinternalized to AMF-R tubules via a nonclathrin endocytic pathway.Under the conditions used in these experiments, internalizationof bAMF to lysosomal structures is also observed. This lysosomallabeling is observed even in the presence of excess unlabeledAMF, indicating that it is not receptor-mediated and due to fluidphase uptake. We have therefore identified a clathrin-independentAMF-R-mediated endocytic pathway that targets bAMF to the ER.The localization of AMF-R and internalized bAMF to cell surfacecaveolae by electron microscopy implicates these smooth invaginationsof the plasma membrane in the endocytosis of AMF-R to the smoothER subdomain for which it is a marker (Benlimame et al., 1995;Wang et al., 1997).

Role of Caveolae in AMF-R Internalization

Whether caveolae are involved in endocytic processes in nonendothelial cells remains a controversial subject. The transientopening and shutting of caveolae at the cell surface, in the absenceof dissociation from the plasma membrane, creates localized ligandconcentrations, which enter the cell via a process called potocytosis(Anderson et al., 1992). Caveolin-positive intracellular endocyticstructures have been identified in elicited macrophages (Kissand Geuze, 1997). Clathrin-independent internalization of thecholecystokinin receptor, apparently via caveolae, targeted thereceptor only to subplasmalemmal vesicles (Roettger et al., 1995).Non-clathrin-mediated endocytosis has been identified in nonendothelialcells for a number of ligands, among them cholera toxin, ricin,and the $beta$ -adrenergic receptor (Montesano et al., 1982; Sandviget al., 1987; Raposo et al., 1989). Cholera toxin and ricin aretargeted to the same endosomes as transferrin receptor (Tran etal., 1987; Hansen et al., 1993), indicating that ligands internalizedvia clathrin and nonclathrin invaginations can follow the endosomal/lysosomalpathway. Disruption of clathrin polymerization does not influencethe extent of bulk flow internalization (Cupers et al., 1994)and whether these clathrin-independent internalization routesinvolve caveolae or clathrin-coated pits without the clathrinremains to be determined (van Deurs et al., 1993).

The receptor-mediated endocytosis of bAMF not to endosomes and lysosomes but to the ER certainly suggests that bAMF endocytosisis not mediated by uncoated clathrin vesicles. Internalizationof anti-AMF-R mAb to intracellular tubular structures has alsobeen visualized in metastatic K1735 melanoma cell variants (Sillettiet al., 1994). Furthermore, alternate internalization routes involvingcaveolae have been described. Treatment of A431 cells with thephosphatase inhibitor okadaic acid enhances the ability of caveolaelabeled with cholera toxin to dissociate from the plasma membrane;internalized cholera toxin was targeted to intracellular tubularprofiles and clusters of caveolae, some of which were not labeledby fluid phase uptake (Parton et al., 1994). Cholesterol depletionresults in the internalization of caveolin and its recycling viathe ER, ERGIC, and the Golgi apparatus to the plasma membrane(Smart et al., 1994; Conrad et al., 1995). SV40 virus associateswith caveolae and is internalized via smooth plasmalemmal vesiclesto smooth tubules that are extensions of the ER (Kartenbeck etal., 1989; Anderson et al., 1996; Stang et al., 1997). The internalizationpathway of SV40 to the ER (Kartenbeck et al., 1989) is thereforeremarkably similar to that of AMF-R described here, and the localizationof both AMF-R and SV40 to cell surface caveolae certainly implicatescaveolae in this ER-directed endocytic pathway. It can be arguedthat the caveolae to which AMF-R is localized at steady stateare not necessarily involved in its clathrin-independent endocytosis;however, we would argue that the best interpretation of our datais that AMF-R internalization to the ER occurs via caveolae. Distinctreceptor-mediated caveolae internalization pathways have beendescribed in endothelial cells of the rete mirabile (Bendayanand Rasio, 1996), and it is conceivable that morphologically indistinguishablebut functionally distinct subpopulations of caveolae exist. AMFactivation of AMF-R may stimulate both transduction of the AMFmotility-stimulating signal and internalization of AMF-R, perhapswithin the same cell surface caveolar domain.

The identification of caveolin as a phosphorylated substrate for the src tyrosine kinase is indicative of a role for caveolaein cellular transformation (Glenney, 1989). AMF-R localizationto these cell surface structures further implicates them in tumorcell malignancy and metastasis. Oncogene transformation of NIH-3T3cells results in the loss of caveolin expression and disappearanceof caveolae (Koleske et al., 1995) while treatment with the tumorpromotor, phorbol 12-myristate 13-acetate, also results in thedisappearance of caveolar invaginations (Smart et al., 1993).In lymphocytes or Sf21 insect cells that lack caveolin and caveolae,the formation of cell surface caveolae as well as intracellularcaveolar vesicles can be induced after transfection with caveolin,suggesting that caveolin expression is necessary for caveolarinvagination (Fra et al., 1995; Li et al., 1996). Alternatively,caveolin may serve to stabilize caveolar invaginations at thecell surface.

AMF Recycling and Cell Motility

The established role of AMF-R in cell motility and metastasis implicates AMF-R internalization, and subsequent recycling tothe cell surface, in the motile process (Nabi et al., 1992; Sillettiand Raz, 1996). The potential involvement of a caveolae-mediatedrecycling pathway via an ER-associated organelle in cell motilitycomplements the previously described role for coated pit internalizationand recycling (Bretscher, 1984; Altankov and Grinnell, 1993),the targeting of Golgi-derived membrane vesicles (Bergmann etal., 1983; Rogalski et al., 1984; Peränen et al., 1996), andthe recycling of early endosomal or lysosomal proteins (Bretscher,1989; Garrigues et al., 1994; Hopkins et al., 1994) in cellularmovement. The extension of lamellipodia by the motile cell requiresthe continual generation of de novo polarized membrane domains.The targeting of the bulk of intracellular membrane traffic towardthe site of formation of new membrane domains, the leading edge,is therefore not surprising. Targeting of intracellular membranetraffic is, in large part, mediated by the microtubule cytoskeleton(Kelly, 1990; Cole and Lippincott-Schwartz, 1995) whose role indetermining the directionality of membrane traffic to the leadingedge as well as the directionality of cell movement has been demonstrated(Rogalski et al., 1984; Tanaka et al., 1995). AMF-R tubules associatewith a pericentriolar microtubule subdomain enriched in stabilizedmicrotubules in Moloney sarcoma virus-transformed epithelial MDCKcells, supporting a role for microtubules in the intracellulartargeting of AMF-R tubules (Nabi et al., 1997). The role of microtubulesin the directionality of lamellipodial extension and cell movementmay be to target intracellular membrane traffic to the leadingedge of the motile cell. It should be noted, however, that whilecells in serum culture are continually motile, cell motility insitu occurs in response to specific motile stimuli (Stoker andGherardi, 1991). A recycling pathway stimulated by a cytokine,such as AMF, may represent a motility-specific membrane-targetingpathway.

	ACKNOWLEDGMENTS

These studies were made possible by the prior work of Avraham Raz and Hideomi Watanabe. We thank Danièle Simard for her earlycontributions to this project and M. Bendayan, L. Ghitescu, andM. Desjardins for helpful discussions throughout the work andfor critical reading of the text. The technical assistance ofGinette Guay and the photographic work of Jean Leveillé are sincerelyappreciated. This work was supported by grants from the MedicalResearch Council of Canada, the National Cancer Institute of Canada,and by an establishment grant from Fonds pour la Formation deChercheurs et l'Aide à la Recherche.

	FOOTNOTES

^* Corresponding author.

REFERENCES

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

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