Heparin-binding EGF-like growth factor (HB-EGF) is a ligand for EGF receptor (EGFR) and possesses the ability to signal in juxtacrine, autocrine and/or paracrine mode, with these alternatives being governed by the degree of proteolytic release of the ligand. Although the spatial range of diffusion of released HB-EGF is restricted by binding heparan-sulfate proteoglycans (HSPGs) in the extracellular matrix and/or cellular glycocalyx, ascertaining mechanisms governing non-released HB-EGF localization is also important for understanding its effects. We have employed a new method for independently tracking the localization of the extracellular EGF-like domain of HB-EGF and the cytoplasmic C-terminus. A striking observation was the absence of the HB-EGF transmembrane pro-form from the leading edge of COS-7 cells in a wound-closure assay; instead, this protein localized in regions of cell-cell contact. A battery of detailed experiments found that this localization derives from a trans interaction between extracellular HSPGs and the HB-EGF heparin-binding domain, and that disruption of this interaction leads to increased release of soluble ligand and a switch in cell phenotype from juxtacrine-induced growth inhibition to autocrine-induced proliferation. Our results indicate that extracellular HSPGs serve to sequester the transmembrane pro-form of HB-EGF at the point of cell-cell contact, and that this plays a role in governing the balance between juxtacrine versus autocrine and paracrine signaling.
Introduction
Heparin-binding epidermal-growth-factor (EGF)-like growth factor (HB-EGF) is a ligand in the EGF receptor (EGFR) family that activates the EGFR (Higashiyama et al., 1991) and ErbB4 (also known as HER4) (Elenius et al., 1997), and binds heparan-sulfate proteoglycans (HSPGs) present on the cell surface and in the extracellular matrix (Higashiyama et al., 1991) by means of a heparin-binding domain (HBD) (Thompson et al., 1994). As with all EGFR-family ligands, HB-EGF is synthesized in pro-form as a transmembrane protein that is proteolytically cleaved from the cell surface to yield a soluble form that can activate receptors in autocrine and/or paracrine mode (Harris et al., 2003; Singh and Harris, 2005; Higashiyama et al., 2008) or bind to HSPGs. However, HB-EGF also has the ability to signal in juxtacrine mode by activating receptors on a neighboring cell while still being anchored to the plasma membrane. HB-EGF associates with the tetraspanin protein CD9, which enhances its juxtacrine activity (Higashiyama et al., 1995; Iwamoto et al., 1991) and links HB-EGF to α3β1 integrins (Nakamura et al., 1995). CD9 also interacts with HB-EGF via its HBD (Sakuma et al., 1997).
HB-EGF juxtacrine signaling and autocrine and/or paracrine signaling have been shown to elicit different phenotypes, with autocrine and/or paracrine activity leading to cell proliferation and migration (Higashiyama et al., 1991; Yahata et al., 2006), and juxtacrine activity causing growth inhibition and in some cases apoptosis (Iwamoto et al., 1999; Pan et al., 2002). HB-EGF proteolytic cleavage and subsequent autocrine signaling drives physiologically beneficial migration of a variety of tissue cells, such as keratinocytes (Shirakata et al., 2005; Tokumaru et al., 2000), corneal epithelial cells (Block et al., 2004; Xu et al., 2004), smooth-muscle cells (Bakken et al., 2009), peritoneal mesothelial cells (Faull et al., 2001) and mesenchymal stem cells (Ozaki et al., 2007) during wound healing. Soluble HB-EGF stimulation is also crucially involved in invasive motility of aggressive solid tumors, particularly ovarian cancer (Yagi et al., 2008; Matsuzaki et al., 2005; Tanaka et al., 2005; Miyamoto et al., 2004) among others (Normanno et al., 2001).
We have previously shown that soluble HB-EGF can operate in a highly localized spatial domain following its proteolytic release (Yoshioka et al., 2005), owing to a combination of restricted diffusion and fast binding to cell surface receptors. Both of these localization processes might arise from interactions with HSPGs – residing in extracellular matrix for the former, or on the cellular glycocalyx for the latter. Moreover, human mammary epithelial cells, driven by proteolytic release of the soluble autocrine EGF ligand, migrate in a more directionally persistent manner compared with cells treated with EGF ligand exogenously (Maheshwari et al., 2001). We have shown by computational modeling that the EGFR system might be capable of producing spatially localized autocrine signaling loops (Maly et al., 2004), and have found in ensuing experimental studies that autocrine EGF drives migration effectively (Joslin et al., 2007).
Because of the disparity in cell phenotypic responses to juxtacrine HB-EGF signaling versus autocrine and/or paracrine HB-EGF signaling, and the prospective importance of spatial localization of both the transmembrane pro-form as well as the soluble mature form, ascertaining mechanisms responsible for governing localization and proteolytic cleavage of this ligand is important for understanding its physiological and pathological effects. Previous work has provided crucial insights into the roles played by the membrane-anchoring domain of the ligand (Dong et al., 2005), regulatory signaling pathways (Herrlich et al., 2008) and extracellular-matrix HSPGs (Forsten-Williams et al., 2008). Thus, we endeavor here to offer a contribution elucidating how HSPGs in the cellular glycocalyx might influence localization and/or release of HB-EGF.
Our goal is complicated by the growing evidence that the C-terminal fragment of HB-EGF, consisting of the transmembrane and cytoplasmic domains, might provide signaling information separately from the extracellular domain (Higashiyama et al., 2008). This fragment can translocate to the nucleus and reverse gene repression of the transcriptional repressors promyelocytic leukemia zinc finger protein (PLZF) and Bcl6 (Kinugasa et al., 2007; Nanba et al., 2003). Therefore, in exploring processes governing HB-EGF localization, it is imperative to distinguish the extracellular EGF-like domain from the intracellular C-terminal fragment, because they are both signaling molecules that can have different localization after ligand cleavage. To address this challenge, we incorporated different visualization tags at the extracellular and intracellular domains of pro-HB-EGF. For the former, we employed an acceptor peptide enabling biotinylation for subsequent visualization with a streptavidin-conjugated fluorophore and attached green fluorescent protein (GFP) to the C-terminus for the latter. This construct facilitated novel examination of interactions between HSPGs and membrane-anchored HB-EGF (pro-HB-EGF), and consequent of the effects on ligand behavior. A key finding is that pro-HB-EGF binding to HSPGs on adjacent cells (in trans) is responsible for localization of pro-HB-EGF to sites of cell-cell contact, prevents proteolytic cleavage and promotes growth inhibition. This suggests a novel negative control mechanism for HB-EGF autocrine and/or paracrine signaling through sequestration of the pro-form by HSPGs.
Results
Pro-HB-EGF is localized at sites of cell-cell contact and is absent from the wound edge
In order to independently track the C-terminal tail and the extracellular domain of HB-EGF, a construct [acceptor-peptide (AP)–HB-EGF–GFP] was designed to allow two-color tracking of the localization of each fragment. A 14-amino-acid acceptor-peptide tag was inserted before the shortest of the five N-terminal cleavage sites in the extracellular domain of murine HB-EGF (Fig. 1A). The acceptor-peptide tag allows for biotinylation of one specific lysine residue in the sequence with the enzyme biotin ligase (BirA) (Beckett et al., 1999) and subsequent fluorescent labeling with a streptavidin-conjugated fluorophore (Fig. 1B). GFP was conjugated to the cytoplasmic C-terminus of HB-EGF. Acceptor-peptide labeling has the advantage that only the cell-surface pool of the protein is labeled, because streptavidin is not permeable to the cell membrane, whereas the GFP signal represents the total intracellular and plasma-membrane fraction of AP–HB-EGF–GFP. Insertion of the acceptor peptide near the N-terminus of HB-EGF and biotinylation of the tag did not affect the autocrine- and/or paracrine-growth-factor activity of the protein, as assessed by phosphorylation of the EGFR (Fig. 1C). Biotinylated AP–HB-EGF was purified from the conditioned media of COS-7 cells with heparin beads and used to stimulate naïve COS-7 cells. The purified growth factor phosphorylated the EGFR at tyrosine 1148 in the same manner as recombinant human HB-EGF (rhHB-EGF). Additionally, a heparin-bead eluant from cells lacking AP–HB-EGF expression to control for other heparin-binding growth factors in the media showed little activation of the EGFR. The activity of streptavidin-bound AP–HB-EGF was not assessed, because streptavidin labeling was only performed immediately before image acquisition. The localization of AP–HB-EGF (no GFP) and HB-EGF–GFP (no AP) were identical, suggesting that neither insertion of the AP nor GFP conjugation disrupted the localization of the protein (see supplementary material Fig. S1).
AP–HB-EGF–GFP was successfully expressed in COS-7 cells and labeled with a streptavidin-conjugated fluorophore. Cells were co-transfected with the AP–HB-EGF–GFP construct and a plasmid encoding BirA with an endoplasmic-reticulum localization sequence (BirA-ER). BirA-ER expression leads to biotinylation of acceptor-peptide-tagged proteins in the endoplasmic reticulum, utilizing endogenous ATP and biotin supplemented in the media. After 24 hours of transfection, biotinylated proteins on the cell surface were visualized with an engineered monovalent streptavidin-fluorophore conjugate that does not promote protein crosslinking (Howarth et al., 2006; Howarth and Ting, 2008) (mSA-AF568) in all experiments with the exception of those in Fig. 2, in which streptavidin-Cy5 was utilized after paraformaldehyde fixation to allow for co-staining with N-cadherin to visualize sites of cell-cell contact. In some of the cells, only the GFP fluorescence (green, Fig. 2) but no acceptor peptide labeling (red, Fig. 2) was observed, which is probably due to inefficient co-transfection with BirA-ER. In most cells, however, the colocalization of the HB-EGF extracellular acceptor peptide (red, Fig. 2A), intracellular HB-EGF C-terminal GFP tail (green, Fig. 2A), and the cell-cell adhesion protein N-cadherin (white, Fig. 2A), showed that AP–HB-EGF–GFP was present on the cell surface in the uncleaved pro-form at sites of cell-cell contact, which is consistent with previous reports (Goishi et al., 1995; Singh et al., 2004). The localization of the two HB-EGF tags occasionally differed in the perinuclear region, where only the GFP signal was present in intracellular vesicles, which are probably part of the secretory pathway.
To determine the localization of the extracellular and intracellular domains of HB-EGF during cell migration, a wound-closure assay was employed to directionally control cell migration. Confluent monolayers of COS-7 cells expressing AP–HB-EGF–GFP were scratch-wounded and allowed to close for 4 hours, then the extracellular biotinylated acceptor peptide was labeled with streptavidin-Cy5 and sites of cell-cell contact were visualized with N-cadherin immunostaining. We observed that both the extracellular EGF-like domain (red, Fig. 2B) and cytoplasmic tail (green, Fig. 2B) of HB-EGF were completely absent from the wound edge, and remained only at sites of cell-cell contact. Because of the well-established role of HB-EGF in wound healing and chemotaxis, we hypothesized that HB-EGF was preferentially cleaved from the wound edge, inducing a polarized autocrine loop of EGFR activation and cleavage at the leading edge of the cell. To test this hypothesis, treatments aimed at blocking the autocrine signaling loop were used on COS-7 cells before induction of the wound. These included inhibition of proteolytic cleavage of pro-HB-EGF with batimastat and GM6001, blocking of EGFR-ligand binding with mAb225, inhibition of EGFR kinase activity with AG1478, and inhibition of intracellular pathways downstream of the EGFR using inhibitors to ERK (PD98059), Src (PP2) and PI3K (LY294002). However, none of these treatments prevented the loss of HB-EGF from the leading edge of transfected cells after wounding (see supplementary material Fig. S2). Pro-HB-EGF was also localized only at sites of cell-cell contact and was absent from any free edges in sparsely plated COS-7 cells (Fig. 2C). This suggested that, rather than loss by cleavage, it was loss of cell-cell contact that led to the absence of HB-EGF from the leading edge of cells at the wound edge. The fraction of HB-EGF at sites of cell-cell contact was quantified by measuring the amount of extracellular AP–HB-EGF–GFP colocalized with N-cadherin immunostaining normalized to the total HB-EGF area in cells that were sparse, at the wound edge or in confluent monolayers. Additionally, the fraction of the cell perimeter in cell-cell contact was calculated by measuring the length of the cell periphery positive for N-cadherin immunostaining, and normalizing this to the total cell periphery. These data indicate that the fraction of HB-EGF at sites of cell-cell contact remains constant at approximately 80%, independent of the degree of cell-cell contact (Fig. 2D).
Role of the HBD in pro-HB-EGF localization to sites of cell-cell contact
Because pro-HB-EGF was observed primarily at sites of cell-cell contact, the question arose of what molecular interactions between cells led to pro-HB-EGF concentration in this area. Because the extracellular domain of pro-HB-EGF has the ability to interact with cell-surface HSPGs, we hypothesized that this interaction might control localization of HB-EGF to sites of cell-cell contact. To test this hypothesis, we sought to compete for HSPG binding to pro-HB-EGF with exogenous heparin and heparan sulfate. We found that heparin and heparan sulfate (100 μg/ml) dramatically changed the localization of AP–HB-EGF–GFP (Fig. 3A,B). The extracellular (red, Fig. 3) and intracellular (green, Fig. 3) domain of AP–HB-EGF–GFP changed from localization primarily at sites of cell-cell contact to a homogenous distribution over the entire cell surface. Although the results shown in Fig. 3 are after 4 hours of treatment, changes in pro-HB-EGF localization were observed as soon as 5 minutes following heparin addition (see supplementary material Fig. S3). The minimum concentration required to change the localization of HB-EGF after 4 hours was determined to be approximately 0.1 μg/ml of heparin and 10 μg/ml of heparan sulfate. The addition of the glycosaminoglycan chondroitin sulfate (100 μg/ml) did not affect the localization of AP–HB-EGF–GFP (Fig. 3C). At 24 hours after the removal of heparin, AP–HB-EGF–GFP localized back to sites of cell-cell contact as observed before the addition of heparin (R.N.P., unpublished). These data indicate that an interaction with HSPGs was responsible for localizing HB-EGF to sites of cell-cell contact.
To further test our hypothesis, we aimed to diminish HSPG–pro-HB-EGF interactions by manipulating HSPGs. Culture of COS-7 cells expressing AP–HB-EGF–GFP for 24 hours with 50 mM sodium chlorate, an inhibitor of protein sulfation that blocks the enzyme ATP sulfurylase (Baeuerle and Huttner, 1986), led to a homogeneous distribution of AP–HB-EGF–GFP over the cell surface (Fig. 4A), similar to the effect seen with the addition of heparin. Additionally, digestion of cell-surface heparan sulfate with heparinase III (1.6 mU/ml) for 4 hours similarly changed the localization of AP–HB-EGF–GFP, although some AP–HB-EGF–GFP remained at sites of cell-cell contact (Fig. 4B). It might be that some heparan-sulfate chains bound to HB-EGF are protected from degradation by heparinase, as is the case with bFGF and mammalian heparanase (Tumova and Bame, 1997). Competition for 4 hours with an HBD peptide (100 μM) consisting of the 21-amino-acid sequence of the HBD of murine HB-EGF also changed the localization of HB-EGF (Fig. 4C). Neither treatment with heparin nor heparinase III affected cell-cell junctions, as assessed by N-cadherin immunostaining after 4 hours of treatment (Fig. 4D). Thus, the reduction of all sulfated proteins with sodium chlorate, the removal of cell-surface heparan sulfate with heparinase III and competition with an HBD peptide reduced the amount of AP–HB-EGF–GFP at sites of cell-cell contact, leading to a more homogenous distribution over the cell surface.
As a complementary approach to reduce the interaction of pro-HB-EGF with cell-surface HSPGs, we made four different mutants of AP–HB-EGF–GFP to inhibit the ability of HB-EGF to interact with heparan sulfate (Table 1). The HBD of HB-EGF consists of amino acids 93-113 of the mouse protein, which contains 12 basic lysine and arginine residues that are responsible for the HB-EGF interaction with heparin (Thompson et al., 1994). Residues 108-113 lie within the EGF-like domain and contain three of the basic amino acids. Deletion of the portion of the HBD that lies outside the EGF-like domain (93-105) (AP–delHBD-HB-EGF–GFP) led to a homogeneous distribution of HB-EGF over the cell surface (Fig. 5A), similar to that seen with the addition of heparin. By contrast, mutation of the first five positive lysine residues (93-97) in the HBD to non-polar alanine (AP–97A-HB-EGF–GFP) had no effect on the localization of HB-EGF (Fig. 5B). Mutation of an additional four lysine and arginine residues to alanine (93-105) (AP–105A-HB-EGF–GFP) was nonetheless sufficient to change the localization of AP–HB-EGF–GFP to a homogenous distribution over the cell surface (Fig. 5C). The same result was observed with the mutation of all 12 basic amino acids in the HBD to alanine, including those within the EGF-like domain (AP–113A-HB-EGF–GFP) (Fig. 5D). Correct localization of HB-EGF to the plasma-membrane fraction was observed in all HBD mutants, as well as after treatment with heparin and heparinase III (see supplementary material Fig. S4A). Additionally, paracrine stimulation with the AP–113A-HB-EGF mutant activated the EGFR in the same manner as AP–HB-EGF, suggesting that mutation of the HBD caused no gross changes in molecular conformation (see supplementary material Fig. S4B). The fraction of cell-surface HB-EGF at sites of cell-cell contact was quantified with fluorescence microscopy by measuring the area of acceptor-peptide-labeled HB-EGF that overlapped with N-cadherin immunostaining divided by the total HB-EGF area per cell. Treatment with heparin, heparinase III, or mutation of the HBD (AP–113A-HB-EGF–GFP) led to a reduction in the fraction of HB-EGF at sites of cell-cell contact from 0.8 to between 0.25 and 0.35 (Fig. 5E). These data suggest that binding of HB-EGF via the HBD to HSPGs on the cell surface is required for HB-EGF localization to sites of cell-cell contact.
HSPGs interact with pro-HB-EGF in trans
Demonstrating that HSPGs were required for HB-EGF localization to sites of cell-cell contact raised the question of the source of HSPGs for this interaction. HB-EGF could interact in cis with HSPGs on the same cell that expresses HB-EGF, holding it at sites of cell-cell contact. Alternatively, HB-EGF might interact with HSPGs in trans, and therefore HSPGs would be required on the neighboring cell for localization to sites of cell-cell contact. To distinguish between these two possibilities, CHO-K1 cells (wild type) and CHOpgsD-677 cells (Lidholt et al., 1992), which are heparan-sulfate deficient, were transfected with AP–HB-EGF–GFP (green, Fig. 6) or mCherry (red, Fig. 6) and co-cultured together in different combinations. The positive control (Fig. 6A) showed AP–HB-EGF–GFP at sites of cell-cell contact between mCherry-transfected and AP–HB-EGF–GFP-transfected wild-type CHO-K1 cells. Additionally, the negative control (Fig. 6D) showed no cell-cell-contact localization of AP–HB-EGF–GFP between mCherry-transfected and AP–HB-EGF–GFP-transfected CHOpgsD-677 cells. However, CHOpgsD-677 cells transfected with AP–HB-EGF–GFP showed localization of HB-EGF to the sites of cell-cell contact with a wild-type CHO-K1 mCherry-transfected neighbor (Fig. 6B). Wild-type CHO-K1 cells transfected with AP–HB-EGF–GFP showed no HB-EGF localization to sites of cell-cell contact with an mCherry-transfected CHOpgsD-677 neighbor (Fig. 6C). Additionally, the trans-bound AP–HB-EGF–GFP was dissociated from sites of cell-cell contact with the addition of heparin (100 μg/ml) for 15 minutes or the HBD peptide (100 μM) for 2 hours (Fig. 6E,F), resulting in a diffuse localization. Because CHO cells do not express cadherins (Niessen and Gumbiner, 2002), we were unable to study endogenous cell-cell junctions. These data demonstrate that the localization of pro-HB-EGF to sites of cell-cell contact is dependent on interaction with HSPGs on a neighboring cell only, and thus pro-HB-EGF interacts with HSPGs in trans.
Pro-HB-EGF interaction with HSPGs prevents ligand cleavage
Because heparin dramatically changed the localization of pro-HB-EGF from sites of cell-cell contact to a homogeneous distribution over the cell surface, we hypothesized that this localization change might increase access to proteases and affect ligand cleavage. To assess release of HB-EGF into the media, human placental alkaline phosphatase was inserted into the extracellular domain of AP–HB-EGF–GFP and AP–113A-HB-EGF–GFP near the N-terminus. The addition of heparin (100 μg/ml) increased alkaline-phosphatase activity in the media (Fig. 7A) of confluent monolayers of COS-7 cells transfected with wild-type HB-EGF (AlkPhos–AP–HB-EGF–GFP), suggesting that the heparin-induced localization change of pro-HB-EGF away from sites of cell-cell contact upregulates ligand cleavage. Treatment with the protease inhibitor batimastat (10 μM) inhibited heparin-induced cleavage of both wild-type and mutant HB-EGF. Interestingly, the HBD-mutant alkaline-phosphatase fusion (AlkPhos–AP–113A-HB-EGF–GFP) had higher levels of cleavage compared with wild-type HB-EGF and was unaffected further by the addition of heparin. Heparin increased the release of HB-EGF into the media in a dose-dependent manner, with concentrations above 1 μg/ml leading to maximum release after 2 hours of treatment (Fig. 7B). These data suggest that the trans interaction of pro-HB-EGF with HSPGs at sites of cell-cell contact prevents proteolytic release of the ligand. The interaction of HB-EGF with CD9, which also involves the HBD, might also serve to inhibit proteolytic release of the ligand, because we found a similar increase in alkaline-phosphatase activity in the medium for AlkPhos–AP–113A-HB-EGF–GFP when using the HSPG-lacking CHOpgsD-677 cells (see supplementary material Fig. S5). Because the CD9 interaction seems to operate in cis (Sakuma et al., 1997), and therefore ought not to depend on HB-EGF localization to sites of cell-cell contact, the two HBD interactions might work in series to provide a multi-layer control on ligand release. Despite the upregulation in AP–113A-HBEGF release, no detectable difference in EGFR phosphorylation at tyrosine 1148 was detected in cells transfected with AP–113A-HB-EGF–GFP, AP–HB-EGF–GFP or GFP (see supplementary material Fig. S4C). However, transfection with AP–HB-EGF–GFP led to growth inhibition, because [3H]thymidine incorporation was decreased 48% compared with a GFP-transfected control (Fig. 7C). Interestingly, mutation of the HBD of HB-EGF not only reversed the growth inhibition of HB-EGF transfection, but also led to cell proliferation, with a 42% increase in [3H]thymidine incorporation. Because HB-EGF juxtacrine signaling has been reported to be growth inhibitory (Iwamoto et al., 1999; Pan et al., 2002), we hypothesize that mutation of the HBD decreases the juxtacrine interaction by decreasing the concentration of pro-HB-EGF at sites of cell-cell contact. Additionally, because mutation of the HBD increased the rate of ligand cleavage from the cell surface, we hypothesize that an increase in autocrine signaling stimulates cell proliferation. These data would suggest that HSPGs might act as an important regulator in the balance between juxtacrine and autocrine HB-EGF, which can induce opposite cell fates of growth inhibition versus proliferation.
Heparin binding controls amphiregulin localization, but engineered heparin binding is insufficient for cell-cell-contact localization
HB-EGF is not the only ligand in the EGFR family capable of heparin binding, because amphiregulin, betacellulin and some isoforms of neuregulin also interact with HSPGs. HB-EGF and amphiregulin have similar HBDs located at the N-terminus of the protein before the EGF-like domain. These domains are both 21 amino acids in length, with over half of the residues represented by basic lysine or arginine, which allow the domain to interact with negatively charged heparin and heparan sulfate (Thompson et al., 1994). We sought to test whether heparin changed the localization of amphiregulin in the same manner as it does HB-EGF to determine whether HSPG-mediated localization was a common control mechanism for heparin-binding EGFR ligands. Acceptor-peptide labeling of the extracellular portion of amphiregulin, and a C-terminal GFP tag, showed that amphiregulin is similar to HB-EGF in that the extracellular and intracellular fluorophores were colocalized, suggesting that amphiregulin is primarily present in the pro-form (Fig. 8A). Additionally, amphiregulin was also concentrated around the perimeter of the cell at sites of cell-cell contact and the addition of heparin (100 μg/ml) for 4 hours led to a homogenous distribution of amphiregulin over the cell surface (Fig. 8B). Similarly, mutation of all lysine and arginine residues in the HBD of amphiregulin to alanine led to an identical distribution (R.N.P., unpublished), suggesting that the HBD of amphiregulin is also responsible for its localization to sites of cell-cell contact.
To test whether the HBD of HB-EGF was sufficient to localize any transmembrane protein to sites of cell-cell contact, we engineered an artificial protein consisting of an extracellular acceptor-peptide sequence followed by the portion of the HBD of HB-EGF that lies outside the EGF-like domain (residues 93-105), a 15-amino-acid flexible linker, cyan fluorescent protein (CFP), then the transmembrane domain (TM) of the PDGF receptor. This construct (AP-HBD-CFP-TM) (Fig. 8D) showed the same homogenous localization over the cell surface as a control construct (Fig. 8C) lacking an HBD (AP-CFP-TM). Therefore, the HBD alone was insufficient to localize any protein to sites of cell-cell contact. This suggests that an additional cofactor or specific structural feature of EGFR ligands is required for HB-EGF and amphiregulin localization to sites of cell-cell contact.
Discussion
HSPGs, which are present on the cell surface and in the extracellular matrix, are capable of binding many growth factors. Traditionally, this interaction has been proposed to restrain soluble, diffusible ligands, thus increasing their local concentration and ability to activate receptors (Schlessinger et al., 1995). Additionally, heparan-sulfate binding is known to modulate the activity of signaling molecules and protect them from proteolytic degradation (Conrad, 1998). Most ligands that have been reported to interact with HSPGs are soluble secreted factors, such as fibroblast growth factors (Gospodarowicz et al., 1984; Maciag et al., 1984; Shing et al., 1984), vascular endothelial growth factor (Ferrara and Henzel, 1989), hepatocyte growth factor (Nakamura et al., 1984; Zhou et al., 1999) and platelet-derived growth factor (Schilling et al., 1998). However, HSPGs also interact with some growth factors that remain anchored to the cell surface via a transmembrane domain, particularly those that belong to the EGFR-ligand family, including HB-EGF (Higashiyama et al., 1991), amphiregulin (Cook et al., 1991), betacellulin (Shing et al., 1993) and certain isoforms of neuregulin (Holmes et al., 1992; Loeb and Fischbach, 1995).
To extend our knowledge and understanding of the role of HSPGs on growth-factor regulation, we investigated their interactions with transmembrane pro-HB-EGF. One of our key findings was that a trans interaction between HSPG and the HB-EGF HBD is responsible for localizing pro-HB-EGF to sites of cell-cell contact (Figs 2, 3, 4, 5 and 6). HSPGs also modulated the localization of pro-amphiregulin in a similar manner (Fig. 8), suggesting that this might be a common mechanism for transmembrane heparin-binding ligands of the EGFR family. Because HB-EGF (Higashiyama et al., 1995), amphiregulin (Inui et al., 1997) and betacellulin (Tada et al., 1999) are heparin-binding and also capable of signaling in a juxtacrine mode, the role of this interaction could be to assist in sequestering prospective juxtacrine ligands at sites of cell-cell contact to facilitate receptor binding, probably in concert with CD9, to bind a receptor on a neighboring cell. This idea is supported by the observation that the HBD of HB-EGF and amphiregulin inhibits binding to the receptor except when in complex with heparin or heparan sulfate (Higashiyama et al., 1993; Johnson and Wong, 1994; Piepkorn et al., 1994; Takazaki et al., 2004), and that presence of an intact HB-EGF N-terminus prevents the ligand from activating its receptor during intracellular transport (Dong et al., 2005). Together, these data support the idea that HSPGs act as a permissive factor for juxtacrine signaling at sites of cell-cell contact.
Using wild-type and mutant CHO cells lacking cell-surface heparan sulfate, we demonstrated that the interaction of HSPGs with pro-HB-EGF occurs in trans (Fig. 6). The localization of HB-EGF to sites of cell-cell contact is unlikely to depend on interaction with EGFR, because CHO-K1 cells lack endogenous EGFR yet still show strong localization of HB-EGF to sites of cell-cell contact. This experiment also suggests that HSPGs are not required as an intracellular chaperone for pro-HB-EGF during transport, because cells lacking heparan sulfate were still able to localize HB-EGF to the cell surface. HSPGs have previously been shown to interact in trans with VEGFR-2 in VEGFR-mediated angiogenesis (Jakobsson et al., 2006) and with the Xenopus receptor caALK4 via the cofactor Vg1 during mesoderm migration in early left-right development (Kramer and Yost, 2002). Additionally, this interaction probably plays a role in blastocyst implantation during pregnancy, because the interaction between HB-EGF on the lumenal epithelium with EGFR and HSPGs on the adjacent blastocyst is required for successful attachment, which is reduced by exogenous heparin or blastocyst heparinase treatment (Farach et al., 1987; Farach et al., 1988; Raab et al., 1996).
A further key finding from our work here is that exogenous heparin and mutation of the HBD can upregulate HB-EGF proteolytic release in COS-7 cells, suggesting that association with HSPGs at sites of cell-cell contact protects pro-HB-EGF from proteolysis (Fig. 7A). However, this protection is not likely to be due to physical association of pro-HB-EGF with HSPGs, because soluble heparin increased proteolytic cleavage of the ligand. We speculate that the sequestration of pro-HB-EGF at sites of cell-cell contact reduces access to metalloproteinases, consistent with evidence that ectodomain cleavage is regulated at the substrate level (Herrlich et al., 2008). Mutation of the HBD not only reversed the growth inhibition observed with expression of pro-HB-EGF (Fig. 7C), but also stimulated cell proliferation. We hypothesize that the reversal of growth inhibition is due to a reduction in juxtacrine signaling, because less HB-EGF is present at sites of cell-cell contact when the HBD is not intact. Additionally, because the HBD mutant is cleaved at a higher rate, this probably increases autocrine HB-EGF signaling, stimulating cell growth. These data suggest that interaction with HSPGs plays an important role in the balance between juxtacrine and autocrine HB-EGF signaling and the resulting opposite cell fates of growth inhibition versus proliferation.
It is conceivable that heparin and heparan sulfate also operate in vivo to dissociate pro-HB-EGF from HSPGs, thus stimulating ligand cleavage. However, results reported here should be treated with some caution, because experiments were performed in transformed cells with overexpression of the ligand. In vivo, free heparin is secreted by mast cells upon degranulation, and both mast cells and HB-EGF signaling are implicated in the biological processes of wound healing (for a review, see Noli and Miolo, 2001) (Tokumaru et al., 2000), as well as angiogenesis (for a review, see Galinsky and Nechushtan, 2008) (Ongusaha et al., 2004) and the pathogenesis of atherosclerosis (for a review, see Kalesnikoff and Galli, 2008) (Nakata et al., 1996). Additionally, dermal mast cells themselves express HB-EGF mRNA (Artuc et al., 2002). Extracellular free heparan sulfate is generated by degradation of cell-surface HSPGs with heparanase, the expression of which is upregulated in all analyzed human cancers (Vlodavsky et al., 2007). It is possible that heparanase leads to a local concentration of free heparan sulfate that is high enough in the interstitial space to dissociate pro-HB-EGF from sites of cell-cell contact and stimulate cleavage of pro-HB-EGF. Fully understanding these complicated effects will probably require detailed mathematical modeling studies in the future along the lines analogously undertaken for the fibroblast-growth-factor system (Forsten-Williams et al., 2008).
Materials and Methods
Reagents
The following reagents were used: biotin (Sigma B4501), heparin (Sigma H3149), heparan sulfate (Sigma H7640), chondroitin sulfate (Sigma C4384), heparinase III (Sigma H8891), sodium chlorate (Sigma 244147), HBD peptide KKKKKGKGLGKKRDPCLRKYK (Neopeptide),
Cell culture
COS-7 cells were cultured in high-glucose Dulbecco's modified eagle medium (DMEM) with L-glutamine (Gibco 11965), supplemented with 10% fetal bovine serum (FBS) and 1% penicillin-streptomycin. CHO-K1 and CHOpgsD-677 cells (Lidholt et al., 1992) were cultured in Ham's F12 media with L-glutamine (BioWhittaker 12-615F), supplemented with 10% FBS and 1% penicillin-streptomycin. For microscopy experiments, cells were plated on 35-mm glass-bottom dishes (Mattek) coated with 0.1% gelatin (COS-7) or 1 μg/ml of fibronectin (CHO cells) for 1 hour at 37°C.
Plasmid constructs
The murine HB-EGF coding region was subcloned into pEGFP-N1 (Clontech) using the EcoRI and XhoI restriction sites from an adenoviral plasmid (Yoshioka et al., 2005). The acceptor peptide was inserted via site-directed mutagenesis (Geiser et al., 2001) with the primer 5′-GTGAAGTTGGGCGTGGCTAGCTCCCACCGAATTCTGCAGTCGACGGTACCGCGGGCC-3′ and its reverse complement. From here the following primers and their reverse complements were used to mutate the HBD: AP-delHBD-HBEGF-GFP with 5′-AAATCGAATGGCACGAAGGGGACCCATGCCTCAGGAAATA-3′, AP-97A-HBEGF-GFP with 5′-AAATCGAATGGCACGAAGGGGCGGCAGCCGCTGCGGGAAAGGGGTTAGGGAAGAAGA-3′, AP-105A-HBEGF-GFP with 5′-AAATCGAATGGCACGAAGGGGCGGCAGCCGCTGCGGGAGCAGGGTTAGGGGCGGCAGCCGACCCATGCCTCAGGAAATA-3′ and AP-105A-HBEGF-GFP was used as the base plasmids to make AP-113A-HBEGF-GFP with 5′-CAGCCGACCCATGCCTCGCAGCGTACGCAGACTACTGCATCCACGGGGA-3′. Human amphiregulin cDNA was subcloned into pEGFP-N1 and the acceptor peptide inserted after V107 with the primer 5′-TCAGTCAGAGTTGAACAGGTAGTTGGCCTGAACGACATCTTCGAAGCCCAGAAAATCGAATGGCACGAAAAGCCCCCCCAAAACAAG-3′ and its reverse complement. The HBD of HB-EGF (93-105) was inserted into AP-CFP-TM (Chen et al., 2005) between CFP and the AP sequence to make AP-HBD-CFP-TM with the primer 5′-AGTGGCACGAG GGCGCGCCGAAAAAGAAGAAGAAAGGAAAGGGGTTAGGGAAGAAGAGAGCGGGCGGCATGGTGAGCAAGGGCGAGGA-3′ and its reverse complement. Then, a flexible linker (SEGGGSEGGTSGATG) was added between CFP and AP to allow the HBD better access to HSPGs. This was done by PCR on AP-HBD-CFP-TM with the primer 5′-GAAGAAGAGAGCGGGCGGCTCTGAAGGCGGCGGCAGCGAAGGCGGCACCAGCGGCGCGACCGGAATGGTGAGCAAGGGCGAGGA-3′ and its reverse complement. Human placental alkaline phosphatase was amplified from a human HB-EGF alkaline-phosphatase fusion protein (Raab et al., 1996) with forward primer 5′-CCTGGCCACCCCAAGCAAAGAAAGGAATATCATCCCAGTTGAGGAGGAGAACCCGGACTTCTGGAACCGC-3′ and reverse primer 5′-TTTCTGGGCTTCGAAGATGTCGTTCAGGCCGTCGGTGGTGCCGGCGGGG-3′. The PCR product was gel purified and then used as the primer for a QuikChange insertion modified for large inserts on the base plasmid AP–HB-EGF–GFP and AP–113A-HB-EGF–GFP.
Purification of AP–HB-EGF
Three confluent 150-cm2 cell-culture dishes of COS-7 cells with 10 μM biotin in the media were transfected with AP–HB-EGF and BirA-ER or BirA-ER alone. After 24 hours, cell-culture media was replaced with serum-free media with 50 mM sodium chlorate and 10 μM biotin. After an additional 24 hours, the media was replaced with phosphate buffered saline (PBS) with sodium and magnesium, 50 mM sodium chlorate, 4 μM phorbol 12-myristate 13-acetate (Sigma P8139), 0.0003% H2O2 and 10 μM biotin. The following day, the PBS solution was collected after spinning out dead cells and incubated at 4°C overnight with 50 μl of heparin acrylic beads (Sigma H5263). After washing with PBS, the biotinylated AP–HB-EGF was eluted from the heparin beads with 50 μl of 2 M NaCl in PBS. The concentration of biotinylated AP–HB-EGF was estimated by western blotting with streptavidin-HRP in comparison with a standard of biotinylated acceptor-peptide-tagged maltose-binding protein (Avidity BIS-300).
Bioactivity of AP–HB-EGF
COS-7 cells were serum starved for 24 hours and stimulated for 1 minute with recombinant human HB-EGF (R&D Systems, 259-HE), heparin-bead-purified biotinylated AP–HBEGF or an equal volume of a control heparin-bead eluant. Cells were washed with PBS, then lysed with RIPA buffer [PBS with 1% NP-40, 0.5% sodium deoxycholate, 0.1% SDS, 1 mM sodium orthovanadate, 0.57 mM PMSF, protease inhibitor cocktail (Sigma P8340), and phosphatase inhibitor cocktail II (Sigma P5725)]. Lysates were subjected to SDS-PAGE and immunoblotted for total EGFR (C74B9) (Cell Signaling Technology, 2464) and phospho-EGFR Tyr1148 (Cell Signaling Technology, 4404) according to standard protocols. This experiment was repeated twice.
Biotinylation and cell-surface labeling of the acceptor peptide
Acceptor-peptide fusion constructs and a variant of BirA that was engineered to localize to the ER (BirA-ER) (Howarth and Ting, 2008) were co-transfected into COS-7 cells with Fugene6 or Mirus LTI Transfection reagent at equal molar ratios and cell-culture media was supplemented with 10 μM biotin. After 24 hours, cells were washed with PBS with calcium and magnesium and the acceptor peptide was labeled with mSA-AF568 or streptavidin-Cy5 (Invitrogen 43-8316) at 1 μg/ml in 5% dialyzed bovine serum albumin (BSA) in PBS for 10 minutes on ice. Cells were washed twice with PBS before imaging and imaged in PBS. Monovalent streptavidin–Alexa-Fluor-568 was produced as previously published (Howarth et al., 2006; Howarth and Ting, 2008). Each fluorescent labeling experiment was repeated three or more times, with 20 or more cells evaluated per experiment.
Immunostaining and fluorescence quantification
Cells were fixed with 2% paraformaldehyde for 10 minutes, blocked with 5% horse serum, incubated with anti-N-cadherin (H-63) antibody (Santa Cruz 7939) at 1:50, then anti-rabbit AF568 (Invitrogen A11011) at 1:500. The area in pixels for N-cadherin immunostaining and streptavidin-fluorophore-labeled extracellular HB-EGF was measured from fluorescence micrographs using thresholding with the ImageJ software package to define positive fluorescence. An N-cadherin mask was then applied to the HB-EGF images to quantify the number of pixels per cell that overlapped N-cadherin compared with the total number of HB-EGF-positive pixels.
Alkaline-phosphatase cleavage assay
COS-7 cells were plated on 96-well dishes (6500 cells per well) for 1 day, then transfected with AlkPhos–AP–HB-EGF–GFP or AlkPhos–AP–113A-HB-EGF–GFP. The following day, designated samples were pre-treated with batimastat (10 μM) in PBS with calcium and magnesium for 1 hour, then stimulated with a 100 μl solution of heparin in PBS supplemented with 1% BSA. Supernatants were collected at various time points, then washed for 1 minute with 100 μl of 1.5 M NaCl in PBS supplemented with 1% BSA to remove any soluble HB-EGF bound to HSPGs. The salt wash was combined with the supernatant and 40 μl was combined with 100 μl of p-nitrophenyl phosphate (Millipore ES009), incubated for 2 hours at 37°C, then optical density was read at 410 nm.
[3H]thymidine incorporation
COS-7 were plated at 25,000 cells per well in a 12-well dish (BD Falcon) for 24 hours, then transfected and serum starved. After 1 day, 1 μCi/ml of [3H]thymidine (Perkin Elmer NET027E001MC) was added for 3 hours, then the cells were washed with PBS and 5% tricholoroacetic acid, and lysed with 1 ml of 0.1 N NaOH + 0.1% SDS. After the addition of 4 ml of scintillation cocktail (Ecolume 88247005), samples were read on a Beckman Coulter LS6500 scintillation counter.
Microscopy
Phase-contrast and fluorescent images were obtained with a digital CCD camera (CoolSNAP HQ, Roper Scientific) and an inverted microscope (Olympus IX-70) with a 20× phase-contrast objective (Olympus LCPlanF NA 0.40) or 40× water-immersion objective (Olympus UApo/340 NA 1.15) for fluorescence. Confocal images were acquired at 60× with a Nikon TE2000-U inverted microscope.
Statistical analysis
A two-tailed, unpaired Student's t-test assuming unequal variance was utilized.
Acknowledgements
We wish to thank our funding sources, including NIBIB Grant EB003805, NCI Grant CA96504, MIT Poitras Predoctoral Fellowship and the National Science Foundation (NSF) Graduate Research Fellowship. Additionally, we would like to thank Lee Opresko, Rosalyn Adam, Leslie Mebane, Rachel Miller and Alan Grodzinsky for reagents. For helpful scientific discussion, we are grateful to Matthew Nugent. Deposited in PMC for release after 12 months.