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© The Rockefeller University Press,
0021-9525/2001//1087 $5.00
The Journal of Cell Biology, Volume 152, Number 5,
, 2001 1087-1098
Original Article |
Mammalian Sprouty-1 and -2 Are Membrane-Anchored Phosphoprotein Inhibitors of Growth Factor Signaling in Endothelial Cells
christofori{at}nt.imp.univie.ac.at
Growth factor–induced signaling by receptor tyrosine kinases (RTKs) plays a central role in embryonic development and in pathogenesis and, hence, is tightly controlled by several regulatory proteins. Recently, Sprouty, an inhibitor of Drosophila development-associated RTK signaling, has been discovered. Subsequently, four mammalian Sprouty homologues (Spry-1–4) have been identified. Here, we report the functional characterization of two of them, Spry-1 and -2, in endothelial cells. Overexpressed Spry-1 and -2 inhibit fibroblast growth factor– and vascular endothelial growth factor–induced proliferation and differentiation by repressing pathways leading to p42/44 mitogen-activating protein (MAP) kinase activation. In contrast, although epidermal growth factor–induced proliferation of endothelial cells was also inhibited by Spry-1 and -2, activation of p42/44 MAP kinase was not affected. Biochemical and immunofluorescence analysis of endogenous and overexpressed Spry-1 and -2 reveal that both Spry-1 and -2 are anchored to membranes by palmitoylation and associate with caveolin-1 in perinuclear and vesicular structures. They are phosphorylated on serine residues and, upon growth factor stimulation, a subset is recruited to the leading edge of the plasma membrane. The data indicate that mammalian Spry-1 and -2 are membrane-anchored proteins that negatively regulate angiogenesis-associated RTK signaling, possibly in a RTK-specific fashion.
Key Words: angiogenesis • endothelial cells • fibroblast growth factors • signal transduction • vascular endothelial growth factor
© 2001 The Rockefeller University Press
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Introduction |
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Since RTK signaling pathways appear to be highly conserved during evolution, it was conceivable that, in analogy to DSpry, a mammalian Spry may also regulate RTK signaling during mammalian development and pathogenesis. Recently, three human, four murine, and two avian genes have been identified that encode protein homologues of DSpry (Hacohen et al. 1998; de Maximy et al. 1999; Minowada et al. 1999; Tefft et al. 1999; Chambers and Mason 2000). Overexpression of mSpry (mouse Sprouty)-2 and -4 resulted in the repression of FGF-mediated limb development in chicken (Minowada et al. 1999), whereas ablation of Spry-2 expression in cultured embryonic mouse lungs lead to an increase in lung branching morphogenesis, a process that is thought to be induced by FGFs (Tefft et al. 1999). Moreover, similar to results obtained in Drosophila development (Hacohen et al. 1998), expression of mSprys and chicken Sprys is also upregulated by the FGF signaling pathway (Minowada et al. 1999; Chambers and Mason 2000), suggesting a feedback loop involved in the regulation of growth factor–mediated signal transduction. However, as in Drosophila, the mammalian Sprys' physiological role and, in particular, the mechanisms by which they inhibit RTK signaling are also not understood in any detail.
Similar to the tracheal system in Drosophila, during the development of the cardiovascular system, the formation of new blood vessels from preexisting ones (angiogenesis) also involves sprouting of endothelial cells out of an epithelial layer and branching of tubular structures (Flamme et al. 1997). In the adult, angiogenesis only takes place during the female reproductive cycle, wound healing, and in pathological situations, including tumor growth, diabetic retinopathy, arthritis, atherosclerosis, and psoriasis (Folkman 1995; Flamme et al. 1997; Risau 1997). Angiogenesis is tightly regulated by a balance between inducing and inhibitory signals (Hanahan and Folkman 1996; Hanahan 1997). Peptide growth factors, such as vascular EGF (VEGF), FGF, and angiopoietins, by binding to their cognate RTKs, positively regulate angiogenesis by inducing endothelial cell proliferation, migration, differentiation, and survival (Hanahan 1997; Gale and Yancopoulos 1999). In contrast, factors that negatively regulate angiogenesis by specifically blocking RTK signaling are less well characterized.
Motivated by the intriguing similarities in cell biological processes and gene function between Drosophila trachea development and mammalian angiogenesis, we have investigated the functional role of mammalian Sproutys in endothelial cells. Our results demonstrate that Spry-1 and -2 inhibit FGF- and VEGF-induced endothelial cell proliferation and differentiation, at least in part, by repressing pathways leading to p42/44 MAP kinase activation. Our data also demonstrate that Spry-1 and -2 are anchored to membranes by palmitoylation, posttranslationally modified by phosphorylation, and tightly associated with caveolin-1 in perinuclear and vesicular structures and in the plasma membrane. Moreover, their expression levels and their subcellular localization are modulated by growth factor stimulation. The results indicate that mammalian Sprys are membrane-anchored proteins that modulate RTK-mediated signal transduction in endothelial cells.
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GT11 (CLONTECH Laboratories, Inc.) following the manufacturer's recommendations. For all mSprys, the nucleotide sequence of both strands of the coding region was determined.
Adenovirus Vectors
The cDNAs encoding mSpry-1 and -2 were subcloned and integrated into recombinant E1/E3 defective adenoviruses using homologous recombination in Escherichia coli as described (Chartier et al. 1996). All genes of interest were under control of the cytomegalovirus immediate early promoter, followed by a rabbit β-globin intron/polyadenylation signal. Virus cultures were initiated by transfecting the linearized genomes into 293 cells using polyethylenimine (Baker et al. 1997). After amplification of the culture, virus was purified by banding twice on CsCl gradients, transferred into HBS/40% glycerol by passage over a gel filtration column, and stored at –80°C as previously described (Michou et al. 1999). Viral quantitation was based on protein content using the conversion of 1 mg viral protein/3.4 x 1012 virus particles.
Cell Culture
Human umbilical vein endothelial cells (HUVECs) and mouse microvascular endothelial cells (1G11) (Dong et al. 1997) were cultured in DME medium supplemented with 20% FCS (GIBCO BRL), 2 mM glutamine, 40 µg/ml bovine brain extract, 80 U/ml heparin, and antibiotics. The medium for bovine capillary endothelial cells (BCEs) was supplemented with 10% FCS and FGF2 (2.5 ng/ml). For viral infections, the culture medium was replaced with starvation medium (5% FCS for HUVECs, 2% FCS for BCEs, 0% for 1G11) containing 5,000 particles per cell (PPC). After 4 h, the medium was replaced with fresh growth medium.
DNA Synthesis Assay
Endothelial cells were plated in triplicate in 24-well dishes (30,000/well) and infected with adenoviruses (5,000 PPC) in reduced serum medium for 2–3 h. Cells were starved for 24 h in serum-free 1G11, 2% FCS medium (BCE), or 5% FCS medium (HUVEC), and then stimulated overnight with recombinant FGF2 (Promega) or VEGF (R&D Systems). After stimulation, 1 µCi of [3H]thymidine (Amersham Pharmacia Biotech) was added per well, and incorporation of thymidine was determined by scintillation counting as described (Shing et al. 1993).
Differentiation Assay
HUVECs were infected with 5,000 PPC of adenoviruses; after 4 d, they were resuspended in 5% FCS medium and plated in 24-well plates (40,000 cells/well) in the presence of growth factors on a thin layer of Matrigel (Becton Dickson) diluted 1:1 with 5% FCS medium.
Subcellular Fractionation
HUVECs (106) were infected with AdmSpry-1, or AdeGFP; and, after 48 h, the cells were extracted with 90 mM KAc, 2.5 mM MgCl2, 1 mM EDTA, 0.2 mM CaCl2, 12 mM glucose, 0.003% digitonin, 0.5 mM NaVO4, 10 mM NaF, 10 mM Pefabloc, 1 mM aprotinin, 1 mM leupeptin. After 7 min on ice, the supernatant (cytoplasmic extract) was collected, and the remaining cells were reextracted with Na2CO3 (pH 11). After 10 min on ice, the supernatant (peripheral membrane protein 1) was collected. The remaining cells were homogenized in PBS and centrifuged at 1,000 g to sediment nuclei and unbroken cells. Membranes in the postnuclear supernatant were pelleted at 100,000 g, and the supernatant was collected (peripheral membrane protein 2). The membrane pellet was extracted twice with Na2CO3 for 10 min on ice. Proteins in the aqueous phases (peripheral membrane proteins 3) were pooled with peripheral membrane protein fractions 1 and 2, precipitated as described (Oliferenko et al. 1999), and analyzed by SDS-PAGE and immunoblotting together with the proteins in the membrane pellet (integral membrane proteins).
Flotation Assay
Actively proliferating HUVECs infected with AdmSpry-1 or AdeGFP were washed twice with ice-cold PBS, removed from the plates by scraping in PBS, and centrifuged at 1,000 g at 4°C. Cells were lysed in 200 µl TN (25 mM Tris-HCl, pH 7.5, 150 mM NaCl, 1 mM DTT, protease inhibitors as above, 10% sucrose, and 1% Triton X-100) on ice and incubated for 30 min on ice. Samples were mixed with 400 µl ice-cold OptiprepTM, transferred into SW60 centrifuge tubes, and overlaid with each 600 µl of 35, 30, 25, 20, and 0% OptiprepTM in TN. The gradients were centrifuged at 35,000 rpm in a SW60 rotor for 12 h at 4°C. Fractions were collected from top to bottom of the centrifuge tubes, and proteins were precipitated and analyzed by immunoblotting.
Immunoblotting
Total cell lysates, protein fractions, or immunoprecipitates was analyzed by SDS-PAGE and immunoblotting as described (Yu and Sato 1999). Rabbit sera against mSpry-1 and -2 were generated with peptides corresponding to the NH2-terminal residues AVEGRQRLDYDRDTQ of mSpry-1 and HERLHGLPEHRQPPRLQPSQVHSSRAP of mSpry-2 conjugated to keyhole limpet hemocyanin. Antibodies from rabbit sera were affinity purified on antigenic peptides coupled to Sepharose. The specificity of the antibodies against mSpry-1 and -2 was further confirmed by peptide competition experiments, as well as by excluding cross-reactivity with mSpry-4. The following antibodies against other proteins were used: p42/44 MAP kinase and total p42/44 MAP kinase (Sigma-Aldrich), activated MAP kinase kinase (MEK) and total MEK (New England Biolabs, Inc.), β-catenin and caveolin-1 (Signal Transduction Laboratories), lactate dehydrogenase (LDH) (Chemicon International Ltd.), annexin II (Santa Cruz Biotechnology, Inc.), transferrin receptor (a gift from L. Huber, Research Institute of Molecular Pathology, Vienna, Austria).
Immunofluorescence
HUVECs were plated on gelatine-coated glass coverslips and grown to 70% confluency. For the stimulation experiments, the cells were starved for 24 h and then stimulated with 10 ng/ml FGF2 for various times. The cells were rinsed twice with PBS, fixed with 3% paraformaldehyde in PBS for 20 min at room temperature, permeabilized with 0.3% Triton X-100 for 3 min on ice, and washed with PBS. After blocking first with 3% BSA/PBS and then with 1% goat serum/0.1% BSA/PBS, the cells were incubated with the primary antibody for 30 min at room temperature and were washed with 0.1% BSA/PBS, followed by 30 min incubation with a secondary antibody conjugated to a fluorochrome. After washing with 0.05% Tween-20 in 0.1% BSA/PBS, the coverslips were mounted onto slides in mounting medium. Mouse monoclonal antibodies against caveolin-1, syntaxin-4, ergic-53, giantin, protein disulfide isomerase, transferrin receptor, and VE–cadherin were from Signal Transduction Laboratories; secondary antibodies anti–rabbit or anti–mouse IgG (Cy2 or Cy3 conjugated) were from Jackson ImmunoResearch Laboratories.
Immunoprecipitations
HUVECs infected with AdmSpry-1, AdmSpry-2, or AdeGFP were lysed in different extraction buffers (150 mM NaCl, 10 mM Tris, 10 mM NaF, 2 mM Na3VO4, 10 mM Pefabloc, 1 mM aprotinin, 1 mM leupeptin, 1 mM DTT, 1% Triton X-100 or 1% digitonin). After 30 min incubation (at room temperature for the samples in 1% digitonin and on ice for the samples in Triton X-100, lysates were cleared by centrifugation (14,000 g for 30 min), and equal amounts of lysates were immunoprecipitated with anti-Spry antibodies and protein G agarose at 4°C. The immunoprecipitates were washed three times at room temperature with the corresponding lysis buffers; immunoprecipitated proteins were resolved by 12% SDS-PAGE.
Radiolabeling
HUVECs infected with AdmSpry-1 or -2 were metabolically labeled with [35S]methionine/[35S]cysteine (Amersham Life Science) in methionine and cysteine serum-free medium for the time indicated, or with [3H]palmitate (30–60 Ci/mmol; DuPont) in DME containing 10% FCS for 2 h. For orthophosphate labeling, serum-starved HUVECs overexpressing mSpry-1 or mSpry-2 were labeled for 4 h in phosphate-free medium containing 5% FCS and 1 mCi/ml [32P]orthophosphate (Amersham Life Science) and then stimulated with FGF2 (10 ng/ml). Cells were then lysed, and mSpry-1 and -2 were immunoprecipitated with affinity-purified antibodies against mSpry-1 and -2, resolved by SDS-PAGE, and visualized by autoradiography and fluorography, respectively. For phosphoamino acid analysis, the proteins were transferred to polyvinyldifluoride membranes and hydrolyzed in 6 M HCl for 60 min at 110°C. The hydrolytic products were separated in the presence of phosphoserine, phosphothreonine, and phosphotyrosine markers in two dimensions on TLC plates (pH 1.9 and 3.5).
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mSpry-1 and -2 Inhibit MAP Kinase Activation
Previously, it has been reported that DSpry inhibits tyrosine kinase receptor signal transduction by inhibiting pathways that lead to the activation of p42/44 MAP kinase (Reich et al. 1999). The mitogenic function of the angiogenic factors FGF and VEGF also requires the activation of p42/44 MAP kinase (Marshall 1995; Yu and Sato 1999). Thus, we investigated whether overexpression of mSpry is able to affect p42/44 MAP kinase activity. HUVECs were infected with AdmSpry-1, AdmSpry-2, or AdeGFP, and, after serum starvation, the cells were stimulated with VEGF (50 ng/ml) for different times. Activation of MAP kinase was determined by immunoblotting with an antibody that specifically recognized the phosphorylated (activated) form of p42/44 MAP kinase (Fig. 3 A). Adenoviral expression of either mSpry-1 or -2 but not of eGFP resulted in a significant reduction in the levels of activated p42/44 MAP kinase, whereas the overall levels of p42/44 MAP kinase were unaffected, as determined by probing the immunoblot with an antibody that recognizes all forms of p42/44 MAP kinase (Fig. 3 A). Adenoviral expression of mSpry-1 and -2 was confirmed by probing the immunoblot with affinity-purified antibodies generated against mSpry-1 and -2 peptides (Fig. 3 A).
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Regulation of mSpry Expression by Angiogenic Factors
In Drosophila, DSpry not only interferes with growth factor–mediated signal transduction, but the expression of DSpry is also induced by the factors it subsequently inhibits. For example, DSpry expression is induced by FGF during trachea development (Hacohen et al. 1998) and EGF during oogenesis and eye development (Casci et al. 1999; Reich et al. 1999); in other regions, DSpry expression is induced with active EGF receptor signaling (Kramer et al. 1999). During chicken and mouse embryogenesis, Spry expression was found specifically in centers of FGF signaling or was upregulated in areas where recombinant FGF was applied to cultured embryos (Minowada et al. 1999; Chambers and Mason 2000). To assess whether Sprys are regulated in a similar way in endothelial cells upon stimulation with angiogenic factors, HUVECs (data not shown) and 1G11 cells (Fig. 4) were serum starved and then stimulated with FGF2 for different times. Levels of mRNAs for endogenous Spry-1 and -2 were determined by Northern blot hybridization (Fig. 4). Although Spry-1 mRNA was found at high levels in starved cells, it was transiently downregulated 2 h after treatment with FGF2 and regained high levels of expression 6 h after growth factor stimulation. Inhibition of protein synthesis by cycloheximide during growth factor stimulation prevented the transient degradation of Spry-1 mRNA (data not shown). In contrast, expression of Spry-2 (Fig. 4) and -4 (data not shown) was low in starved cells; it was induced 2 h after treatment with FGF2 and subsequently downregulated at later time points. The results indicate that the expression of Sprys is directly modulated by growth factor stimulation and that the various members of the Spry family may be affected in different ways.
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Caveolin-1 is a principal component of cell surface invaginatons called caveolae (Kurzchalia et al. 1992; Rothberg et al. 1992). Caveolae represent a subset of lipid rafts, cholesterol- and sphingolipid-rich membrane microdomains that are functionally implicated in cellular transport processes and in signal transduction–related events (Simons and Toomre 2000). The association of mSpry-1 with caveolin-1, thus, raised the question whether mSpry-1 was localized in lipid rafts. To test for this possibility, HUVECs were infected with AdmSpry-1 and AdeGFP, respectively, and cells were extracted with Triton X-100, a procedure that disrupts conventional membranes but does not affect detergent-resistant lipid rafts (Simons and Toomre 2000). Triton X-100 lysates were sedimented on Optiprep gradients, and the presence of mSpry-1 in the gradient fractions was analyzed by immunoblotting (Fig. 8 C). These experiments revealed that most of mSpry-1 and caveolin-1 sedimented as soluble proteins. Only a very small amount of mSpry-1 and caveolin-1 was found to float on top of the gradient, indicating that, in cultured endothelial cells, the vast majority of both caveolin-1 and mSpry-1 are not found in detergent-resistant rafts. This result is somewhat surprising since endothelial cells are known to contain abundant numbers of caveolae; however, our results are consistent with previous reports demonstrating that, in cultured endothelial cells, the majority of caveolin-1 is soluble in Triton X-100 (Venema et al. 1997).
Hence, consistent with the subcellular localization data (Fig. 6), the immunoprecipitation and the biochemical fractionation results indicate that, in cultured endothelial cells, Sprys tightly associate with membranes and with caveolin-1, but the majority of both Sprys and caveolin-1 are not part of detergent-resistant lipid rafts.
mSpry-1 and -2 Are Phosphorylated and Palmitoylated
The membrane association of Spry-1 and -2 and the apparent lack of membrane targeting motifs in their amino acid sequence, together with the observation that Sprys were found with varying electrophoretic mobilities (data not shown), suggested that Sprys are posttranslationally modified. To examine this, we performed a pulse–chase experiment to investigate the kinetics of mSpry-1 and -2 biosynthesis and processing. HUVECs were infected with AdmSpry-1 and metabolically labeled with [35S]methionine/cysteine for different times, and mSpry-1 was immunoprecipitated from protein lysates and analyzed by SDS-PAGE. At early time points, mSpry-1 was detected as a single band with the molecular mass predicted from its amino acid sequence (34 kD; Fig. 9 A, lane 1). With increasing time of labeling, a second band with lower electrophoretic mobility appeared that became predominant at later times (lanes 2–5). When the pulse experiments were followed by a chase with normal medium, a complete shift to the slower migrating form was observed (lane 6). Identical results were obtained for mSpry-2 (data not shown). These results raise the possibility that newly synthesized mSpry-1 and -2 undergo posttranslational modifications. The presence of tunicamycin in the culture medium or endoglycosidase treatment did not affect the electrophoretic mobility of mSpry-1 and -2, excluding protein glycosylation (data not shown). In contrast, alkaline phosphatase treatment of uninfected 1G11 cell lysates induced a shift of endogenous mSpry-1 to a faster migrating form, indicating that it was modified by phosphorylation (Fig. 9 B). Consistent with this notion, mSpry-1 and -2 were found to be labeled by the incorporation of [32P]orthophosphate in immunoprecipitation experiments (Fig. 9 C). However, when AdmSpry-1- or -2–infected HUVECs were starved and then stimulated with FGF2, incorporation of [32P]orthophosphate into mSpry-1 and -2 was not significantly changed with time (Fig. 9 C). Varying the experimental conditions, such as timing of the [32P]orthophosphate pulse and growth factor addition, also did not reveal a strong correlation between growth factor stimulation and mSpry phosphorylation, indicating that phosphorylation of mSprys was not directly affected by growth factor stimulation (data not shown). Phosphoamino acid analysis of [32P]orthophosphate-labeled and -immunoprecipitated mSpry-1 and -2 revealed that both mSpry-1 and -2 were phosphorylated exclusively on serine residues (Fig. 9 D).
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We also report for the first time the subcellular localization of endogenous Spry in mammalian cells. Consistent with the previously reported localization of Dspry to membranes (Casci et al. 1999), our studies demonstrate a tight association of Sprys with membranes. First, mSpry-1 and -2 and hSpry-1 and -2 significantly colocalize with caveolin-1 to the perinuclear region, vesicular structures, and the plasma membranes of endothelial cells. Second, the modification by palmitoylation and the lack of glycosylation suggest that Spry-1 and -2 are tightly associated with membranes by a lipid anchor. Third, immunoprecipitation experiments reveal a tight association between Spry-1, Spry-2, and caveolin-1, raising the possibility that Sprys are part of lipid rafts or caveloae (see below; Simons and Ikonen 1997; Simons and Toomre 2000).
Upon growth factor stimulation of starved endothelial cells, a significant subset of the proteins is translocated to the plasma membrane, predominantly to the lamellipodia at the leading edge of the cells, a site where the majority of growth factor receptors is known to localize. Consistent with the observations on DSpry reported by Casci and co-workers (1999), we were not able to detect Spry-1 or -2 in the supernatant or in the extracellular matrix of cultured cells, even when overexpressing the proteins (data not shown).
The specific subcellular localization of mammalian Sprys and the relocalization induced by growth factors provides some insights into the mechanisms by which Sprys inhibit RTK signaling. Several signaling factors, including EGF receptor, platelet-derived growth factor receptor, Src kinases, G
subunits, phospholipase C 
, protein kinaes C, Ras, Raf, and MAP kinases, have been shown to associate with lipid rafts or to cofractionate with caveolin-1 (Okamoto et al. 1998; Smart et al. 1999). Hence, lipid rafts and/or caveolae are thought to play an important role in signal transduction, possibly by assembling signaling complexes or by resetting or recycling receptors (Liu et al. 1997a,Liu et al. 1997b; Furuchi and Anderson 1998). Recently, Simons and Toomre 2000 proposed to distinguish four types of lipid rafts: native rafts that are only detectable in living cells, clustered rafts that are induced by cross-linking, detergent-resistant rafts that are characterized by, for example, their resistance to Triton X-100, and caveolae that are characterized by raft proteins, caveolins and lipids. Consistent with a previous report (Venema et al. 1997), our biochemical fractionation experiments with cultured endothelial cells have revealed that the majority of caveolin-1 and mSpry-1 is not found in detergent-resistant lipid rafts. Moreover, depletion of cholesterol from lipid rafts by treating HUVECs with methyl-β-dextrin did not affect the inhibitory function of overexpressed mSpry-1 on VEGF-induced MEK activation (data not shown), suggesting that functional Spry may not be part of lipid rafts. On the other hand, the small subset of mSpry-1 that, together with caveolin-1, is found in lipid rafts may represent functional Spry and may not be affected by methyl-β-dextrin because it is not exposed on the outer side of the plasma membrane, for example, within caveolae. Hence, it remains to be elucidated whether their association with caveolin-1 and/or their subcellular localization brings Sprys into contact with RTK signaling components to exert their inhibitory function.
DSpry has been shown to directly bind Gap-1 and the Grb-2 homologue Drk, both adaptor molecules of RTK signaling pathways (Casci et al. 1999). However, in endothelial cells, under the conditions used to identify caveo–lin-1 in a tight complex with Spry-1 and -2, these signaling adaptors did not coprecipitate with Sprys (data not shown). Hence, the molecular mechanisms by which Sprys negatively modulate RTK signaling remain to be elucidated. Based on the association of Sprys with caveolin-1 and the inability of Sprys to inhibit EGF-induced MAP kinase activation, it is tempting to speculate that Sprys may not simply interfere with the activation of the MAP kinase pathway. Rather, they may modulate the assembly of RTK signaling complexes, promote the resetting of RTK activity, or play a role in the regulation of RTK recycling. The latter functions would be compatible with the observation that in previously published reports (Chambers and Mason 2000; de Maximy et al. 1999; Minowada et al. 1999; Tefft et al. 1999) and, in our experiments, the inhibitory function of vertebrate Sprys is exclusively demonstrated by overexpression of the proteins. Hence, the function of endogenous Sprys may differ fundamentally from the effect of overexpressed Sprys. For example, Sprys, similar to or together with caveolin-1, may act as scaffolding proteins for the assembly of signaling complexes, and increasing Spry levels by overexpression may disturb the stoichiometry of complex assembly and prevent the formation of functional signaling complexes.
Consistent with previous reports on DSpry (Reich et al. 1999), mSpry, and chicken Spry (Minowada et al. 1999; Chambers and Mason 2000) during embryogenesis, mRNA levels of Spry-1 and -2 are also tightly regulated by growth factor stimulation in endothelial cells. Notably, expression of Spry-1 and the expression of Spry-2 appear to be inversely regulated. Although the expression of Spry-1 is repressed by growth factor stimulation, the expression of Spry-2 is upregulated. Both Sprys are phosphorylated on serine residues, however, phosphorylation does not appear to be modulated by growth factor stimulation, and the functional role of this modification remains to be elucidated. For example, it is not known whether Spry-1 and -2 phosphorylation is required for their recruitment to the plasma membrane or for their inhibitory function. Thus, identification of the Spry phosphorylation sites and/or the kinase(s) that phosphorylate Sprys may shed some light on Sprys' mode of action. Moreover, the observation that Sprys are palmitoylated membrane proteins and associate with caveolin-1 sets the stage for future experiments aimed at unraveling Sprys' physiological functions.
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This work was supported in part by the Austrian Industrial Research Promotion Fund. M.-A. Impagnatiello was supported by a Marie-Curie Training Mobility Research fellowship (FMBICT983206).
Note added in proof. An inhibitory function in angiogenesis of murine Sprouty-4 has been reported recently by Lee and coworkers (Lee, S.H., D.J. Schloss, L. Jarvis, M.A. Krasnow, and J.L. Swain. 2001. J. Biol. Chem. 276:4128–4133).
Submitted: 25 July 2000
Revised: 6 November 2000
Accepted: 17 January 2001
Abbreviations used in this paper: BCE, bovine capillary endothelial cell; DSpry, Drosophila Sprouty; EGF, epidermal growth factor; FGF, fibroblast growth factor; hSpry, human Sprouty; HUVEC, human umbilical vein endothelial cell; LDH, lactate dehydrogenase; MAP, mitogen-activating protein; MEK, MAP kinase kinase; mSpry, mouse Sprouty; PPC, particles per cell; RTK, receptor tyrosine kinase; VEGF, vascular EGF.
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