The Cell Adhesion Domain in Plasma Vitronectin Is Cryptic*

(Received for publication, January 9, 1997, and in revised form, March 10, 1997)

Dietmar Seiffert Dagger § and Jeffrey W. Smith par

From the Dagger  Department of Vascular Biology, The Scripps Research Institute, La Jolla, California 92037 and  The Burnham Institute, La Jolla, California 92037

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
REFERENCES


ABSTRACT

Vitronectin (Vn) is a major adhesive glycoprotein in blood. However, many of the functions of Vn are regulated by its conformational state and degree of multimerization. Here, the ability of native and denatured Vn to bind to integrin adhesion receptors was compared. Three lines of evidence suggest that the native, plasma form of Vn is not an adhesive glycoprotein. (i) Antibodies that bind in close proximity to the cell adhesion domain of Vn fail to bind to native Vn present in unfractionated plasma. (ii) Denatured Vn binds to both glycoprotein IIb/IIIa and alpha vbeta 3 in a dose-dependent manner. In contrast, native Vn is unable to bind either integrin. (iii) Thermal denaturation of native Vn, or its complexation with type 1 plasminogen activator inhibitor, exposed the cell adhesion domain of Vn. Thus, while plasma Vn is unable to bind integrins and is not an adhesive glycoprotein, the conformationally altered from of the protein binds avidly to both alpha vbeta 3 and glycoprotein IIb/IIIa. The data presented here indicate that such conformational changes in Vn are likely to occur in areas of tissue injury and thrombosis.


INTRODUCTION

Vitronectin (Vn),1 an adhesive glycoprotein present in blood and in a variety of tissues, belongs to a group of molecules that contain the RGD cell adhesion sequence and play key roles in the attachment of cells to their surrounding matrix (1, 2). In addition, Vn has several other functions in the complement, coagulation, and fibrinolytic system. For example, Vn is identical to the S protein of the complement system and thus inhibits complement-mediated cell lysis (3, 4). Vn competes with heparin binding to antithrombin III, thereby preventing the rapid inactivation of thrombin and factor Xa by this protease inhibitor (5, 6). Vn also binds to and stabilizes the biological activity of type 1 plasminogen activator inhibitor (PAI-1), the physiological inhibitor of both tissue- and urinary-type plasminogen activators (7, 8). Thus, Vn provides unique regulatory links between cell adhesion and proteolytic enzyme cascades, although it is not clear how the multiple functions of Vn are coordinately regulated.

Vn is a conformationally labile molecule, and this lability is likely to play a large role in regulating the functions of the protein. This notion is based on the observation that different preparations of Vn exhibit differing abilities to bind to the glycosaminoglycan heparin. Only 2% of the Vn in plasma is capable of binding to heparin-Sepharose, whereas this fraction is increased to 7% by the generation of serum (9). In addition, the formation of complexes of Vn with PAI-1 (10), thrombin-antithrombin III (11), or complement C5b-C9 (12) induces conformational changes in the molecule, which expose the heparin binding domain. Moreover, conformational changes are also induced by denaturation with chaotropic agents, heat-treatment and acidification. These changes are accompanied by the spontaneous formation of disulfide-linked multimers of Vn. Using a panel of conformationally sensitive antibodies, we provided evidence that conformational changes within Vn are not limited to the heparin binding domain, but also occur in the N-terminal half of the molecule, including the N-terminal somatomedin B (SMB) domain (13), a site that encompasses the RGD sequence.

Understanding the interrelationship between the binding domains of Vn has been complicate, because the exposure and function of these sites depends on the conformational state of this molecule. For example, a number of ligands interact preferentially with the conformationally altered and multimeric (i.e. denatured form) of Vn. These include collagen (14), glycosaminoglycans (15, 16), beta -endorphin (17), PAI-1 (18), and urokinase receptor-urokinase complex (19, 20). In contrast, thrombin-antithrombin III complexes appear to preferentially interact with native, plasma Vn (21). The function of native and denatured Vn in promoting cell adhesion is even more complicated. Native Vn was reported to bind specifically and saturably to glycoprotein (GP) IIb/IIIa on stimulated platelets (22-24). The binding of denatured Vn to platelets are conflicting (25). In addition, Vn has been reported to both block (26) and stimulate (23) platelet aggregation. The reasons for these discrepancies remain unclear.

Vn is one of many adhesive proteins that bind to cell surface receptors called integrins (27, 28). Each integrin is a noncovalently associated alpha beta heterodimer that spans the plasma membrane. To date, nine integrin alpha  subunits and 12 beta  subunits have been identified. Since the ligand binding specificity of each receptor is conferred by its subunit composition, functional diversity within the family of integrins is achieved by heterologous pairing between subunits. Three different integrins have been identified as receptors for Vn, GPIIb/IIIa (also known as alpha IIbeta 3 (29)), alpha vbeta 3, expressed by endothelial cells and implicated in angiogenesis (30), and alpha vbeta 5 (31). Vn contains a single RGD sequence located adjacent to the SMB domain (3, 4). Site-directed mutagenesis of the RGD motif shows that this sequence is required for cell adhesion and can not be compensated for by other parts of the molecule (32, 33). A number of reports indicated that the cell adhesion domain is exposed on both native and denatured Vn (1, 34). Consequently, the adhesive capacity of the protein is not thought to be regulated by the conformational lability of the molecule. However, this concept is challenged by two observations. First, only denatured Vn induces tyrosine phosphorylation in endothelial cells by binding to the alpha vbeta 3 integrin on the cell (35). Second, alpha vbeta 5-dependent endocytosis of Vn by skin fibroblasts was only observed using denatured Vn, the native form of Vn is not internalized (36, 37).

In the present report, we compare the binding of native and denatured Vn to purified GPIIb/IIIa and alpha vbeta 3. Evidence is provided that native Vn is incapable of binding to integrin adhesion receptors and that its RGD sequence is not exposed. Conformational changes in Vn, induced by chemical or thermal denaturation, or by complexation with PAI-1, expose the integrin binding site on Vn, allowing it to bind tightly to both alpha vbeta 3 and GPIIb/IIIa.


MATERIALS AND METHODS

Proteins and Antibodies

Denatured Vn was purified by heparin affinity chromatography in the presence of 8 M urea (38). Vn was also isolated under nondenaturing conditions (i.e. native Vn) according to published procedures (39). Protein concentrations were determined by the bicinchoninic acid method (Pierce). The final Vn preparations were devoid of fibrinogen and fibronectin immunoreactivity as judged by immunoblotting using rabbit anti-human fibrinogen or fibronectin (Calbiochem). Denatured Vn was biotinylated using NHS-LC-biotin (Pierce). Briefly, 1.5 mg of Vn was dissolved in 50 mM sodium phosphate buffer, pH 8.5, at 20 µM and incubated with 3 mg of biotinylation reagent dissolved in 100 µl of Me2SO for 3 h at 37 °C, followed by extensive dialysis against phosphate-buffered saline (PBS). GPIIb/IIIa was obtained from Enzyme Research Laboratories, and alpha vbeta 3 was isolated from human placenta extracts by affinity chromatography (40). Human fibrinogen was obtained from Calbiochem. PAI-1 was purified as described (41), activated with 4 M guanidinium hydrochloride (42), dialyzed against 5 mM sodium phosphate, 1 mM EDTA, 0.345 M NaCl, pH 6.5, to stabilize the biological activity of PAI-1 (43), and the specific activity was determined by titration against urinary-type plasminogen activator (Calbiochem). Prior to each experiment, PAI-1 was dialyzed into ice-cold PBS. Latent PAI-1 was prepared by incubation of activated PAI-1 at 37 °C for 24 h. After this incubation step, the structural integrity of the resulting PAI-1 preparation was confirmed by SDS-polyacrylamide gel electrophoresis followed by staining with silver nitrate. The remaining PAI-1 activity after this incubation was determined by binding to immobilized tissue-type plasminogen activator (Calbiochem) (44) and was less than 0.5% of the starting material (not shown). Monoclonal antibodies (mAbs) 611, 153, and 1244 were obtained by standard hybridoma techniques using denatured Vn as immunogen (41). IgG was produced in mice as ascites fluid and purified by using protein A-Sepharose. The generation of rabbit anti-human Vn was described previously (41). Biotin-labeled secondary antibodies, streptavidin alkaline phosphatase, and substrate were from Zymed. Conformational changes in the Vn molecule were quantified by competitive enzyme-linked immunosorbent assay (13). Briefly, microtiter wells were coated with denatured Vn (1 µg/ml in PBS, 4 °C, 16 h), and nonspecific binding sites on the plastic dishes were blocked by incubating the washed wells for 1 h at 37 °C in PBS containing 3% casein and 0.05% Tween 20. The wells were co-incubated for 1 h with a constant amount of IgG (50 ng/ml final concentration) and the indicated concentration of Vn in PBS containing 0.1% casein and 0.1% Tween 20. Bound IgG was detected with biotin-conjugated goat anti-mouse IgG, followed by streptavidin alkaline phosphatase conjugate and the chromogenic substrate p-nitrophenyl phosphate (Zymed). The change of absorbance at 405 nm of duplicate wells was determined and the absorbance of wells not incubated with antibodies but otherwise treated identically was subtracted.

Effect of mAbs to Vn on Cell Adhesion

The human fibrosarcoma cell line HT 1080 was obtained from ATCC and maintained in Dulbecco's modified Eagles's medium/F-12 medium containing 10% fetal bovine serum as described (45). Semiconfluent cultures were labeled for 16 h with [35S]methionine (Amersham Corp; 100 µCi/ml in 80% methionine-deficient medium, 20% complete growth medium). After washing with PBS, the cells were detached by treatment with PBS containing 0.2 mM EDTA for 5 min and washed three times in adhesion buffer (1 × Hanks' balanced salt solution, 50 mM Hepes, 1 mg/ml bovine serum albumin, 1 mM CaCl2, 1 mM MgCl2, 1 mM MnCl2, pH 7.4) and resuspended at 2 × 105 cells/ml in adhesion buffer. Flat-bottomed microtiter wells were coated with 100 ng/well denatured Vn. Following an 18-h coating period at 4 °C, the plates were blocked with PBS containing 10 mg/ml bovine serum albumin. Antibodies (50 µl) were prebound to the wells at 37 °C for 1 h. Cells (1 × 104) were added to the antibody containing wells in triplicate and allow to adhere for 1 h. The wells were washed gentle three times in PBS to remove nonadherent cells, and the bound cells were solubilized in 1% SDS and quantified by beta -counting. The radioactivity associated with bovine serum albumin coated wells was subtracted from that of the Vn-coated wells. Results are expressed as percentage cell binding in the absence of antibodies.

Protein Binding Analysis

The binding of purified Vn preparations to immobilized integrins was analyzed with the methods essential as described previously (46). Briefly, integrins were immobilized at 50 ng/well (alpha vbeta 3) or 250 ng/well (GPIIb/IIIa) for 18 h at 4 °C. Subsequently, nonspecific protein binding sites on the plates were blocked with 50 mM Tris, pH 7.4, containing 150 mM NaCl, 1 mM MgCl2, 1 mM CaCl2, 1 mM MnCl2 (binding buffer), and 35 mg/ml bovine serum albumin. After washing with binding buffer, unlabeled Vn was added for 1 h at 37 °C in binding buffer containing 0.1% bovine serum albumin. Bound Vn was detected using rabbit anti-human Vn IgG (10 µg/ml), followed by biotin-labeled anti-rabbit IgG, streptavidin alkaline phosphatase, and substrate. The change of absorbance (405 nm) of duplicate wells was determined. Specific binding was determined by subtracting the binding to wells incubated with the same concentration of Vn in the presence of 10 mM EDTA. For competitive ligand binding studies, biotin-labeled denatured Vn (1 µg/ml; a concentration required to obtain half- maximal binding) was co-incubated (3 h, 37 °C) with unlabeled native Vn, denatured Vn, or fibrinogen on integrin-coated plates (see above). After washing, bound Vn was detected using streptavidin alkaline phosphatase and substrate. Specific binding was determined by subtracting the binding of biotin-labeled wells incubated in the presence of 10 mM EDTA from that incubated in the presence of divalent cations. Results are expressed as percentage binding in the absence of soluble competitor.


RESULTS

Characterization of mAbs That Block Cell Adhesion to Vn

The effects of three different anti-Vn mAbs on cell adhesion to immobilized Vn were determined (Fig. 1A). Microtiter wells were coated with denatured Vn and incubated with the indicated concentration of antibody and metabolically labeled HT 1080 cells. Cells were allowed to attach for 1 h. Bound cells were quantified by beta -counting. mAb 153 and 611 inhibited cell adhesion to Vn in a dose-dependent manner, whereas mAb 1244 was significantly (approximately 20-fold) less effective. The observed difference was apparently not due to a lower affinity of mAb 1244 for denatured Vn, since this antibody and clone 153 differ in the affinity for denatured Vn only by factor 2 (41). In contrast, no inhibition was observed using normal mouse IgG (data not shown). The mAbs 153 and 611 bind to Vn polypeptides encompassing amino acids 1-51, a fragment of Vn containing the RGD sequence, whereas the control antibody interacts with amino acids 52-239 (41) (data not shown).


Fig. 1. Characterization of mAbs that block cell adhesion to vitronectin. A, effect of mAbs to Vn on HT 1080 cell adhesion. Microtiter wells coated with denatured Vn were preincubated with the indicated concentration of mAb 153 (open circles), mAb 611 (closed circles), or mAb 1244 (closed squares), followed by the addition of 35S-labeled HT 1080 cells for 1 h. After gentle washing, bound cells were quantified by beta -counting. Results are expressed as percentage of cells specifically bound (see "Materials and Methods"). B, expression of conformationally sensitive epitopes in Vn. The indicated concentration of denatured Vn (squares), native Vn (triangles), or unfractionated platelet-poor plasma (circles) were incubated with a constant concentration of anti-Vn IgG (closed symbols, mAb 153; open symbols, mAb 611) in microtiter wells coated with denatured Vn. The wells were washed, and bound antibodies were detected (see "Materials and Methods"). Results are expressed as percentage binding of antibodies in the absence of soluble competitor.
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We previously provided evidence that an immunoepitope (mAb 153) located in the SMB domain of Vn (amino acids 1-51) is cryptic in plasma Vn (13). Experiments were performed to understand whether lack of reactivity with native plasma Vn is a general feature of antibodies derived to this region of the Vn molecule. Competitive enzyme-linked immunosorbent assays were employed to determine the reactivity of mAB 611 with purified preparations of native and denatured Vn and Vn present in unfractionated plasma (Fig. 1B). Results were compared with mAb 153. Microtiter wells coated with denatured Vn were incubated with a constant amount of anti-Vn IgG and increasing concentrations of different types of Vn (Fig. 1B). Denatured Vn competes with the binding of both antibodies to immobilized denatured Vn in a dose-dependent manner, whereas neither antibody reacted well with Vn present in unfractionated plasma. The reactivity with purified native Vn with these two conformationally sensitive antibodies was at least 50-fold lower than that of denatured Vn.

Binding of Native and Denatured Vn to GPIIb/IIIa and alpha vbeta 3

Based on the strong reactivity of the inhibitory antibodies with denatured Vn, and the inability of these antibodies to bind native Vn, we hypothesized that the RGD sequence in native Vn is cryptic. This hypothesis was tested by measuring the binding of native and denatured Vn to purified integrins (Figs. 2 and 3). To measure binding, microtiter wells were coated with purified integrin and then incubated with a range of either native or denatured Vn. Bound Vn was detected with an polyclonal antibody against Vn. Denatured Vn bound to GPIIb/IIIa in a dose-dependent manner and approached saturation at 5 µg/ml. Specific binding did not further increase using 10 µg/ml denatured Vn. In the concentration range presented in Fig. 2A, specific binding was more than 85% of total binding. In contrast, little binding of native Vn was observed under the same conditions.


Fig. 2. Binding of native and denatured Vn to GPIIb/IIIa. A, direct binding of Vn to GPIIb/IIIa. Microtiter wells were coated with purified GPIIb/IIIa and incubated with the indicated concentration of either denatured (closed circles) or native (open circles) Vn. Bound Vn was detected with rabbit anti-human Vn, followed by biotin anti-rabbit IgG, streptavidin alkaline phosphatase, and substrate. Results are expressed as mOD/min (change of absorbance at 405 nm). B, competition of Vn for binding of biotin Vn to GPIIb/IIIa. A constant concentration of biotin-labeled denatured Vn was incubated on GPIIb/IIIa- coated microtiter wells in the presence of the indicated concentration of native (open circles), denatured (closed circles) Vn, or fibrinogen (closed squares). Bound labeled Vn was detected using streptavidin alkaline phosphatase and substrate. Results are expressed as percentage binding in the absence of unlabeled competitor.
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Fig. 3. Binding of native and denatured Vn to alpha vbeta 3. A, direct binding of Vn to alpha vbeta 3. Microtiter wells were coated with purified alpha vbeta 3 and incubated with the indicated concentration of either denatured (closed circles) or native (open circles) Vn. Bound Vn was detected with rabbit anti-human Vn, followed by biotin anti-rabbit IgG, streptavidin alkaline phosphatase, and substrate. Results are expressed as mOD/min (change of absorbance at 405 nm). B, competition of Vn for binding of biotin-labeled Vn to alpha vbeta 3. A constant concentration of biotin-labeled denatured Vn was incubated on alpha vbeta 3 coated microtiter wells in the presence of the indicated concentration of native (open circles), denatured (closed circles) Vn, or fibrinogen (closed squares). Bound labeled Vn was detected using streptavidin alkaline phosphatase and substrate. Results are expressed as percentage binding in the absence of unlabeled competitor.
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To exclude the possibility that the lack of binding of native Vn to GPIIb/IIIa was due to reduced reactivity of the rabbit anti-Vn IgG with native Vn, competitive binding assays were employed to confirm the results of the direct binding studies (Fig. 2B). In this assay, immobilized GPIIb/IIIa was co-incubated with a constant amount of biotinylated denatured Vn and a range of competing native or denatured Vn. Fibrinogen was also used as a competitor, because it is the physiological ligand for GPIIb/IIIa. Fibrinogen was 10-50-fold more efficient in competing with the binding of labeled Vn for GPIIb/IIIa than denatured Vn. More importantly, no competition was observed using native Vn, confirming the inability of the native form of Vn to bind to GPIIb/IIIa.

GPIIb/IIIa is only one of several integrins that are reported to bind Vn. The alpha vbeta 3 integrin is also considered a receptor for Vn and was originally named the "vitronectin receptor." To determine whether the alpha vbeta 3 integrin also exhibited preferential binding to the denatured form of Vn, similar binding studies were performed using immobilized alpha vbeta 3 (Fig. 3A). Denatured Vn bound to alpha vbeta 3 in a dose-dependent manner and again approached saturation at 5 µg/ml Vn. In contrast, native Vn showed little binding. Again, results were confirmed in competitive binding studies and compared with fibrinogen. Native Vn failed to compete with the binding of denatured Vn for binding to alpha vbeta 3. Both denatured Vn and fibrinogen competed for the binding of biotinylated Vn to alpha vbeta 3. Little difference was observed in the extent of competition between the latter two ligands.

Denaturation of Native Vn Exposes the RGD Sequence

Only about 7% of the total Vn present in plasma is recovered using a purification procedure that maintains the protein in its native conformation (39). This raised the possibility that a nonintegrin-binding subpopulation of native Vn could have been purified and employed in the binding studies. To address this issue, a heat denaturation procedure was employed to convert native Vn into conformationally altered, multimeric Vn (Fig. 4). Heat treatment of native Vn resulted in the exposure of the mAb 611 epitope (Fig. 4A) and mAb 153 epitope (not shown) to a similar extent as in denatured Vn. In addition, the electrophoretic mobility of heat-treated native Vn on native polyacrylamide gel electrophoresis was indistinguishable from denatured Vn (i.e. heat treatment resulted in the formation of high molecular weight multimers that failed to enter the separating gel) (not shown). The interaction of heat-treated native Vn with alpha vbeta 3 was compared with that of purified denatured Vn (Fig. 4B). Heat-treated Vn binds to immobilized alpha vbeta 3 in a dose-dependent manner similar to denatured Vn (Fig. 4B). In addition, heat-treated native Vn competes with labeled denatured Vn for binding to this integrin to an extent comparable with that of denatured Vn (Fig. 4C). Similar results were obtained when binding to GPIIb/IIIa was examined (not shown). In addition, an alternative denaturation procedure (i.e. treatment of native Vn with 8 M urea) also induced integrin binding (not shown). These observations indicate that denaturation of native Vn results in the exposure of the cryptic cell binding domain and that the inability of native Vn to bind to alpha vbeta 3 or GPIIb/IIIa was not due to the purification of a nonintegrin-binding subpopulation of Vn from plasma.


Fig. 4. Effects of thermal denaturation of Vn on mAb epitope expression and binding to alpha vbeta 3. A, heat-treatment induces the mAb 611 epitope. The mAb epitope expression was determined in competitive enzyme-linked immunosorbent assays (see Fig. 1B) using purified native Vn (open circles), heat-treated native Vn (55 °C, 1 h; closed squares), and compared with denatured Vn (closed circles). Results are expressed as percentage binding of control wells in the absence of soluble competitor. B and C, heat-treatment of native Vn induces the binding to alpha vbeta 3. Native Vn was heat-treated as in A. In B, the binding of unlabeled Vn forms to alpha vbeta 3 was determined as in Fig. 3A. Results are expressed as mOD/min (change of absorbance at 405 nm). In C, the competition of unlabeled Vn conformers for the binding of biotinylated denatured Vn to alpha vbeta 3 was determined as in Fig. 3B. Results are expressed as percentage binding in the absence of soluble competitor. The designation of the symbols in B and C is as in A.
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Effects of PAI-1 on the Adhesive Functions of Native and Denatured Vn

Vn binds to a number of plasma proteins, and these interactions alter the conformation of this molecule (10-12). Experiments were performed to test whether physiological ligands of native Vn can induce the exposure of the cell adhesion domain. The binding of native Vn to active PAI-1 results in the formation of Vn multimers that express epitopes for conformationally sensitive antibodies like mAbs 153 (10) and 611 (data not shown). Interestingly, PAI-1·Vn complexes are relatively labile and PAI-1 readily dissociates from Vn, but Vn remains multimeric and conformationally altered (10). We reasoned that the binding of PAI-1 to native Vn is likely to expose the integrin binding site on Vn. Native Vn was incubated with a 2-fold molar excess of active PAI-1 for 16 h at 37 °C. After this incubation period, more than 99% of the PAI-1 was converted into the latent conformation as based by binding to immobilized tissue-type plasminogen activator (not shown). Little competition of native Vn (Fig. 5A, left closed bar) for mAB 153 binding to immobilized denatured Vn was observed. Incubation of native Vn with active PAI-1 (Fig. 5A, left open bar) resulted in the exposure of the conformationally sensitive mAb 153 epitope. In contrast, no effects of latent PAI-1 on the exposure of this epitope was observed (Fig. 5A, left hatched bar). The mAb 153 does not detect Vn in complex with PAI-1 (41), confirming that the majority of the Vn was present in an uncomplexed, conformationally altered form. In parallel experiments, the effects of pretreatment of native Vn with PAI-1 on its ability to bind to alpha vbeta 3 (Fig. 5A, right bars) was analyzed. Again, while little binding of native Vn (Fig. 5A, right closed bar) to alpha vbeta 3 was observed, PAI-1 induced Vn multimers (A, right open bar) demonstrated increased binding to alpha vbeta 3. In contrast, latent PAI-1 (Fig. 5A, right hatched bar) had failed to induce alpha vbeta 3 binding of native Vn.


Fig. 5. Modulation of the adhesive functions of Vn by PAI-1. A, PAI-1 induces the exposure of conformationally sensitive epitopes and alpha vbeta 3 binding site in native Vn. Native Vn (20 µg/ml; closed bars) was incubated with active PAI-1 (40 µg/ml; open bars) or latent PAI-1 (40 µg/ml; hatched bars) for 16 h at 37 °C and tested for the exposure of the conformationally sensitive mAb 153 epitope as in Fig. 1 or for binding to immobilized alpha vbeta 3 as in Fig. 3 (10 µg/ml final concentration of Vn). Results are expressed as percentage inhibition (mAb 153) or binding (alpha vbeta 3) in comparison with denatured Vn (10 µg/ml). Identical results were obtained in three independent experiments with a standard error of less than 10%. B, effects of PAI-1 on the binding of denatured Vn to alpha vbeta 3. Increasing concentrations of active (closed circles) or latent (open circles) PAI-1 were co-incubated with denatured Vn (500 ng/ml) on alpha vbeta 3-coated plates. Bound Vn was detected with rabbit anti-human Vn IgG, followed by biotin-labeled anti-rabbit IgG, streptavidin alkaline phosphatase, and substrate, Results are expressed as percentage binding in the absence of PAI-1. Closed squares, alpha vbeta 3-coated wells were preincubated with denatured Vn (500 ng/ml), washed, and then incubated with the indicated concentration of active PAI-1 for 1 h at 37 °C. Bound Vn was detected as above.
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The PAI-1 and integrin binding sites in denatured Vn are structurally distinct but located in close proximity, raising the possibility that PAI-1 may modulate the adhesive functions of denatured Vn. To test this hypothesis, microtiter wells were co-incubated with a constant amount of denatured Vn (which binds to alpha vbeta 3) and increasing concentrations of either active or latent PAI-1 in this binding assay (Fig. 5B). Active PAI-1 blocked the binding of denatured Vn to immobilized alpha vbeta 3 in a dose-dependent manner. At the highest concentration of PAI-1, approximately 80% inhibition was observed. The competition reached a plateau at a 10-fold molar excess of active PAI-1 over denatured Vn. In contrast, latent PAI-1 has little effect on the binding of Vn to alpha vbeta 3. These findings are consistent with the observation that latent PAI-1 lacks high-affinity binding to denatured Vn (41). However, when Vn·alpha vbeta 3 were preformed on microtiter wells, active PAI-1 failed to dissociated these complexes (data not shown).


DISCUSSION

The observations in this report demonstrate that native Vn, present in blood, is not an adhesive glycoprotein. This conclusion is based on the findings that antibodies against Vn that block its adhesive function fail to bind to the native form of Vn. These blocking antibodies are capable of binding to denatured Vn or PAI-1-induced Vn multimers. In addition, direct binding studies prove that denatured Vn binds to both GPIIb/IIIa and alpha vbeta 3, but that native Vn is unable to bind to these integrins. Moreover, native Vn, which is not adhesive, could be converted into an adhesive glycoprotein by chemical and thermal denaturation. It should be noted that at high concentration, binding of native Vn to integrins was observed. This finding is probably related to the presence of some denatured Vn in the native Vn preparation. This conclusion is supported by the observation that unfractionated plasma was unreactive with conformationally sensitive antibodies, whereas the native Vn employed in this study showed exposure, although limited in comparison with denatured Vn, of conformationally sensitive epitopes. Based on the observations presented here, the majority of Vn present in vivo (i.e. in plasma) is not expected to bind to integrins. A number of consideration suggest that the adhesive functions of Vn are mediated through the N-terminal SMB domain rather then the C-terminal glycosaminoglycan binding domain. First, site-directed mutagenesis studies revealed that the RGD motif located between amino acids 45 and 47 is required for cell adhesion to Vn (32, 33). Second, heparin does not effect the adhesion of HT 1080 or a number of other cell lines to immobilized Vn.2 Similarly, heparin was without effect in the purified receptor binding assay. Third, recent studies from our laboratory indicate that native Vn binds heparin, implying that the glycosaminoglycan binding domain is exposed in the native conformation.3

Interestingly, PAI-1 can have opposing effects on the adhesive properties of Vn. First, active PAI-1 blocked the binding of denatured Vn to alpha vbeta 3 in a dose-dependent manner. The binding site for active PAI-1 has been localized to amino acids 1 to 40 (41), a region in close proximity to the RGD sequence at residues 45-47 of Vn (3, 4). RGD-containing peptide has no effect on the binding of PAI-1 to Vn (41), suggesting that PAI-1 is not binding directly to the cell adhesion domain in Vn. The close proximity of both sides makes it likely that the competition of PAI-1 is due to steric hinderance. In contrast, latent PAI-1, which does not bind to the N-terminal high affinity PAI-1 binding site in Vn (41), failed to compete with integrin binding of Vn. In addition, PAI-1 failed to dissociate pre-existing Vn·alpha vbeta 3 complexes. Thus, PAI-1 is not expected to detach anchored cells, but may modulate biological processes dependent on de novo formation of adhesive contacts between Vn and alpha vbeta 3, including cell migration. These observations have been confirmed in a recent publication (47).

Second, active PAI-1 had an additional affect on Vn binding to integrins. PAI-1 induced the formation of conformationally altered Vn multimers, and these multimers present, after dissociation from PAI-1, an exposed cell adhesion domain. The Vn concentration in plasma is between 2.5 and 5 µM (1, 2), whereas normal PAI-1 levels are approximately 0.4 nM (48). Plasma levels of PAI-1 are regulated under pathophysiological conditions, and for example endotoxinemia results in a dramatic up-regulation of plasma PAI-1 levels to 20 nM (48). However, these concentrations are still 100-fold lower than that of Vn. Using this ratio of PAI-1 and Vn, we were unable to detect PAI-1 induced Vn multimers (10). Thus, PAI-1 induced Vn multimerization in plasma is expected to have little affects on the adhesive properties of Vn. The scenario may be quite different in tissues and in platelets. PAI-1 and Vn are both contained within platelet alpha -granules (49, 50), and platelets contain 26 nM Vn and 12 nM PAI-1 per 109 platelets (49, 51, 52). Interestingly, platelet Vn is present in high molecular weight multimers that express the mAB 153 epitope (50). It should be noted that the expression of the cryptic mAB 153 epitope appears to correlate with the adhesive properties of Vn. These observation suggest that platelet Vn is adhesion competent. Platelet-derived proteins concentrate up to 200-fold in areas of thrombosis, suggesting that platelet-derived adhesion competent Vn will accumulate in areas of tissue injury and thrombosis. Similarly, increased tissue-associated levels of PAI-1 have been reported in a number of pathophysiological conditions, including endotoxinemia (48), raising the possibility that PAI-1 will regulate the adhesive properties of Vn in inflamed tissues. Taken together, these observation support the concept that plasma Vn is in a latent form. Interactions with either free proteases inhibitors or inhibitors in complex with the respective target protease results in the exposure of the cryptic RGD motif.


FOOTNOTES

*   This work was supported by Grant 4KT-0192 from the California Tobacco-related Disease Research Program (to D. S.) and by National Institutes of Health Grants HL50704 (to D. S.) and AR42750 and CA56483 (to J. W. S.). This is publication number 10379-VB from the Department of Vascular Biology.The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
§   To whom correspondence should be addressed. Present address: DuPont Merck Research Laboratories, P. O. Box 80400, Wilmington, DE 19880-400. Tel.: 302-695-7069; Fax.: 302-695-4162; E-mail: seiffeda{at}a1.lldmpc.umc.dupont.com.
par    Established Investigator of the American Heart Association and Genentech.
1   The abbreviations used are: Vn, vitronectin; GPIIb/IIIa, glycoprotein IIb/IIIa; mAb, monoclonal antibody; PAI-1, type 1 plasminogen activator inhibitor; PBS, phosphate-buffered saline; SMB, somatomedin B.
2   D. Seiffert and J. W. Smith, unpublished observation.
3   D. Seiffert, unpublished observation.

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