Regulation of platelet membrane levels of glycoprotein VI by a platelet-derived metalloproteinase

doi:10.1182/blood-2004-04-1549

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Blood, 1 December 2004, Vol. 104, No. 12, pp. 3611-3617.
Prepublished online as a Blood First Edition Paper on August 12, 2004; DOI 10.1182/blood-2004-04-1549.

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HEMOSTASIS, THROMBOSIS, AND VASCULAR BIOLOGY
Regulation of platelet membrane levels of glycoprotein VI by a platelet-derived metalloproteinase
Elizabeth E. Gardiner, Jane F. Arthur, Mark L. Kahn, Michael C. Berndt, and Robert K. Andrews
From the Department of Biochemistry and Molecular Biology, Monash University, Melbourne, Australia; and Department of Medicine, University of Pennsylvania, Philadelphia, PA.

   Abstract

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Thrombosis can be initiated when activated platelets adhereto injured blood vessels via the interaction of subendothelialcollagen with its platelet receptor, glycoprotein (GP) VI. Herewe observed that incubation of platelets with convulxin, collagen,or collagen-related peptide (CRP) resulted in GPVI signaling-dependentloss of surface GPVI and the appearance of an approximately55-kDa soluble fragment of GPVI as revealed by immunoblotting.Ethylenediaminetetraacetic acid (EDTA) or GM6001 (a metalloproteinaseinhibitor with broad specificity) prevented this loss. In otherreceptor systems, calmodulin binding to membrane-proximal cytoplasmicsequences regulates metalloproteinase-mediated ectodomain shedding.In this regard, we have previously shown that calmodulin bindsto a positively charged, membrane-proximal sequence within thecytoplasmic tail of GPVI. Incubation of platelets with calmodulininhibitor W7 (150 µM) resulted in a time-dependent lossof GPVI from the platelet surface. Both EDTA and GM6001 preventedthis loss. Surface plasmon resonance demonstrated that W7 specificallyblocked the association of calmodulin with an immobilized syntheticpeptide corresponding to the calmodulin-binding sequence ofGPVI. These findings suggest that disruption of calmodulin bindingto receptor cytoplasmic tails by agonist binding to the receptortriggers metalloproteinase-mediated loss of GPVI from the plateletsurface. This process may represent a potential mechanism toregulate GPVI-dependent platelet adhesion.

   Introduction

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Platelets adhere to sites of endothelial cell damage in a processrequiring rapid activation of multiple signaling events. Underconditions of low shear stress, the platelet membrane receptorglycoprotein (GP) VI is able to bind collagen and mediates intracellularsignaling events that lead to an up-regulation of platelet adhesionreceptors including platelet P-selectin and the fibrinogen receptoron platelets, ${alpha}$ _IIb ${beta}$ ₃ integrin.^1,2 Platelet adhesion to exposedcollagen is then stabilized by an additional collagen receptor, ${alpha}$ ₂ ${beta}$ ₁ integrin.
GPVI is a 60- to 65-kDa protein containing 2 extracellular immunoglobulin(Ig)–like domains, a single transmembrane domain and acytoplasmic tail of about 51 amino acids.^3,4 Along with collagen,other ligands such as collagen-related peptide (CRP)⁵ and thesnake venom protein convulxin⁶ can bind to the extracellularregion of GPVI, rapidly inducing intracellular tyrosine phosphorylationof numerous proteins, leading to the activation of ${alpha}$ _IIb ${beta}$ ₃ integrinand formation of platelet aggregates. The rate and strengthof an observed intracellular signal appears to be proportionalto the potency of each GPVI agonist to cross-link the receptorand induce clustering of GPVI molecules.^1,7,8 Although the precisemechanism by which GPVI signals remains unclear, the receptoris homologous to immune receptors and associates with the Fcreceptor (FcR) ${gamma}$ subunit of FcR^9,10 via a salt bridge withinthe platelet membrane. This association allows ligand-boundGPVI to use a single immunoreceptor tyrosine-based activationmotif (ITAM) within the cytoplasmic tail of FcR ${gamma}$ and signal viaSyk tyrosine kinase.¹¹ More recently, the Src tyrosine kinase,Lyn,¹² and calmodulin¹³ have been demonstrated to bind directlyto the cytoplasmic tail of GPVI, suggesting that the tail ofGPVI also plays a direct role in GPVI-mediated signaling. Indeed,a requirement for the entire cytoplasmic tail of GPVI as wellas associated FcR ${gamma}$ for complete convulxin-mediated signalinghas been confirmed.¹⁴
Loss of GPVI from the surface of mouse platelets is protectiveagainst thrombosis in a mouse carotid artery model of thromboembolism.¹⁵The loss of GPVI in this study¹⁵ was induced by treatment ofmouse platelets with the anti-GPVI rat monoclonal antibody JAQ1¹⁶and was proposed to be mediated primarily through receptor internalizationmechanisms, although proteolytic shedding of GPVI was not excluded.Regulation of activated adhesion receptors through proteolysisis well recognized as a mechanism for modulation of cell surfaceproteins^17,18 and has been identified in a number of systemsincluding proteolytic cleavage of Notch,¹⁹ and adhesion proteins,^20-22as well as numerous cytokines, growth factors, and their receptors.^17,23-25In the majority of cases, one or more membrane-bound metalloproteinasesappear to be responsible for the extracellular processing observed.^26,27A role for calmodulin in the metalloproteinase-dependent releaseof L-selectin from leukocytes has also been described.²⁸ Thisectodomain proteolysis of L-selectin was dependent on loss ofbinding of calmodulin to a membrane proximal amphipathic helixwithin the cytoplasmic tail of L-selectin.²⁹
In the course of our studies on the association of calmodulinwith the GPVI cytoplasmic tail,¹³ we investigated whether GPVIwas lost from the platelet surface under both resting conditionsand conditions of activation. On ligation of GPVI, or when calmodulinwas dissociated from the cytoplasmic tail of GPVI, we observeda loss of up to 90% of GPVI from the surface of platelets thatcould be blocked by inclusion of a metalloproteinase inhibitor.These results show for the first time that levels of GPVI receptorcan be down-regulated on human platelets and support the hypothesisthat calmodulin binding to cytoplasmic sequences of membrane-expressedreceptors is a specialized control mechanism for proteolyticshedding common to several different cell and receptor types.

   Materials and methods

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Materials
Soybean trypsin inhibitor, thrombin, and pepstatin A were purchasedfrom Sigma (St Louis, MO). Leupeptin and thrombin-related agonistpeptide (TRAP) were purchased from Auspep (Parkville, Australia).Horseradish peroxidase (HRP)–conjugated or fluoresceinisothiocyanate (FITC)–conjugated antimouse and antirabbitimmunoglobulin (Ig) antibodies raised in sheep were from Chemicon(Melbourne, Australia). GM6001 (a hydroxamic acid-based metalloproteinaseinhibitor with broad specificity)³⁰ and the calmodulin inhibitorW7 (N-(6-aminohexyl)-5-chloro-1-naphthalenesulfonamide) as wellas inhibitors of intracellular signaling molecules, PP1 andPP2 (Src kinase inhibitors), piceatannol (Syk inhibitor), andwortmannin (phosphatidylinositol 3 kinase [PI3K] inhibitor)were obtained from Calbiochem (La Jolla, CA). Purified convulxinfrom the venom of the South American rattlesnake Crotalus durissusterrificus was a kind gift from Dr Kenneth Clemetson (Berne,Switzerland). von Willebrand factor from human factor VIII concentratesand botrocetin from Bothrops jararaca were purified as previouslydescribed.^31,32 A monoclonal antibody, 6B12-3, against humanplatelet GPVI was raised essentially as described elsewhere.⁷6B12-3 recognized GPVI on intact platelets by flow cytometry(not shown) and recognized a single platelet protein of approximately60 kDa by Western blot analysis at an immunoglobulin proteinconcentration of approximately 2 µg/mL (100-fold dilutionof hybridoma medium).
Synthetic peptides with sequence corresponding to the cytoplasmiccalmodulin-binding sequence of human GPVI or the C-terminusof human GPIb ${alpha}$ were purified by reverse-phase high-pressure liquidchromatography and characterized by mass spectrometry (Mimotopes,Clayton, Victoria, Australia). The GPVI-specific agonist, CRPwith amino acid sequence GCO(GPO)₁₀GCOG-NH₂ where O representshydroxyproline, was a kind gift of Dr Su Kulkarni (Monash University).Cysteinyl residues at the N- and C-termini of CRP were cross-linkedusing the chemical cross-linker (3-(2-pyridyldithio)propionicacid N-hydroxysuccinimide (Sigma) as described.³³
Shedding of GPVI from platelets
Human platelets were isolated from venous blood using acid-citratedextroseas anticoagulant and washed 3 times by centrifugation in 0.15M NaCl containing 37.5 mM sodium citrate and 5 mM glucose, pH7.0, as previously described.³⁴ Platelets were counted and resuspendedin Tyrode buffer (5 x 10⁸ platelets/mL). To examine the effectof GPVI ligands on platelet GPVI levels, aliquots (0.1 mL) ofplatelets were mixed with 0.1 mL Tyrode buffer containing (finalconcentration) convulxin (0.5 µg/mL), collagen (20 µg/mL),CRP (20 µg/mL), W7 (0.1 mM), thrombin (1 U/mL), or botrocetin(2.5 µg/mL) plus von Willebrand factor (10 µg/mL)and incubated at room temperature for the indicated times. Someplatelet suspensions also contained 1 to 10 mM leupeptin, pepstatinA, soybean trypsin inhibitor, GM6001, or ethylenediaminetetraaceticacid (EDTA). In experiments investigating a role for intracellularsignaling events in GPVI shedding, platelet suspensions weretreated with 10 µM PP1, 10 µM PP2, 0.1 µMwortmannin, or 30 µg/mL piceatannol for 10 minutes priorto addition of convulxin. Where appropriate, an equivalent volumeof dimethyl sulfoxide (DMSO; vehicle) was added to samples.Incubations were halted by addition of 0.1 mL of 10 mM EDTAand platelets were pelleted by centrifugation at 15 000g for1 minute. The supernatant fraction was isolated and mixed with0.1 mL sodium dodecyl sulfate (SDS) sample loading buffer. Theplatelet pellet was treated with 0.3 mL lysis buffer (0.01 MTris [tris(hydroxymethyl)aminomethane], pH 7.5, containing 0.15M NaCl, 5 mM EDTA, 1% Triton X-100, 10 µg/mL each of soybeantrypsin inhibitor, leupeptin, and pepstatin, and 1 mM sodiumfluoride, sodium orthovanadate, and 5 mM phenylmethylsulfonylfluoride) on ice for 30 minutes. Platelet lysates were thenmixed with 0.1 mL SDS sample loading buffer. All aliquots ofplatelet lysates or supernatants were electrophoresed on 5%to 20% polyacrylamide-SDS gels, electrotransferred to nitrocellulose,and immunoblotted with anti-GPVI monoclonal antibody 6B12-3.Alternatively, some nitrocellulose filters were probed withthe anti- ${beta}$ ₃ integrin monoclonal antibody CRC54,³⁵ the antiplateletendothelial cell adhesion molecule 1 (PECAM-1) monoclonal antibody,WM59,³⁶ or the anti-GPIb ${alpha}$ monoclonal antibody WM23.³⁷ All blotswere probed with HRP-labeled antimouse IgG secondary antibody(Silenus, Hawthorn, Australia) and visualized using the enhancedchemiluminescence (ECL) detection method (Amersham, Buckinghamshire,United Kingdom).
Convulxin-dependent association of GPVI with GPIb by immunoprecipitation
For immunoprecipitation experiments, washed platelets (5 x 10⁸/mL)were resuspended in 0.01 M HEPES (N-2-hydroxyethylpiperazine-N'-2-ethanesulfonicacid) buffer, pH 7.6, containing 5 mM EDTA and 0.15 M NaCl,and left untreated or treated with GPVI agonists for 60 minutes.Platelets were then lysed by the addition of ice-cold lysisbuffer (final concentration: 20 mM Tris-HCl, pH 7.4, 5 mM EGTA[ethylene glycol tetraacetic acid], 1% Triton X-100, Completeprotease inhibitor cocktail [Roche Diagnostics, Basel, Switzerland]).Lysates were centrifuged at 15 000g for 10 minutes at 4°Cto pellet insoluble material. Immunoprecipitation of GPIb ${alpha}$ fromthe Triton-soluble supernatant was performed by addition of10 µg purified polyclonal antiglycocalicin (or nonimmunerabbit immunoglobulin) to precleared platelet lysates incubatedovernight at 4°C as previously described.^34,38 Immunoprecipitatedproteins were resolved by 5% to 20% SDS-polyacrylamide gel electrophoresis(PAGE) and transferred to nitrocellulose membrane for Westernblotting/ECL. Membranes were initially probed with anti-GPVImonoclonal antibody 6B12-3, followed by an HRP-labeled antimouseIgG secondary antibody (Silenus), and visualized using ECL.Membranes were stripped and reprobed with a monoclonal anti-GPIb ${alpha}$ antibody (WM23).
Effect of W7 on binding of calmodulin to its GPVI interaction sequence
A cDNA encoding full-length human calmodulin was cloned intothe pGEX-2T vector (Pharmacia, Uppsala, Sweden) using BamH1and Xho1 restriction sites and the sequence was verified byDNA sequencing. For expression of the GST-calmodulin fusionprotein, the construct was transfected into the BL21 strainof Escherichia coli and grown in the presence of 1 mM isopropylthiogalactoside(IPTG) for 4 hours at 37°C with constant shaking. The cellswere lysed and expressed protein was isolated by affinity chromatographyon glutathione-Sepharose, then GST was removed by treating theisolated protein with thrombin according to the manufacturer'sinstructions (Pharmacia). A second affinity chromatography stepon a column of W7 immobilized on Affigel 10/15 resin³⁹ was usedto isolate calmodulin.
The association of calmodulin with cytoplasmic sequences ofGPVI was measured by surface plasmon resonance using a BIAcore3000 (Pharmacia Biosensor AB, Uppsala, Sweden) maintained at25°C. Aliquots (5-10 µL) of biotinylated peptides(10 µM in 10 mM HEPES-saline, pH 7.0) with sequences matchingeither the calmodulin-binding sequence of GPVI, RRKRLRHRGRAVQRPL,or the final 10 residues of the cytoplasmic tail of GPIb ${alpha}$ , VSIRYSGHSL,were passed over streptavidin-coated sensor chips (SA5; Pharmacia)to an equivalent of 200 to 250 resonance units (RU) at a flowrate of 20 µL/min. A preparation of calmodulin (analyte)was dialyzed and diluted in 0.01 M HEPES-saline, pH 7.0, containing1 mM CaCl₂, to protein concentrations ranging from 10 nM to30 µM and volumes of 10 to 50 µL injected at a constantflow rate of 10 µL/min. To regenerate the surface aftereach sample, 10 µL 0.5% SDS in HEPES-saline was injectedto dissociate the calmodulin/peptide complex without disturbingthe biotinylated peptide/streptavidin interaction. The capacityof the peptide-coated sensor chip to bind calmodulin alone wasidentical at the start and at the end of each experiment.

   Results

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Treatment of platelets with GPVI agonists induces loss of GPVI from the platelet surface
Initially we investigated whether the level of GPVI was regulatedon platelets under conditions where GPVI was bound by a ligand.Washed platelets were resuspended in Tyrode buffer and incubatedat room temperature for various times with convulxin, CRP, orcollagen, all of which bind GPVI and activate platelets. Plateletand supernatant samples were analyzed by SDS-PAGE, transferredto nitrocellulose, and immunoblotted with an anti-GPVI monoclonalantibody 6B12-3. Figure 1A shows that 6B12-3 recognizes a singleband of molecular weight about 60 kDa in untreated platelets.In contrast, in platelets treated with either CRP, convulxin,or collagen, the 60-kDa band was lost with time, and a bandof molecular weight about 55 kDa appeared in the correspondingsupernatant fraction probed with 6B12-3. Although convulxinhas been reported to also bind GPIb ${alpha}$ ,^40,41 the release of GPVIfragment was not detected after treatment for 1 hour with eitherthrombin (Figure 1A) or a combination of von Willebrand factorand botrocetin (Figure 1B). Loss of more than 80% of GPVI proteinfrom platelets isolated from 5 different donors was observedwith convulxin after a 1-hour incubation (data not shown). Bycomparison, removal of GPVI from platelets treated with theweaker GPVI agonists, CRP or collagen, was less evident; however,after 30 minutes, the 55-kDa GPVI fragment could be detectedin the platelet supernatant (Figure 1A). Levels of PECAM-1 onplatelets remained stable throughout the experiment (Figure 1A).Inclusion of 10 mM EDTA in the platelet incubation mediumprior to the addition of convulxin, collagen, or CRP abrogatedthe loss of GPVI from the platelet surface suggesting a rolefor one or more metalloproteinases in GPVI shedding. Surfacelevels of other platelet membrane proteins such as PECAM-1 and ${alpha}$ _IIb ${beta}$ ₃ integrin (Figure 2) or GPIb ${alpha}$ (data not shown) remained constantthroughout the 1-hour incubation with GPVI agonists. We didnot analyze supernatants for release of receptors other thanGPVI; however, platelet-associated levels of these proteinsare essentially maintained under conditions where virtuallyall of the GPVI is shed (Figures 1, 2).

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Figure 1.. Treatment of platelets with GPVI agonists induces loss of GPVI from the platelet surface. (A) Washed human platelets (5 x 10⁸/mL) were resuspended in Tyrode buffer and treated with either 20 µg/mL CRP or collagen or 0.5 µg/mL convulxin (Cvx) for up to 60 minutes, or 1 U thrombin (Thr) for 60 minutes. EDTA (10 mM), where indicated, was included in some incubations. Platelet suspensions were incubated at room temperature, then mixed with 10 mM EDTA (final concentration) and centrifuged to isolate platelets from incubation medium supernatants. Platelet pellets were lysed in 1% Triton X-100 and aliquots of platelet extracts or supernatants were electrophoresed on SDS/acrylamide gels, transferred to nitrocellulose, then probed with anti-PECAM-1 antibody WM59 or anti-GPVI monoclonal antibody 6B12-3. An aliquot of resting platelet lysate is included on the left hand side of supernatant fractions for molecular weight comparison. Data are representative of at least 3 experiments with different donors. Two separate preparations each of collagen and CRP were tested and no difference was observed between each preparation of GPVI agonist for production of GPVI fragment. (B) Washed platelets were treated with 0.5 µg/mL convulxin or a combination of 2.5 µg/mL botrocetin (Botr0) plus 10 µg/mL von Willebrand factor (VWF) for 60 minutes. Incubations were then treated and analyzed as described for panel A.

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Figure 2.. Treatment of platelets with GPVI agonists does not induce loss of PECAM-1 or ${beta}$ ₃ integrin from platelets. Samples of resting and convulxin-treated platelet lysates were prepared as described in Figure 1 and were analyzed for levels of GPVI, PECAM-1, or ${beta}$ ₃ integrin by SDS-PAGE and immunoblotting with 6B12-3, WM59, or CRC54, respectively.

To further characterize the type of protease responsible forthe shedding of GPVI, washed platelets were treated with 0.5µg/mL convulxin in the presence of various proteolyticinhibitors (Figure 3A). Treatment of platelets with either EDTAor the hydroxamic acid-based, broad-range metalloproteinaseinhibitor, GM6001, but not pepstatin A, leupeptin, or soybeantrypsin inhibitor blocked the loss of GPVI from the plateletsurface and the liberation of the 55-kDa GPVI fragment intothe supernatant (Figure 3A). This concentration of GM6001 (100µM) has been used previously to demonstrate the involvementof metalloproteinases in loss of receptors from the surfaceof aging platelets.⁴² Those studies demonstrated that GM6001did not inhibit platelet receptor/agonist binding or act viaa nonspecific interaction with the platelet membrane.⁴² Ourresults thus suggest that the observed loss of GPVI from plateletstreated with convulxin, CRP, or collagen, is also mediated bymetalloproteinase-derived proteolysis.

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Figure 3.. Release of GPVI from platelets is blocked by a broad-spectrum metalloproteinase inhibitor. Washed human platelets were resuspended in Tyrode buffer and treated with 0.5 µg/mL convulxin in the presence of (A) 100 µM GM6001 or DMSO, 5 mM EDTA, 0.1 mM pepstatin A, 0.1 mM leupeptin, or 0.1 mM soybean trypsin inhibitor (SBTI) or (B) 10 µM PP1, 10 µM PP2, 0.1 µM wortmannin, 30 µg/mL piceatannol, or DMSO. Platelets were incubated at room temperature for 1 hour, then pelleted and lysed in buffer containing proteinase inhibitors and Triton X-100 as described in "Materials and methods." Aliquots of supernatants and platelet lysates were electrophoresed on SDS/acrylamide gels, transferred to nitrocellulose, and probed with anti-GPVI monoclonal antibody. An aliquot of resting platelet lysate is included on the left hand side of supernatant fractions for molecular weight comparison in panel A. Data are representative of at least 3 experiments with different donors.

To further characterize the mechanism of loss of GPVI from platelets,platelets were preincubated with inhibitors of intracellulartyrosine kinases including Src tyrosine kinases (PP1, PP2),PI3K (wortmannin), and Syk kinase (piceatannol) at concentrationsknown to interfere with GPVI-related signaling events.^6,13,43Shedding of GPVI was induced by addition of convulxin and levelsof GPVI fragment in samples of platelet supernatant were assessedby Western blot as described in "Materials and methods." Figure 3Bshows that inhibitors of Src, PI3K, and Syk blocked the releaseof GPVI fragment from convulxin-treated platelets, suggestinga role for these signaling proteins in the platelet GPVI-sheddingmechanism.
A GPVI⁺ fragment of approximately 55 kDa was also evident inincreased amount in the pellet of convulxin-treated plateletsas well as in the supernatant (Figures 1A and 3A). Convulxinis a disulfide-linked heterodimer consisting of homologous ${alpha}$ and ${beta}$ chains further linked by disulfide bridges to form cyclic ${alpha}$ 4 ${beta}$ 4 heterotetramers.⁴⁴ Because both GPIb and GPVI bind convulxin,⁴⁰it is likely that the increased association of shed GPVI withplatelets treated with convulxin is due to convulxin-bridgingassociation of the shed GPVI with membrane-bound GPIb. To investigatewhether this is the case, platelets were treated with convulxinin the presence of excess EDTA to prevent GPVI shedding, lysed,immunoprecipitated with anti-GPIb antibody, and Western blottedfor coassociated GPVI. Figure 4 shows that the relative levelsof GPIb-associated GPVI are increased in the presence of convulxinas compared with untreated platelets or platelets treated withCRP or collagen, although some GPVI was detectable in theselanes. In this regard, we have observed that GPVI is associatedwith GPIb-IX-V in both resting and activated platelets (J.F.A.et al, manuscript in preparation).

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Figure 4.. Immunoprecipitation of GPIb-GPVI complexes is increased by treatment of platelets with convulxin. Washed human platelets (5 x 10⁸/mL) were resuspended in HEPES-saline buffer, pH 7.4, containing 10 mM EDTA, and treated with either 20 µg/mL CRP or collagen or 0.5 µg/mL convulxin for 60 minutes, then lysed in the same buffer containing Triton X-100 and proteinase inhibitors as described in "Materials and methods." Platelet lysates were precleared, mixed with 10 µg/mL of either antiglycocalicin antibody or a nonimmune rabbit control antibody and immune complexes precipitated by mixing with protein A-Sepharose. After washing the beads, captured proteins were eluted in SDS sample loading buffer and analyzed for levels of GPVI by SDS-PAGE and immunoblotting using the anti-GPVI monoclonal antibody, 6B12-3. Blots were stripped and reprobed with the anti-GPIb ${alpha}$ monoclonal antibody, WM23. Data are representative of at least 3 experiments with different donors. IP indicates immunoprecipitation; WB, Western blotting; NT, not treated; and NIR, nonimmune rabbit IgG.

Inhibition of calmodulin induces loss of GPVI from platelets
We have previously identified that calmodulin binds to a positivelycharged membrane-proximal sequence within the cytoplasmic tailof GPVI. This association of calmodulin with GPVI was reducedin platelets treated with GPVI agonists but not other plateletreceptor agonists.¹³ Several other receptors including L-selectinand the epidermal growth factor (EGF) receptor are known tobe associated with calmodulin via positively charged cytoplasmicsequences.^29,45 Interestingly, these receptors undergo rapidextracellular domain shedding either on activation or aftertreatment with calmodulin inhibitors such as W7.^28,46 In bothinstances, shedding has been proposed to be a mechanism forautoregulation of each receptor's biologic activity. We thereforeinvestigated whether inhibition of calmodulin in platelets alsoresulted in a loss of GPVI from the platelet surface. Figure 5shows that the amount of surface GPVI in suspensions of washedplatelets in Tyrode buffer was stable for up to 4 hours, withno detectable levels of the 55-kDa fragment in the supernatant.However, after treatment of washed platelets with 150 µMW7 for 1 hour, more than 80% of GPVI was lost from the plateletsurface coinciding with the appearance of a 55-kDa fragmentin the supernatant (Figure 5). Loss of GPVI was observed atW7 concentrations from 25 to 300 µM (data not shown).This loss of GPVI from platelets was also observed with comparableconcentrations of a different calmodulin inhibitor, trifluoperazine(data not shown). Similar to treatment of platelets with GPVIagonists, convulxin, CRP, and collagen, the loss of GPVI inducedby calmodulin inhibition was blocked by both EDTA (Figure 5)and GM 6001 (data not shown).

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Figure 5.. Treatment of platelets with a calmodulin inhibitor induces loss of GPVI from the platelet surface. Washed human platelets were resuspended in Tyrode buffer and treated with 150 µM W7. EDTA (10 mM) was included in some incubations. Platelet suspensions were incubated at room temperature for up to 4 hours, then mixed with 10 mM EDTA (final concentration), and centrifuged to isolate platelets from the incubation medium supernatant. Platelet pellets were lysed in buffer containing Triton X-100 and proteinase inhibitors and aliquots of platelet extracts or supernatants were electrophoresed on SDS/acrylamide gels, transferred to nitrocellulose, and probed with anti-GPVI monoclonal antibody, 6B12-3. Data are representative of at least 3 experiments with different donors.

W7 causes the dissociation of calmodulin from its GPVI interaction site
W7 is known to bind calmodulin and thus is thought to competewith other binding partners such as amphipathic positively chargedpeptide sequences as occur in L-selectin, the EGF receptor,and GPVI.^13,29,45 To directly test whether W7 is able to disruptcalmodulin binding, surface plasmon resonance was performedusing immobilized biotinylated synthetic peptides either withsequence matching the known calmodulin binding sequence of GPVIor with control peptides. Peptides were immobilized on streptavidin-coatedbiosensor chips and unoccupied binding sites were blocked withexcess biotin. Preparations of purified calmodulin (analyte)were passed over the peptide surface and the interaction ofcalmodulin determined. Figure 6 shows sensorgrams depictingthe interaction over time of calmodulin with immobilized GPVIpeptide, but not a control GPIb ${alpha}$ peptide (data not shown). Theassociation of calmodulin with the immobilized peptide couldbe disrupted by mixing the fusion protein with 150 µMW7 or 10 mM EDTA prior to passing the analyte solution acrossthe sensor surface.

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Figure 6.. W7 causes the dissociation of calmodulin from its GPVI interaction site. Aliquots of purified calmodulin (10 µM) were passed over a surface plasmon resonance sensor chip containing immobilized biotinylated peptide with sequence matching the calmodulin-binding region of GPVI cytoplasmic tail, as described in "Materials and methods." The association of calmodulin in HEPES-buffered saline containing 1 mM CaCl₂ (trace A) or the same buffer containing 10 mM EDTA (trace B) or calmodulin that had been mixed with 150 µM W-7 prior to passage across the chip (trace C) was measured by surface plasmon resonance.

The mechanism of release of GPVI from platelets does not require active ${alpha}$ _IIb ${beta}$ ₃ integrin
At least one other protein, CD40 ligand (CD40L), can be proteolyticallyshed from the surface of activated platelets.⁴⁷ Although thisshedding results from stimulation of platelets with a wide varietyof agonists and is thus distinct from the GPVI agonist-dependentshedding observed in the present study, additional experimentswere performed to further evaluate whether a similar mechanismapplied for both events. CD40L shedding from activated plateletsis almost completely inhibited by blockade of ${alpha}$ _IIb ${beta}$ ₃ integrinwith RGD mimetics.^48,49 In contrast, blockade of ${alpha}$ _IIb ${beta}$ ₃-integrinfunction by RGD peptide had no effect on overall GPVI-dependentshedding induced by convulxin or by W7 (Figure 7). The availabledata therefore suggest that a specific metalloproteinase-dependentmechanism exists for the selective cleavage of GPVI on activatedplatelets.

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Figure 7.. Treatment of platelets with RGD peptide does not block ligand-induced loss of GPVI from platelets. Washed human platelets (5 x 10⁸/mL) were resuspended in Tyrode buffer alone or containing 100 µM RGD peptide and treated with either 0.5 µg/mL convulxin, 150 µM W7, or 1 U thrombin (Thr) for 90 minutes at room temperature. The treated platelets were then mixed with 10 mM EDTA and the platelets isolated by centrifugation. The platelet pellets were lysed in buffer containing Triton X-100 and proteinase inhibitors, and aliquots of the platelet extracts were electrophoresed on SDS/acrylamide gels, transferred to nitrocellulose, then probed with the anti-GPVI monoclonal antibody 6B12-3. This experiment is representative of at least 3 experiments with different donors.

   Discussion

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Abstract
Introduction
Materials and methods
Results
Discussion
References

In the present study, we have made the novel finding that treatmentof platelets with specific GPVI agonists such as collagen, convulxin,and CRP not only results in platelet activation but also subsequentproteolytic shedding of GPVI. Concomitant with loss of GPVIfrom the platelet surface, a soluble 55-kDa fragment of GPVIwas detected in the platelet supernatant. Convulxin was themost powerful inducer of GPVI proteolysis, with more than 90%of the platelet GPVI shed within 30 minutes (Figure 1A). Therelative abilities of different GPVI agonists to induce GPVIshedding correlates with their ability to induce tyrosine phosphorylation,platelet aggregation, and other readouts of platelet activation.^6,11The latter are likely to depend on the multimeric nature ofeach GPVI ligand and the relative ability of the GPVI agonistto induce clustering or cross-linking (or both) of the receptor.^1,2,8Our results imply that cross-linking may also facilitate sheddingalthough further studies are required to confirm this possibility.The ligand-induced loss of GPVI could be abrogated by both EDTAand a broad range metalloproteinase inhibitor, but not by inhibitorsof calpain, pepsin, and cathepsins (leupeptin and pepstatin)or trypsin (soybean trypsin inhibitor; Figure 3A), suggestingthat release of the GPVI ectodomain was mediated by a platelet-derivedmetalloproteinase.
Three lines of evidence suggest GPVI shedding involves a specificmechanism regulated by GPVI-associated calmodulin. First, onlyGPVI-binding ligands, but not other platelet agonists (thrombin,von Willebrand factor), induced loss of GPVI from plateletsand appearance of the soluble GPVI fragment in the supernatant(Figure 1). In contrast, collagen, convulxin, and CRP did notcause depletion of other platelet membrane glycoproteins underconditions where GPVI was completely lost (Figures 1, 2). Second,the metalloproteinase-dependent shedding of GPVI could be inducedin the absence of ligand by treating platelets with the calmodulininhibitor, W7 (Figure 5). Again, loss of GPVI was specific,and W7 blocked binding of calmodulin to a peptide based on thecalmodulin-binding sequence of GPVI in vitro (Figure 6). Convulxin-induceddissociation of calmodulin from GPVI is at least partly inhibitableby PP1,¹³ implying an activation-dependent mechanism of calmodulinrelease and is consistent with the present study, where inhibitionof GPVI-related signaling molecules Src, PI3, and Syk kinasesalso inhibits shedding (Figure 3B). Third, the mechanism forshedding is apparently different from that reported for theother platelet receptors, such as GPIb-IX-V⁴² or CD40L.⁴⁸ Inthe case of CD40L, shedding was dependent on ${alpha}$ _IIb ${beta}$ ₃ integrin andinhibitable by RGD mimetics. In contrast, GPVI shedding wasnot affected by RGD-dependent blockade of ${alpha}$ _IIb ${beta}$ ₃ integrin.
The proteolytic shedding of adhesion receptors is a well-documentedautocrine mechanism to control receptor activity^21,22,27,50and, for platelets, functional autocrine loops mediated by secretedfactors such as adenosine diphosphate (ADP) and CD40L are wellestablished.^47,51-53 Recent work by Bergmeier and coworkersexamining a platelet model of mitochondrial injury has linkedthe profound proteolytic shedding of GPIb ${alpha}$ observed in this systemto a platelet-derived metalloproteinase.⁴² The authors proposedthat levels of soluble GPIb ${alpha}$ ectodomain in plasma could be usedas an indicator of platelet hemostatic status and function.More recently, Boylan and colleagues⁵⁴ reported the detectionof a 52-kDa fragment of GPVI from the plasma of healthy individuals,indicating that a soluble form of GPVI occurs in normal humanplasma. In other systems, the release of soluble adhesion proteins,particularly the ligand-binding domains of proteins includingvascular cell adhesion molecule 1 (VCAM-1), intercellular adhesionmolecule 1 (ICAM-1), L-selectin, and P-selectin have been usedas clinical markers of vascular disorders.⁵⁵ Much less is knownabout the extent to which the shedding of specific adhesionproteins modulates cell adhesion.
The loss of GPVI observed here, together with the work of Nieswandtand colleagues¹⁵ demonstrating lack of responsiveness to collagenin vivo by murine platelets depleted in GPVI by treatment withthe rat monoclonal antibody, JAQ1, implies that removal of GPVIfrom platelet membranes would significantly attenuate plateletinteractions with collagen. Chen and colleagues⁷ also suggestedhuman platelets may respond to collagen in a graded fashiondepending on GPVI receptor density. The GPVI-calmodulin interactionprovides a potential mechanism for liberation of the 55-kDaectodomain fragment of GPVI, and therefore modulation of GPVIfunction. Calmodulin is a ubiquitous intracellular regulatoryprotein.^56,57 Within platelets, calmodulin has been identifiedas a cytoplasmic binding partner for GPVI¹³ and dissociatesfrom the receptor by ligand binding to GPVI.^13,14 Data presentedhere (Figure 6) suggest that W7 or EDTA can also cause dissociationof calmodulin from a calmodulin-binding peptide based on GPVI.W7 binds specifically to calmodulin (K_d $~$ 11 µM) and competesdirectly with the binding of calmodulin-dependent proteins.^58,59The dissociation of calmodulin from cytoplasmic sequences ofmembrane-expressed receptors could represent a specialized controlmechanism for proteolytic shedding.²⁸ We used W7 treatment asan approach to investigate potential mechanisms underlying GPVIshedding, rather than trying to study the effect of W7 on plateletfunction. W7 has been reported to have other inhibitory actionson platelets, for example, blocking collagen-dependent plateletaggregation.⁶⁰
The identity of the metalloproteinases on platelets responsiblefor GPVI ectodomain shedding, as well as the mechanism by whichthe metalloproteinase influences levels of GPVI, remain to beestablished. Four members of the matrix metalloproteinase (MMP)family, MMP-1, MMP-2, MMP-4, and MMP-9, have been identifiedin platelets.^61-64 Platelets also express at least one disintegrinand metalloprotease (ADAM) family member, ADAM10.⁶⁵ Interestingly,a role for platelet-derived MMP-1⁶¹ and MMP-2^62,66 has recentlybeen described in modulating platelet intracellular signalingand aggregation induced by several platelet agonists, althoughthe precise mechanism remains to be elucidated. Although severalother platelet membrane proteins in addition to GPVI are releasedeither via proteolysis or within platelet microparticles,^42,67-71additional studies are clearly necessary to evaluate the physiologicsignificance of this in regulating platelet function.
During submission of this manuscript, a paper by Bergmeier andcolleagues⁷² describing loss of GPVI from murine platelets ina mitochondrial injury model was published. This also involveda metalloproteinase-dependent mechanism generating a soluble55-kDa fragment of GPVI.

   Acknowledgements

We thank Dr Yang Shen for providing the GST-calmodulin constructand Ms Andrea Aprico for outstanding technical assistance.

   Footnotes

Submitted April 23, 2004; accepted July 12, 2004.
Prepublished online as Blood First Edition Paper, August 12,2004; DOI 10.1182/blood-2004-04-1549.

Supported by the National Health and Medical Research Councilof Australia, Monash University, and the National Heart Foundationof Australia.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: Elizabeth E. Gardiner, Department of Biochemistry and Molecular Biology, Monash University, Melbourne, Australia, 3800; e-mail: elizabeth.gardiner{at}med.monash.edu.au.

   References

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

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