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(Circulation. 2005;111:106-112.)
© 2005 American Heart Association, Inc.

Vascular Medicine

Gallic Acid Antagonizes P-Selectin–Mediated Platelet–Leukocyte Interactions

Implications for the French Paradox

Chantal C.M. Appeldoorn, PhD^*; Arnaud Bonnefoy, PhD^*; Bianca C.H. Lutters, PhD; Kim Daenens, MD; Theo J.C. van Berkel, PhD; Marc F. Hoylaerts, PhD; Erik A.L. Biessen, PhD

From the Division of Biopharmaceutics (C.C.M.A., B.C.H.L., T.J.C.v.B., E.A.L.B.), Leiden/Amsterdam Center for Drug Research, Leiden University, Gorlaeus Laboratories, Leiden, the Netherlands, and Center for Molecular and Vascular Biology (A.B., K.D., M.F.H), University of Leuven, Leuven, Belgium.

Correspondence to Marc Hoylaerts, Center for Molecular and Vascular Biology, University of Leuven, UZ Gasthuisberg, Herestraat 49, 3000 Leuven, Belgium. E-mail Marc.Hoylaerts{at}med.kuleuven.ac.be

Received April 28, 2004; revision received August 13, 2004; accepted September 30, 2004.

	Abstract

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Background— Current paradigm attributes the low incidence of cardiovascular disorders in Mediterranean countries despite a high saturated fat intake, the "French paradox," to the antioxidant capacity of red wine polyphenols. Conceivably, other antiinflammatory pathways may contribute to at least a similar extent to the atheroprotective activity of these polyphenols. We have investigated whether gallic acid (GA), an abundant red wine polyphenol, modulates the activity of P-selectin, an adhesion molecule that is critically involved in the recruitment of inflammatory cells to the vessel wall and thus in atherosclerosis.

Methods and Results— GA potently inhibited the binding of a peptide antagonist (IC₅₀, 7.2 µmol/L) and biotin-PAA-Le^a-SO₃H, an established high-affinity ligand, to P-selectin (IC₅₀, 85 µmol/L). Under dynamic flow conditions, GA markedly and dose dependently attenuated the rolling of monocytic HL60 cells over P-selectin-transfected Chinese hamster ovary cells (EC₅₀, 14.5 µmol/L) while increasing the velocity of P-selectin-dependent rolling of human blood leukocytes over a platelet monolayer. In vivo tests established that GA administration to normolipidemic C57/Bl6 and aged atherosclerotic apolipoprotein E–deficient mice impaired the baseline rolling of conjugates between activated platelets and circulating monocytes over femoral vein endothelium, as judged by online video microscopy (ED₅₀, 1.7±0.3 and 1.5±0.4 mg · kg^–1 · h^–1, respectively).

Conclusions— Our findings provide a solid mechanistic foundation through which GA intervenes in major inflammatory pathobiologies by binding and antagonizing P-selectin.

Key Words: atherosclerosis • endothelium • inflammation • nutrition • platelets

	Introduction

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Coronary artery disease (CAD) is the major cause of death in Western society. Intriguingly, in France, where there is a pattern of saturated fat intake similar to that of other Northern European countries and the United States, the incidence of CAD is 50% lower.¹ This so-called "French paradox" has fuelled considerable debate on the actual mechanism underlying this phenomenon, implicating a role for diet components and for the consumption of alcohol-containing beverages, particularly (red) wine.^2–4

Wine is an abundant source of polyphenolic antioxidants, including catechins and gallates. Indeed, wine was shown to inhibit atherosclerosis in hyperlipidemic mice,⁵ a finding that was tentatively attributed to an inhibitory effect on LDL oxidation.^6,7 Although the antioxidant theory may be plausible, recent outcomes of 3 randomized large-scale trials failed to confirm a protective effect of the antioxidant vitamin E on CAD,⁸ despite its inhibitory effect on lipid peroxidation in vivo.⁹ In analogy, treatment with probucol, a bisphenolic antioxidant, yielded contradictory results, depending on animal species and strain. Red wine polyphenols may thus be atheroprotective at least in part through nonantioxidant mechanisms. Catechins were reported to inhibit platelet-derived growth factor receptor-ß (PDGFRß)–mediated signaling in vitro,¹⁰ although inhibition of PDGF signaling may have an adverse effect on plaque stability, aggravating the pathobiology.¹¹ Resveratrol was reported to prevent platelet-leukocyte interaction and to reduce the expression of Mac-1.¹² Moreover, resveratrol and other polyphenols such as quercetin were also shown to enhance endothelial nitric oxide synthase¹³ and to reduce the expression of the procoagulant activity of vascular cells.¹⁴

Our attention was therefore drawn to gallic acid (GA), a major antioxidant constituent in red wine that has been shown to display in situ or as an alkyl derivative antioxidant¹⁵ and anticarcinogenic¹⁶ activity. Interestingly, we previously found that derivatization of peptide antagonists for human P-selectin with GA enhanced their affinity for P-selectin >500-fold.¹⁷ P-selectin is an adhesion molecule that is intrincally implicated in atherothrombosis by mediating leukocyte-endothelium, leukocyte-platelet, and platelet-platelet interactions.^18,19 The absence of P-selectin was found to result in reduced atherosclerotic lesion development and neointimal growth.²⁰ Recent evidence confirms that both endothelial and platelet P-selectin contribute to atherosclerosis, in agreement with the occurrence of P-selectin-dependent and platelet-assisted monocyte rolling over endothelial cells.²¹ In addition, P-selectin has been associated with thrombosis because P-selectin activation induces an improvement in platelet cohesion and mediates platelet-leukocyte aggregation.¹⁹ The surprisingly high affinity of the GA-modified peptides led us to investigate whether GA might bind and antagonize P-selectin by itself, thus providing an additional plausible explanation for the cardioprotective effect of GA and its derivatives.

	Methods

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Cell Culture
Chinese hamster ovary cells stably transfected with human P-selectin (CHO-P cells) were kindly donated by Dr P. Modderman (University of Amsterdam). Cells were grown in DMEM containing 10% FCS, 5 mmol/L L-glutamine, 20 000 U penicillin/streptomycin, and 5 mmol/L nonessential amino acids. Flasks with cells were incubated at 37°C in 5% CO₂ for 3 or 4 days until cells had grown nearly confluent. HL60 cells were from ATCC and grown in RPMI with 10% FCS, 5 mmol/L L-glutamine, and 20 000 U penicillin/ streptomycin.

Competition ELISA
Compounds were assayed for their ability to inhibit TM11-PO binding to human P-selectin²² or that of biotin-PAA-Le^a-SO₃H binding to human and mouse P-selectin and to human E- and L-selectin.²³

HL60 Adhesion Assay
HL60 cells were labeled with 5 µmol/L calcein acetoxymethyl ester (calcein-AM) for 30 minutes at 37°C. HL60 cells (50 000 per well) were added to CHO-P cells (seeded in 96 well plates) in the presence or absence of GA (1 hour at 4°C). After gentle washing, fluorescence was measured.

Platelet Isolation, Labeling, and Preparation of Platelet Monolayer
Platelet-rich plasma was prepared from human²⁴ and murine blood²⁵; then, washed platelets were incubated for 20 minutes at 37°C with 5 µmol/L calcein-AM.²¹ After the platelet suspension was centrifuged at 700g for 25 minutes, fluorescent platelets were resuspended in HEPES-Tyrode’s buffer. A human platelet carpet for subsequent perfusion studies was made by overnight coating of glass coverslips with calf skin collagen (1 mg/mL in 50 mmol/L acetic acid). Coverslips were then rinsed in complete Tyrode’s buffer (containing 2 mmol/L CaCl₂, 1 mmol/L MgCl₂, and 1% human albumin). Whole human blood anticoagulated with 20 µg/mL hirudin was then reperfused over the collagen-coated surface in a parallel-flow chamber at a shear rate of 300 s^–1 in the presence of 1 mmol/L tirofiban (Merck). In these conditions, a homogeneous carpet of activated spread platelets formed on the coverslips without the formation of platelet aggregates.

Flow Chamber and Perfusion Studies
Dynamic interactions between HL60 cells and CHO-P cell monolayers grown on glass coverslips coated with 30 µg/mL collagen S (Boehringer) were analyzed in a parallel-plate perfusion chamber as described.²¹ HL60 cell translocation over CHO-P monolayers was measured at wall shear rates of 300 and 600 s^–1. GA was added to the HL60 cell suspensions 2 minutes before the start of perfusion. To prevent oxidation, the GA solution was prepared fresh. The average velocity of HL60 cells rolling over the CHO-P cells was calculated from the rolling distance of the HL60 cells in a 1-second time frame with the NIH Image program. Adhered HL60 cells were counted from pictures taken during the same experiment.

Measurements of Intracellular Ca²⁺ Concentration
HL60 cells (3x10⁶) were incubated for 10 minutes at 37°C with 100 µmol/L of Quin-2 acetoxymethyl ester (Quin 2-AM), centrifuged, and resuspended in 3 mL Hanks’-HEPES buffer supplemented with CaCl₂, glucose, and BSA. Fluorescence was measured with a Perkin Elmer LS5 fluorimeter (_ex=339 nm, _em=492 nm) at 37°C under constant stirring (F_initial). After 1 minute, digitonin (1 µL, 5 mmol/L) was added to achieve F_max. F_min was measured by the addition of 200 µL of 500-mmol/L EGTA. GA (500 µmol/L) was added 1 minute before the initial fluorescence F_initial was measured. The intracellular calcium concentration (in nmol/L) was determined by (F_initial–F_min)/(F_max–F_min)x115.

Leukocyte Rolling Over Collagen-Bound Platelet Monolayers
Coverslips were coated overnight with 1 mg/mL calf skin collagen in 50 mmol/L acetic acid at 4°C and then rinsed in complete Tyrode’s buffer (containing 2 mmol/L CaCl₂, 1 mmol/L MgCl₂, and 1% human albumin) in the presence of 1 mmol/L Aggrastat. Under these conditions, a homogeneous carpet of spread platelets formed on the coverslips. Whole blood anticoagulated with 20 µg/mL hirudin was reperfused in a flow chamber at a shear rate of 300 s^–1 for 5 minutes at 37°C over collagen-coated glass coverslips. Blood was then progressively washed out with complete Tyrode’s buffer containing 1% human albumin and perfused at a constant shear rate of 150 s^–1 in the presence or absence of either 500 µmol/L GA or 25 µg/mL of the anti-P-selectin antibody WAPS12.2. After 3 minutes of washing, leukocytes translocating over the platelet carpet were visualized with an inverted microscope, digital movies were captured, and translocation velocity was calculated by image analysis.

In Vivo Inhibition of Endothelial Cell Inflammation
All animal experiments were reviewed and approved by the Institutional Review Board of the University of Leuven and performed in compliance with the guidelines of the International Society on Thrombosis and Hemostasis.²⁶ For the study of platelet-assisted leukocyte rolling over the endothelial surface of blood vessels in vivo, online video microscopy was performed in C57/Bl6 mice. Healthy wild-type (WT) mice (6 to 12 weeks old) were anesthetized with Nembutal (70 mg/kg IP), and the jugular vein was catheterized. After the femoral vein was exposed, mice were mounted on the table of an inverted epifluorescent microscope so that the blood circulation in the femoral vein could be visualized through a Cohu CCD video camera. Calcein-AM–labeled fluorescent murine platelets (500x10⁶ platelets in 200 µL) were then injected into the catheterized jugular vein, and baseline rolling was recorded for the labeled platelets. After 10 minutes, 50 µg/kg collagen and anti-_IIb/ß₃ antagonist G4120 (1 mg/kg) were injected to activate circulating platelets while preventing their aggregation. After 5 minutes, the collagen-induced rolling and tumbling of leukocyte-platelet conjugates were then recorded for 10 minutes. The number of rosettes rolling was counted in the registered movies. The effect of GA on rosette rolling was investigated in 2 complementary manners. In WT mice, it was injected 5 minutes before collagen administration, and rosette rolling was analyzed as in the controls. Interactions of rosettes with the vessel wall were also studied in the femoral vein of aged atherosclerotic apolipoprotein E–deficient (ApoE^–/–) mice (>1 year). In these mice, tumbling rosettes were counted 10 minutes after collagen injection to measure the steady-state rosette rolling; then, a GA bolus (0.75 to 7.5 mg/kg) was injected, followed by continuous GA infusion for up to 3 hours at 0.75 to 7.5 mg · kg^–1 · h^–1, during which time GA inhibition of vessel wall inflammation was measured in real time. For clarity, unless otherwise stated, "infusion of" indicates the use of a bolus injection of a given dose followed by infusion of the same dose per hour.

Statistical Analysis
Comparisons between groups were analyzed via 2-tailed Student’s t test. The ED₅₀ was calculated via a 4-parameter logistic curve-fitting logarithm with Grafit 3.0 software.

	Results

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The ability of GA to inhibit human P-selectin binding was studied in a competition assay based on a P-selectin-binding peptide (TM11, H₂N-CDVEWVDVSSLEWDLPC-COOH). TM11-PO, a tetrameric complex between streptavidin-PO and TM11-biotin, has previously been shown to bind with high affinity and specificity to human P-selectin.²² Interestingly, GA-derived peptides containing the consensus sequence of this peptide, like GA-(E)WVDV, displayed a considerably higher affinity for P-selectin in this competition assay (IC₅₀, 15 to 37 nmol/L)¹⁷ than the parental peptide, which bound P-selectin at micromolar concentration (IC₅₀, 8 µmol/L). GA by itself appeared to be a potent inhibitor of TM11-PO binding to human P-selectin at low micromolar concentrations (IC₅₀, 7.2 µmol/L) (Figure 1A).

View larger version (15K): [in this window] [in a new window]   Figure 1. GA antagonizes P- and L-selectin but not E-selectin. A, Competition of TM11-PO binding to human P-selectin by GA-EWVDV (), EWVDV (), and GA (). B, Competition of biotin-PAA-Lea-SO3 binding to human P-selectin (), mouse P-selectin (), human L-selectin (), and human E-selectin () by GA. C, Competition of HL60 cell adhesion to CHO-P cells by GA.

The specificity of GA was further assessed in a competition assay based on a biotinylated sulfo-Lewis A derivatized polyacrylamide (ie, biotin-PAA-Le^a-SO₃H, an established selectin ligand)²³ because TM11-PO does not bind to E-selectin. Although GA potently inhibited human P-selectin (85 µmol/L), it was ineffective against E-selectin binding (20% at a concentration of 1 mmol/L; Figure 1B), and it was a moderate inhibitor of L-selectin (IC₅₀, 241 µmol/L). GA binding to P-selectin appeared to be rather species independent because GA also antagonized mouse P-selectin binding with a similar affinity (IC₅₀, 199 µmol/L). Besides GA, n-dodecyl gallate, monophenols (4-hydroxy benzoic acid), and polyphenols [caffeic acid, and (-)-epigallocatechine gallate (EGCG)] were also tested for their capacity to antagonize human P-selectin binding (the Table). Only GA and EGCG were able to inhibit biotin-PAA-Le^a-SO₃ binding to human P-selectin.

View this table: [in this window] [in a new window]   Competition by Various Compounds of the Biotin-PAA-Lea-SO3 Binding to Human P-Selectin

Subsequently, GA was tested in a static cellular competition assay for its ability to inhibit the adhesion of HL60 cells to CHO-P cells. These macrophage-derived HL60 cells have a high expression of P-selectin glycoprotein ligand-1 (PSGL-1), the endogenous high-affinity P-selectin ligand.^27,28 Indeed, GA potently inhibited this interaction (IC₅₀, 14 µmol/L; Figure 1C). Under dynamic flow conditions, with GA added to the HL60 cells just before perfusion, GA dose dependently increased the rolling velocity of HL60 cells across a CHO-P monolayer (wall shear rate, 150 s^–1) at an EC₅₀ of 14.5 µmol/L, which is essentially similar to the capacity of GA to inhibit HL60 cell adhesion (Figure 2A). In the same experimental setup, the number of adhering HL60 cells was determined. Already at 50 µmol/L, GA significantly decreased the HL60 cell adherence to the CHO-P monolayer compared with the untreated control (–34% and –43%, respectively; Figure 2B), regardless of the wall shear rate (300 and 600 s^–1). At 250 µmol/L GA, inhibition was even more pronounced (–41% and –54%, respectively). Calcium influx in HL60 monocytes was not influenced by the addition of GA (500 µmol/L), suggesting that the observed inhibitory activity of GA is not caused by modulating signal transduction (Figure 2C).

View larger version (9K): [in this window] [in a new window]   Figure 2. HL60 cell adhesion to CHO-P cells is attenuated by GA. A, Velocity (µm/s) of calcein-AM–labeled HL60 cells rolling over CHO-P cell-coated coverslip at wall shear rate of 150 s–1 in presence of GA at indicated concentrations was quantified from 26 to 30 real-time movies. For each condition, rolling velocity of 20 individual HL60 cells was measured in 5 to 9 independent perfusion assays. Values represent mean±SEM (**P<0.001). B, Adherence of calcein-AM–labeled HL60 cells to CHO-P cell-coated coverslips at wall shear rate of 300 s–1 (open bars) and 600 s–1 (solid bars) in absence (control) or presence of GA (50 and 250 µmol/L) was quantified from 26 to 30 pictures taken during experiment in 2 independent perfusion assays (**P<0.001) vs control. C, Calcium influx in Quin-2-AM HL60 cells was unaffected by addition of 500 µmol/L GA. Intracellular Ca2+ concentrations were measured fluorometrically at ex=339 nm andem=492 nm (n=4).

Flow cytometry analysis of rosette formation between activated human platelets and monocytes in human blood revealed extensive platelet binding to monocytes when platelets were activated by collagen or the tromboxane A2 analog U46619 (not shown). This binding was entirely P-selectin dependent because the neutralizing anti-P-selectin antibody WAPS12.2 prevented conjugate formation entirely (Figure 3A). When the rolling of resting leukocytes over a carpet of activated platelets was analyzed, GA induced a sharp rise in the rolling speed of those cells retained on the platelet surface (Figure 3B), reflecting impaired adhesion. However, the platelet-endothelium interaction was not disturbed because the number of activated platelets adhering to activated EAhy-926 endothelial cells remained unaltered after the addition of GA (Figure 3C). Similarly, GA did not affect the adherence of calcein-labeled THP-1 cells to activated EAhy-926 endothelial cells (Figure 3D). This implies that intercellular/vascular cell adhesion molecule function is undisturbed in the presence of GA.

View larger version (23K): [in this window] [in a new window]   Figure 3. GA enhances velocity of P-selectin-dependent rosette rolling over activated platelets in vitro. A, Conjugate formation between monocytes and collagen-activated platelets in static conditions in absence (open bars) or presence (solid bars) of neutralizing anti-P–selectin antibody WAPS12.2 (25 µg/mL) as measured by FACS analysis with anti-CD14-FITC (monocytes), anti-CD62P-PE (P-selectin), or anti-CD61-PE (platelets) (P<0.001). B, Leukocyte rolling over platelet monolayer. Box plot representation of velocity distribution during rolling at shear rate of 150 s–1 in absence (control; number of cells analyzed=35) or presence (500 µmol/L) (number of cells analyzed=22) of GA. Mean rolling velocity is given (µm/s) (*P<0.05). C, Adherence of platelets to activated EAhy-926 endothelial cells (per 0.067 mm2) at shear rate of 150 and 300 s–1 in absence (open bars) or presence (250 µmol/L; solid bars) of GA. D, Adhesion of calcein-AM–labeled THP-1 cells to activated EAhy-926 endothelial cells in absence (open bars) or presence (500 µmol/L; solid bars) of GA at shear rate of 150 and 300 s–1. Seventeen to 23 cells were analyzed.

Injecting fluorescently labeled resting platelets into C57/Bl6 mice did not trigger platelet rolling or platelet adhesion on the femoral vein endothelium (not shown). When circulating platelets were activated by the intravenous administration of collagen, with the concomitant injection of anti-_IIb/ß₃ antagonist G4120 to avoid platelet aggregation, conjugates formed in situ between activated platelets and leukocytes. These rosettes were found to tumble along the vessel wall, as illustrated in Figure 4, which shows in each box an individual rosette representing 2 to 3 labeled platelets attached to a single unlabeled, and thus invisible, leukocyte (individual spots in Figure 4). Each box consists of an overlay of a series of consecutive pictures taken at 0.1-second intervals. Calculation of the number of rolling conjugates revealed an average of 46±7 rosettes rolling across the field (0.067 mm²) per minute (n=30 fields).

View larger version (29K): [in this window] [in a new window]   Figure 4. Dynamic tumbling of leukocyte-platelet conjugates over femoral vein endothelium in vivo. Five independent examples of overlay plots of online registered images between in situ-formed rosettes consisting of mouse leukocytes with attached fluorescently labeled collagen-activated mouse platelets. Each image interval represents 0.1 second. To appreciate covered distance, 50-µm scale bar is depicted, and flow direction is indicated by arrow. Leukocytes are unlabeled, and hence invisible, whereas leukocyte-bound platelets (2 to 3 per leukocyte) are labeled and appear as black dots. In example 2, in addition to rolling in direction of flow, conjugate spinning is evident.

Pretreatment of mice with GA before platelet activation dose dependently reduced conjugate tumbling with an ED₅₀ of 1.5±0.4 mg · kg^–1 · h^–1 (representing the dose of a combined injection/infusion protocol as described in Methods) (Figure 5A). Conjugate-vessel wall interactions were almost abrogated at an infusion dose of 2.25 mg GA · kg^–1 · h^–1 (to 6±2 conjugates per field per minute; n=16 fields). Tethering of individual platelets was marginal (Figure 6 and Data Supplement Movies).

View larger version (16K): [in this window] [in a new window]   Figure 5. GA reduces leukocyte-platelet tumbling in vivo. A, Dose-dependent inhibition of conjugate rolling over femoral vein endothelium by GA (administered before platelet activation) in C57/Bl6 mice is expressed as number of conjugates rolling per surface unit (0.067 mm2). B, Dose-dependent inhibition by GA (administered after platelet activation) of rolling of preformed leukocyte platelet conjugates over femoral vein endothelium in aged atherosclerotic ApoE–/– mice expressed relative to that of rolling in absence of GA. GA treatment consisted of single injection followed by infusion of same dose per hour (*P<0.05, **P<0.01).

View larger version (53K): [in this window] [in a new window]   Figure 6. Conjugate rolling and platelet adhesion in control and atherosclerotic mice. Adhesion of single platelets (arrows) and rolling of conjugates (identified by leukocyte-bound platelets circled in red) over femoral vein endothelium in C57/Bl6 mice (WT; left) and atherosclerotic mice (ApoE–/–; right) without (control; top) or with (bottom) prior infusion of GA (7.5 mg · kg–1 · h–1).

Injection of labeled platelets into aged atherosclerotic ApoE^–/– mice and subsequent in situ activation with collagen revealed increased rosette-endothelium interactions, as expected for endothelium activated by hyperlipidemia, ie, overexpressing von Willebrand factor,^24,29 and upregulating other adhesion molecules such as intercellular adhesion molecule-1, vascular cell adhesion molecule-1, or E-selectin.³⁰ In addition to increased rosette tumbling, the femoral venous endothelium of ApoE^–/– mice uncovered increased tethering of single individual platelets (Figure 6), in agreement with in vitro and ex vivo perfusion studies over endothelial cells and rabbit aorta endothelium.²⁴ In analogy to the studies in normolipidemic mice, in atherosclerotic ApoE^–/– mice injected with collagen to activate platelets and preform conjugates, the infusion of 3.75 mg GA · kg^–1 · h^–1 also led to a sharp decrease in the number of preformed tumbling conjugates down to 34±13% of control value (P<0.01) without affecting single platelet tethering (Figure 5B).

	Discussion

Top Abstract Introduction Methods Results Discussion References

 
Polyphenols, (red) wine-derived antioxidants, have received considerable attention during the last decade because they are likely to reduce the risk of CAD (the French paradox).¹ The atheroprotective effect of polyphenols has been tentatively attributed to their capacity to inhibit LDL oxidation^6,7,31 and to inhibit the expression of proinflammatory proteins, including PDGFRß.¹⁰ However, because large-scale trials have been largely inconclusive in showing an effect of other antioxidants, additional nonoxidant pathways may be at least equally prominent. The notion that red wine polyphenols act as a cardioprotective by inhibiting PDGFRß activity is contradicted by recent studies showing that the PDGFRß axis is instrumental in maintaining plaque stability and in preventing aneurysm formation by promoting vascular smooth muscle cell migration to and their proliferation in the cap.^11,32 The present report shows that GA, one of the most abundant polyphenols in red wine, can potently intervene in P-selectin function, an adhesion molecule that is intrincally involved in the initial rolling of monocytes along the inflamed endothelium³³ and in thrombosis.^19,34

Previously, we reported that derivatization of specific human P-selectin-binding peptides with GA led to a dramatically enhanced affinity of the peptide toward P-selectin.¹⁷ This led to the presumption that GA by itself may specifically interact with P-selectin. Indeed, the polyphenol was found to inhibit the binding of 2 different selectin ligands, TM11-PO²² and biotin-PAA-Le^a-SO₃H,²³ to P-selectin at micromolar affinity. Conceivably, the TM11-based assay is most reflective of the functional activity of GA, which is corroborated by the finding that static and dynamic interactions between PSGL-1 displaying HL60 cells and CHO-P monolayers were inhibited by GA. The interaction appears to be rather specific for P-selectin, although GA also displayed some affinity for L-selectin, which is in concordance with previous studies showing that the ligand binding profiles of P- and L-selectin largely overlap.³⁵

In vitro, GA does not disturb platelet-endothelium or leukocyte-endothelium interaction. However, GA induced a sharp rise in the rolling speed of leukocytes retained on the platelet surface, reflecting impaired adhesion. In vivo studies of platelet-assisted inflammation indicate that GA can interrupt platelet-assisted rolling and tumbling of platelet-leukocyte rosettes over the endothelium of normocholesterolemic and hypercholesterolemic mice without affecting the deposition of single platelets on activated endothelium. This effect could be observed when GA was administered before and even after platelets had been activated.

GA effects in vitro and in vivo are not attributable to its antioxidant activity. n-Dodecyl gallate displays an antioxidant activity similar to that of GA, although it is unable to inhibit P-selectin binding at low concentrations. Similarly, other equally potent and structurally related antioxidants such as caffeic acid and dihydroxy benzoic acid are completely ineffective in inhibiting P-selectin. Finally, precautions were taken to prevent oxidation of the gallate during the experiments (which can easily be appreciated because oxidized gallate is dark green/brown).

GA is abundantly available not only in wine (grapes) but also in (green) tea. The total phenolic content in various red wines was analyzed as 1100 to 3165 mg/L, of which GA attributes 35 to 70 mg/L and the epicatechine gallate derivatives attribute 120 to 360 mg/L.³⁶ The GA content of green tea is even higher (2.2 mg/mL, corresponding to 149 mg/g dry leaves).³⁷ A study by Lee et al³⁸ showed that cocoa contained higher total gallate levels than green tea or red wine (611 versus 165 and 340 mg per serving, respectively). Oral administration of only 50 mg GA to a healthy volunteer resulted in plasma levels of GA and its major metabolite 4-O-methylgallic acid in the low micromolar range,³⁹ implying that the observed EC₅₀ values of 15 to 40 µmol/L can be readily reached after consumption of only 100 to 500 mg GA.

In addition to being involved in atherosclerosis and thrombosis, P-selectin was reported to play a role in metastasis by promoting tumor growth and to facilitate the metastatic seeding of mucin-producing carcinomas.⁴⁰ P-selectin deficiency was shown to be accompanied by reduced implanted carcinoma cells growth and reduced metastasis formation.⁴⁰ In addition, P-selectin is expressed by several metastatic pancreatic tumor cells.⁴¹ Thus, it is interesting that Ohno et al⁴² recently demonstrated that GA administration (50 mg/kg) could inhibit metastasis formation and growth.

In conclusion, GA inhibits P-selectin-mediated inflammation both in vitro and in vivo. This study provides for the first time a molecular mechanism through which GA can exert a beneficial effect in several pathobiologies such as CAD, thrombosis, and cancer by binding and antagonizing P-selectin under static and dynamic conditions already at concentrations readily achieved after moderate wine, (green) tea, or cocoa consumption.

	Acknowledgments

 
This study was partly funded by grants from Yamanouchi Japan (C.C.M.A, B.C.H.L), the Netherlands Organization of Scientific Research (NWO grant 016.026.019 to E.A.L.B), and the Dutch Heart Foundation (NHS, 2003T201). The support of the FWO Vlaanderen (project G.0376.01) is recognized. During this study, A.B. was the holder of a Marie Curie fellowship. K.D. is the recipient of a junior fellowship from the University Hospital Leuven. The skillful assistance of Petra Vandervoort during the cell culture and coverslip preparation and of Hans de Bont during Ca flux measurements is highly appreciated.

	Footnotes

 
*Drs Appeldoorn and Bonnefoy contributed equally to this work.

The online-only Data Supplement, which contains 4 movies that supplement the Results, can be found with this article at http://www.circulationaha.org.

	References

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