Thrombospondin-1 Induces Tyrosine Phosphorylation of Adherens Junction Proteins and Regulates an Endothelial Paracellular Pathway

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Vol. 10, Issue 5, 1537-1551, May 1999

Thrombospondin-1 Induces Tyrosine Phosphorylation of Adherens Junction Proteins and Regulates an Endothelial Paracellular Pathway

Simeon E. Goldblum,^* Bradford A. Young,^* Ping Wang,^* and Joanne E. Murphy-Ullrich^§

^*Division of Infectious Diseases, Department of Medicine, Department of Veterans Affairs Medical Center, University of Maryland School of Medicine, Baltimore, Maryland 21201; and ^§Department of Pathology, Division of Molecular and Cellular Pathology, University of Alabama at Birmingham, Birmingham, Alabama 35294

Submitted October 22, 1998; Accepted March 1, 1999
Monitoring Editor: Joan Brugge

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Thrombospondin-1 (TSP) induces endothelial cell (EC) actin reorganization and focal adhesion disassembly and influences multipleEC functions. To determine whether TSP might regulate EC-EC interactions,we studied the effect of exogenous TSP on the movement of albuminacross postconfluent EC monolayers. TSP increased transendothelialalbumin flux in a dose-dependent manner at concentrations $>=$ 1 µg/ml(2.2 nM). Increases in albumin flux were observed as early as1 h after exposure to 30 µg/ml (71 nM) TSP. Inhibition of tyrosinekinases with herbimycin A or genistein protected against the TSP-inducedbarrier dysfunction by >80% and >50%, respectively. TSP-exposedmonolayers exhibited actin reorganization and intercellular gapformation, whereas pretreatment with herbimycin A protected againstthis effect. Increased staining of phosphotyrosine-containingproteins was observed in plaque-like structures and at the intercellularboundaries of TSP-treated cells. In the presence of protein tyrosinephosphatase inhibition, TSP induced dose- and time-dependent incrementsin levels of phosphotyrosine-containing proteins; these TSP doseand time requirements were compatible with those defined for ECbarrier dysfunction. Phosphoproteins that were identified includethe adherens junction proteins focal adhesion kinase, paxillin, $gamma$ -catenin, and p120^Cas. These combined data indicate that TSP can modulate endothelialbarrier function, in part, through tyrosine phosphorylation ofECproteins.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Thrombospondin-1 (TSP)¹ is an ~420-kDa trimeric glycoprotein secreted by numerous tissues, including vascular smooth muscleand endothelial cells (ECs), and is also present in the ECM (Mosher,1990; Lahav, 1993; Bornstein, 1995). TSP is not only expressedin tissues relevant and anatomically proximal to the vasculature,it is also present within the intravascular compartment circulatingboth in the plasma (Lahav, 1993) and in monocytes and the $alpha$ -granulesof platelets (Mosher, 1990; Lahav, 1993). Monocytes and plateletsboth continuously traffic through the microvasculature where theyinteract with the endothelial surface. Whether TSP is presentedto the vascular endothelium, in vivo, through an endocrine, paracrine,and/or autocrine pathway isunknown.

TSP influences multiple EC functions, including cell attachment to and spreading on substrates (Lawler et al., 1988; Mosher,1990; Taraboletti et al., 1990; Lahav, 1993; Bornstein, 1995),cell motility (Taraboletti et al., 1990), and angiogenesis (Tarabolettiet al., 1990; Iruela-Arispe et al., 1991). TSP is a member ofa small but growing number of structurally dissimilar counteradhesiveproteins that have been grouped together on a functional basis(Sage and Bornstein, 1991; Murphy-Ullrich, 1995). By definition,each of these so-called counteradhesive proteins, at least undercertain conditions, can alter cell-substrate interactions andactin cytoskeletal organization. This so-called counteradhesiveeffect includes inhibition of cell-ECM adherens junction or focaladhesion (FA) formation as well as stimulation of FA disassembly(Sage and Bornstein, 1991; Murphy-Ullrich, 1995). This emphasison single-cell morphology and on the cell-matrix interface hasencouraged studies of cells under subconfluent conditions. Onlyrecently has it been appreciated that counteradhesive proteinsmay also influence EC-EC interactions (Goldblum et al., 1994a).

The vascular endothelium presents a selective barrier that actively regulates movement of circulating macromolecules and cellsinto extravascular tissues and compartments (Malik et al., 1989;Luscinskas et al., 1991). A structure-function relationship appearsto exist between EC actin organization/shape and barrier function.Agents that disrupt actin microfilaments increase endothelialpermeability, previous F-actin stabilization protects againstthis increase, and established mediators of permeability induceactin reorganization (Shasby et al., 1982; Bussolino et al., 1987;Goldblum et al., 1993). In EC, F-actin is arranged into both centraltranscytoplasmic cables and a peripheral band (Wong and Gotlieb,1986). These microfilaments are linked to two types of adherensjunctions, FAs (Clark and Brugge, 1995; Parsons and Parsons, 1997)and the zonula adherens (ZA) (Kemler, 1993; Gumbiner, 1996; Barthet al., 1997). The cytoplasmic filaments terminate within theFA, and the subcortical filaments interdigitate with the ZA. Becausethe ZA mechanically couples the peripheral actin cytoskeletonto the surface receptors that mediate homophilic cell-cell adhesion,it is strategically located for regulation of the paracellularpathway. The signal transduction pathways that regulate the stateof assembly of these adherens junctions are incompletely understood;however, protein tyrosine phosphorylation of components withinthe FA (Clark and Brugge, 1995; Parsons and Parsons, 1997) andZA (Kemler, 1993; Gumbiner, 1996; Barth et al., 1997) are associatedwith changes in the state of adherens junction assembly and increasedvascular permeability (Abedi and Zachary, 1997; Esser et al.,1998).

Multiple domains within TSP recognize various EC surface receptors (Mosher, 1990; Lahav, 1993; Bornstein, 1995). Althoughthe specific signaling pathways to which each of these receptorsis coupled remain undefined, several EC receptors, including CD36(Bull et al., 1994), $alpha$ _v $beta$ ₃ (Blystone et al., 1996) and the integrin-associatedprotein (IAP) (Gao et al., 1996), have been coupled to tyrosinephosphorylation events. CD36 tightly associates with several srcfamily kinases (Bull et al., 1994). Sequences within TSP thatbind to the IAP receptor have been demonstrated to induce tyrosinephosphorylation of focal adhesion kinase (FAK), paxillin, anda unidentified 90-kDa protein in human melanocytes (Gao et al.,1996). TSP also interacts with other endogenous proteins includingTGF $beta$ (Murphy-Ullrich et al., 1992; Schultz-Cherry and Murphy-Ullrich,1993), a cytokine associated with multiple biological activities,including wound healing, proliferation, and angiogenesis (Robertsand Sporn, 1993). Activation of latent TGF $beta$ by TSP has been demonstratedboth in vitro (Schultz-Cherry and Murphy-Ullrich, 1993; Schultz-Cherryet al., 1995) and in vivo (Crawford et al., 1998). That TSP activatesTGF $beta$ , induces tyrosine phosphorylation and actin reorganization,and influences angiogenesis supports the concept that TSP bioactivityis mediated through changes in EC-EC homophilic adhesion. In thisstudy, we demonstrate that TSP regulates an endothelial paracellularpathway, in part, through a tyrosine phosphorylation-dependentpathway.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Human TSP Preparation

TSP was purified as described previously (Murphy-Ullrich et al., 1992; Schultz-Cherry and Murphy-Ullrich, 1993). Briefly,fresh human platelets (Birmingham American Red Cross, Birmingham,AL) were thrombin-stimulated, and the platelet releasate was appliedto a heparin-Sepharose CL-6B (Pharmacia, Piscataway, NJ) affinitycolumn preequilibrated with Tris-buffered saline (TBS)-C (0.01M Tris-HCl, 0.15 M NaCl, 0.1 mM CaCl, pH 7.4. The bound TSP waseluted and applied to an A0.5 M gel filtration column (Bio-RadLaboratories, Richmond, CA) preequilibrated with TBS-C, pH 7.4.TSP that was depleted of bound TGF $beta$ , i.e., stripped TSP (sTSP),was similarly prepared except that the gel filtration column wasequilibrated at pH 11.0. TGF $beta$ activity in TSP preparations wasmeasured using the normal rat kidney soft agar colony formationassay as described previously (Murphy-Ullrich et al., 1992; Schultz-Cherryand Murphy-Ullrich, 1993).

Endothelial Cell Culture

Bovine pulmonary artery endothelial cells (ECs) (American Tissue Culture Collection, Rockville, MD) were cultured in DMEM(Sigma, St. Louis, MO) enriched with 20% heat-inactivated (56°C,30 min) fetal bovine serum (Hyclone Laboratories, Logan, UT),L-glutamine 4 mM, nonessential amino acids, and vitamins in thepresence of penicillin (50 u/ml) and streptomycin (50 µg/ml) (Sigma)as described previously (Goldblum et al., 1993). To determinewhether these ECs expressed CD36 at the protein level, EC lysateswere resolved by electrophoresis and electrotransferred. Milk-fatglobule membranes of bovine mammary epithelial cells generouslyprovided by Dr. I. H. Mather (University of Maryland, CollegePark, MD) were used as the positive control for bovine CD36 (Greenwaltand Mather, 1985). The blot was incubated with rabbit anti-humanCD36 antibody (Alessio et al., 1996) kindly provided by Drs. N.N.Tandon and G.A. Jamieson (American Red Cross, Rockville, MD) followedby HRP-conjugated goat anti-rabbit immunoglobulin G (IgG) (Sigma)and developed with enhanced chemiluminescence (ECL) (Amersham,Arlington Heights, IL). In the bovine ECs used in these studies,no CD36 expression was detected (Young, unpublishedobservations).

Assay of Transendothelial Albumin Flux

Transendothelial ¹⁴C-BSA flux was assayed as described previously (Goldblum et al., 1993). Briefly, gelatin-impregnated polycarbonatefilters (Nucleopore, Pleasanton, CA) mounted in chemotactic chambers(ADAPS,, Dedham, MA) were inserted into wells of 24-well plates.Each upper compartment was seeded with 2 × 10⁵ ECs and cultured for 72 h. The baseline barrier function of eachmonolayer was determined by applying ¹⁴C-BSA to each upper compartment (0.5 ml) for 1 h at 37°C, afterwhich the lower compartment (1.5 ml) was counted for ¹⁴C activity. Only monolayers retaining $>=$ 97% of the ¹⁴C-BSA were studied. The monolayers were then exposed to increasingTSP concentrations for 6 h in media containing 10% fetal bovineserum. On the basis of the established dose-response relationship,other monolayers were exposed to TSP-enriched medium at a fixedTSP concentration (30 or 20 µg/ml) for increasing exposure times.Simultaneous controls with medium alone were performed for eachtime point. Transfer of ¹⁴C-BSA across EC monolayers was again assayed and expressed aspicomoles perhour.

To ensure that the increases in ¹⁴C-BSA flux across EC monolayers ascribed to our TSP preparations were due to TSP and not acontaminant(s), a murine monoclonal anti-TSP IgG antibody (Ab133) (Schultz-Cherry and Murphy-Ullrich, 1993) was used. EC monolayerswere exposed for 6 h to TSP (30 µg/ml), TSP preincubated withAb 133 (90 µg/ml, 1 h, 25°C) or Ab 133 alone. Transfer of ¹⁴C-BSA across EC monolayers was then assayed and expressed as picomolesper hour as described above. To exclude the contribution of endotoxinor bacterial lipopolysaccharide (LPS), transendothelial ¹⁴C-BSA flux was assayed after 6 h exposures to 30 µg TSP/ml, TSPpreincubated with polymixin B (PMB) immobilized onto agarose beads(Sigma), LPS derived from Escherichia coli:0111:B4 (Sigma) 100ng/ml, and LPS preincubated with PMB in the presence of 10% fetalbovine serum. Because LPS-induced barrier dysfunction is profoundlyserum dependent, the TSP-induced changes were also studied understrict serum-starvation conditions as described previously (Goldblumet al., 1994).

To determine whether TGF $beta$ might contribute to TSP-induced barrier dysfunction, human recombinant TGF $beta$ ₁, an anti-TGF $beta$ antibody(R&D Systems, Minneapolis, MN), as well as a peptide demonstratedto block activation of latent TGF $beta$ (GGWSHW) (Schultz-Cherry etal., 1995), each were tested in the barrier function assay. Tofurther exclude TGF $beta$ bioactivity, TSP that was depleted of boundTGF $beta$ , i.e. sTSP, was compared with equivalent concentrations ofnative TSP in the same barrier function assay. To determine whetherECM proteins other than TSP could augment transendothelial ¹⁴C-BSA flux, equimolar concentrations to TSP at 30 µg/ml (i.e.,71 nM for trimeric TSP) of human fibronectin, human vitronectin,and bovine type I collagen (all purchased from Collaborative BiomedicalProducts, Bedford, MA) each were simultaneously tested in thebarrier functionassay.

In other experiments, EC monolayers were pretreated with the protein synthesis inhibitor cycloheximide (Sigma) 50 µg/ml, 0.5h before and throughout the TSP or media exposures. This concentrationof cycloheximide inhibited >95% of EC protein synthesis as measuredby [³⁵S] methionine (New England Nuclear, DuPont, Boston, MA) incorporationinto trichloracetic acid-precipitable protein as we have describedpreviously (Goldblum et al., 1993). Simultaneous cycloheximidecontrols were alsoincluded.

Effect of Protein Tyrosine Kinase/Phosphatase Inhibition

To determine whether the state of EC protein tyrosine phosphorylation mediated TSP-induced changes in barrier function, experimentswere performed in the presence of either protein tyrosine kinase(PTK) or protein tyrosine phosphatase (PTP) inhibitors (Younget al., 1998). The concentration of each inhibitor was chosenon the basis of its activity in the barrier function assay; foreach agent the maximal concentration that did not alter albuminflux was used. EC monolayers were pretreated with genistein (50µg/ml or 185 µM), sodium orthovanadate (vanadate) (2.5 µM), orphenylarsine oxide (PAO) (0.1 µM) (Sigma), 0.5 h before and throughoutthe exposure to TSP or media. Herbimycin A (1.0 µM) (Sigma) wasintroduced ~16 h before and throughout the TSP or media exposure.The presence of dimethylsulfoxide 0.1% was controlled for in simultaneousmediacontrols.

Immunoblotting for EC Phosphotyrosine

Phosphotyrosine immunoblotting was performed as described previously (Young et al., 1998). Postconfluent EC monolayers wereexposed to TSP or to media alone, in the presence or absence ofPTK or PTP inhibitors for increasing exposure times. The cellswere then lysed with ice-cold lysis buffer containing 50 mM Tris-HCl,pH 7.4, 1% Nonidet P-40, 0.25% sodium deoxycholate, 150 mM NaCl,1 mM ethylene glycol tetraacetic acid, 1 mM phenylmethylsulfonylfluoride, 1 mg/ml leupeptin, 1 mg/ml pepstatin, 1 mg/ml aprotinin,100 mg/ml type-1 DNAse, 1 mM Na₃VO₄, 1 mM NaF, 10 mM pyrophosphate,500 µM paranitrophenol, and 1 mM PAO (all purchased from Sigma).The lysates were centrifuged, and the supernatants were collected.All samples were assayed for protein concentration with a standardBio-Rad DC Protein assay kit (Bio-Rad Chemical Division). Thesamples were resolved by electrophoresis on an 8-16% gradientSDS-polyacrylamide gel (Novex, San Diego, CA) and were transferredonto polyvinylidene difluoride membranes (ESA, Chelmsford, MA).To insure equal protein loading and transfer, each blot was stainedwith Fast Green concentrate (Sigma). The blot was blocked in 5%nonfat dry milk and incubated with biotinylated antiphosphotyrosinemAb (0.8 µg/ml) (4G10, Upstate Biotechnology, Lake Placid, NY)followed by HRP-conjugated streptavidin (Upstate Biotechnology)(0.5 µg/ml). The blot was developed with ECL and exposed to x-rayfilm (DuPont, Newark, DE) for increasing times. To confirm equivalentprotein loading, blots were stripped with 100 mM 2-mercaptoethanol,2% SDS, and 62.5 mM Tris-HCl, pH 6.7, and incubated with 0.5 µg/mlmurine antiphysarum $beta$ -tubulin IgG 2b (Boehringer Mannheim, Indianapolis,IN) followed by HRP-conjugated anti-mouse IgG (Transduction Laboratories,Lexington, KY), and developed with ECL. Autoradiographs were scannedby laser densitometry (Molecular Dynamics, Sunnyvale, CA). Inselected experiments, ECs exposed to human fibronectin, humanvitronectin, and bovine type I collagen were similarly processedfor phosphotyrosineimmunoblotting.

F-Actin Epifluorescence Microscopy and Immunolocalization of Phosphotyrosines

To maintain EC monolayers under experimental conditions identical to our permeability assay, we stained monolayers directlyon polycarbonate filters as described previously (Goldblum etal., 1993; Young et al., 1998). ECs grown to confluence on filterswere exposed for 6 h to TSP (20 µg/ml) or to media alone. Selectedcultures were incubated with herbimycin A (1.0 µM) for 16 h beforeand throughout the 6 h interval. The monolayers were fixed in3.7% formaldehyde for 20 min, rendered permeable in 0.5% TritonX-100 in HEPES buffer for 5 min, and stained with the F-actinprobe fluorescein-phalloidin (1.65 × 10⁷M) (Molecular Probes, Eugene, OR) for 20 min. In other experiments,ECs cultured on filters were probed for phosphotyrosine-containingproteins as described previously (Young et al., 1998). The monolayerswere washed with PBS containing 1 mM vanadate, fixed in 4% paraformaldehydefor 20 min followed by absolute methanol (10 min, $-$ 20°C), washed,and incubated for 1 h with FITC-conjugated antiphosphotyrosineantibody (5 µg/ml) (UBI). The filters and their attached monolayerswere mounted cell-side up on microscope slides and photographedthrough a Zeiss Axioskop 20 Microscope (Carl Zeiss, Thornwood,NY) equipped forepifluorescence.

Assay of EC Injury

To determine whether TSP-induced changes in endothelial barrier function could be explained by EC injury, TSP-exposed andmedium control monolayers were studied for ⁵¹Cr release as we have described previously (Goldblum et al., 1994).Briefly, ECs were labeled with [⁵¹Cr]-sodium chromate (Amersham), and the labeled monolayers wereincubated for 6 h with either TSP (30 µg/ml) or medium alone.The supernatants were centrifuged and counted. All washed monolayerswere solubilized with 1% Triton X-100 (Sigma) to induce maximumrelease. The lysates were centrifuged, and the supernatants werecounted for ⁵¹Cr activity. EC injury was expressed as [⁵¹Cr supernatant)/(⁵¹Cr supernatant + ⁵¹Cr cell lysate)] × 100%.

Identification of Phosphotyrosine-containing Proteins

EC lysates were precleared by incubation with antimurine IgG cross-linked to agarose (Sigma) for 1 h at 4°C and then incubatedovernight at 4°C with specific murine mAbs raised against paxillin, $beta$ -catenin, $gamma$ -catenin, p120^Cas, (Transduction Laboratories), or FAK (UBI). The resultant immunecomplexes were immobilized by incubation with antimurine IgG cross-linkedto agarose, centrifuged, washed, boiled for 5 min in sample buffer,and again centrifuged. The supernatants were processed for immunoblottingwith antiphosphotyrosine (4G10) antibody as described above. Tocontrol for discrepancies in the amount of immunoprecipitatedprotein, blots were stripped and reprobed with the immunoprecipitatingantibody. The blots were subsequently incubated with HRP-conjugatedantimurine IgG (Transduction Laboratories) and developed withECL. Autoradiographs were scanned by laser densitometry, and thephosphotyrosine-containing bands were normalized to the precipitatedprotein ofinterest.

Statistical Methods

ANOVA was used to compare the mean responses among experimental and control groups for all experiments. The Dunnett and ScheffeF-test was used to determine between which groups significantdifferences existed. A p value of < 0.05 was consideredsignificant.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

Effect of TSP on Transendothelial ¹⁴C-BSA Flux

TSP increased transendothelial ¹⁴C-BSA flux in a concentration-dependent manner (Figure 1A). The mean (±SE) pretreatment transendothelial¹⁴C-BSA flux was 0.008 ± 0.002 pmol/h (n = 30) and the mean (±SE)¹⁴C-BSA transfer across naked filters without EC monolayers was0.189 ± 0.003 pmol/h (n = 6). The lowest TSP concentration thatinduced a significant increment in ¹⁴C-BSA flux compared with the media control was 1.0 µg/ml. Themaximum mean (±SE) ¹⁴C-BSA flux of 0.118 ± 0.002 pmol/h was seen with TSP 30 µg/ml,at which point the TSP-induced effect had begun to plateau orsaturate (Figure 1A). The effect of TSP on endothelial barrierfunction was also time dependent (Figure 1B). Transendothelial¹⁴C-BSA flux was assayed after exposure to TSP (20 µg/ml) or mediaalone over a time period from 10 min to 6 h. ¹⁴C-BSA flux across media control monolayers did not change throughoutthe 6-h study period. TSP (20 µg/ml) induced significant incrementsin ¹⁴C-BSA flux compared with the simultaneous media control at $>=$ 2h (Figure 1B). In other studies, 30 µg/ml TSP significantly increased¹⁴C-BSA flux across EC monolayers as early as 1 h compared withthe simultaneous media control (0.033 ± 0.001 pmol/h, n = 9 vs.0.015 ± 0.002 pmol/h, n = 10, respectively) with further time-dependentincrements (Young, unpublished observations).

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Figure 1. Dose- and time-dependent effect of TSP on transendothelial ¹⁴C-BSA flux. Mean (±SE) pretreatment baseline transendothelial ¹⁴C-BSA flux is shown by the cross-hatched bars. *Significantly increased compared with the simultaneous media control at p < 0.05. (A) Closed circles represent mean (±SE) ¹⁴C-BSA flux in picomoles per hour immediately after 6-h exposures to increasing concentrations of TSP (0, 0.1, 1, 3, 10, and 30 µg/ml) in the presence of 10% serum (n = 5). (B) Circles represent mean (±SE) ¹⁴C-BSA flux in picomoles per hour immediately after increasing exposure times (0, 0.17, 0.5, 1, 2, 3, 4, 5, and 6 h) to TSP (20 µg/ml) ( $open circle$ ) (n = 4) and simultaneous medium controls (

) (n = 4).

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Figure 2. Neutralization of TSP and exclusion of endotoxin and TGF $beta$ . Vertical bars represent mean (±SE) transendothelial ¹⁴C-BSA flux in picomoles per hour. Mean (±SE) pretreatment baseline is shown by the closed bars, and n indicates the number of monolayers studied. (A) ¹⁴C-BSA flux immediately after 6-h exposures to TSP (30 µg/ml) and the simultaneous media control both in the presence of 10% serum, TSP and the media control under serum-free conditions, TSP + Ab 133 (90 µg/ml), PMB (15 µg/ml), LPS (100 ng/ml), LPS + PMB, and TSP + PMB. *Significantly increased compared with the appropriate media control at p < 0.05. **Significantly decreased compared with simultaneous control at p < 0.05. (B) ¹⁴C-BSA flux immediately after 6-h exposures to TSP (30 µg/ml) or stripped TSP (30 µg/ml) (cross-hatched bars) or the simultaneous media control (open bars). *Significantly increased compared with simultaneous media control at p < 0.05.

Effect of TSP on EC Injury

A ⁵¹Cr release assay was used to determine whether a TSP exposure (30 µg/ml, 6 h) that compromises endothelial barrier functionalso might induce EC injury or death over the same time period.This assay detects defects in the plasma membrane that permitpassage of molecules $<=$ 1000 Da. EC monolayers preloaded with ⁵¹Cr were exposed for 6 h to TSP (30 µg/ml) or media alone. Mean(±SE) ⁵¹Cr release from TSP-exposed EC was not significantly differentthan release from the simultaneous media controls (12.68 ± 0.35%,n = 8, vs. 11.97 ± 0.51%, n = 8, respectively), indicating thatTSP-induced changes in barrier function were not the result ofcytotoxicity.

Neutralization of TSP and Exclusion of Endotoxin

To ensure that the TSP-induced increases in ¹⁴C-BSA flux across EC monolayers could be ascribed to TSP bioactivity, TSP wastested both in the absence and presence of anti-TSP 133 IgG (Figure2A). Preincubation of TSP (30 µg/ml) with Ab 133 (Schultz-Cherryand Murphy-Ullrich, 1993) reduced the TSP effect by >80%. Endotoxin,in the presence of serum accessory molecules, is known to influenceendothelial barrier function (Goldblum et al., 1994). One TSPpreparation analyzed for endotoxin activity by a chromogenic limulusamebocyte lysate assay (Associates of Cape Cod, Inc., Woods Hole,MA) was found to contain ~0.36 ng endotoxin/µg TSP. To determinewhether these levels of endotoxin contributed to the TSP effectin the presence of serum, the ability of either serum deprivationor of PMB adsorption to decrease TSP-induced barrier dysfunctionwas examined (Figure 2A). The TSP effect in the presence or absenceof serum was not significantly different. The effect of TSP preincubatedwith a concentration of PMB that neutralizes 100 ng/ml LPS wasnot different from the effect of TSP alone. It is therefore unlikelythat TSP-induced changes in endothelial barrier function can beascribed to endotoxin contamination; however, these findings donot exclude the possibility of synergistic action between TSPand trace amounts ofendotoxin.

Exclusion of TGF $beta$

TSP is associated with variable amounts of active TGF $beta$ , usually ranging from 30 to 70 pg TGF $beta$ /µg TSP. We therefore testedup to >500-fold higher concentrations of TGF $beta$ (0.1-500 ng/ml)in the barrier function assay (Table 1). Six-hour exposures toTGF $beta$ at concentrations of $>=$ 1.0 ng/ml increased albumin flux comparedwith the simultaneous media control; however, the level of fluxobtained with 1.0 ng/ml TGF $beta$ could not account for the level offlux observed with 30 µg/ml TSP. Furthermore, significant incrementsin flux were observed with $>=$ 1.0 µg/ml TSP. At these concentrations,the estimated amount of associated TGF $beta$ ( $>=$ 0.035 ng/ml) activitywould be insufficient to significantly increase flux comparedwith media controls (Table 1). To further assess whether theTSP-associated TGF $beta$ activity contributed to the TSP effect, nativeTSP (30 µg/ml) was preincubated with anti-TGF $beta$ antibody and thentested in the permeability assay. Although the anti-TGF $beta$ antibodyat either 100 or 250 µg/ml diminished the TSP effect (Table 2),it only partially blocked it (30-35% inhibition), suggesting thatassociated TGF $beta$ activity or TSP-stimulated TGF $beta$ activity accountsfor only a fraction of the observed TSP activity. To determinewhether the TSP-associated TGF $beta$ activity was a requirement forthe TSP effect, TSP that was depleted of bound TGF $beta$ , i.e., sTSP,was compared with equivalent concentrations of native TSP withits associated TGF $beta$ activity for the ability to augment transendothelial¹⁴C-BSA flux (Figure 2B). TSP depleted of TGF $beta$ retained its abilityto induce changes in barrier function. In fact, on a molar basis,sTSP induced significantly greater barrier dysfunction than didTSP complexed with TGF $beta$ . Although TGF $beta$ can exert its own intrinsicactivity in the barrier function assay, it also might mask a siteon the TSP molecule that mediates increased vascular permeability.To determine the contribution of latent TGF $beta$ activation, the peptideGGWSHW known to block sTSP activation of latent TGF $beta$ (Schultz-Cherryet al., 1995) and an anti-TGF $beta$ antibody each were tested for theirability to diminish sTSP-induced barrier dysfunction (Table 2).The anti-TGF $beta$ antibody and the GGWSHW peptide each decreased thesTSP effect by ~15%, whereas the control peptide (GGYSHW) didnot. These data suggest that at higher TSP concentrations, TGF $beta$ activity can explain up to 30% of the TSP effect and that approximatelyone-half of this TGF $beta$ contribution (~15%) is due to TSP activationof latent TGF $beta$ .

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Table 1. Concentration-dependent effect of TGF $beta$ on endothelial barrier function

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Table 2. Contribution of TGF $beta$ to TSP-induced endothelial barrier dysfunction

Effect of ECM Proteins on Endothelial Barrier Function

To determine whether ECM proteins other than TSP might similarly influence endothelial barrier function, monolayers were exposedfor 6 h to equimolar concentrations of TSP, fibronectin, vitronectin,type I collagen, or media alone (Table 3). Of the ECM proteinstested, only TSP increased transendothelial ¹⁴C-BSA flux compared with the simultaneous media controls.

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Table 3. Effect of ECM proteins on endothelial barrier function

Effect of Protein Synthesis Inhibition on TSP-induced Changes in Endothelial Barrier Function

The increase in monolayer permeability was evident after 2-6 h of TSP exposure. It is possible that during this prolongedstimulus-to-response lag time, TSP could induce EC synthesis ofa second protein mediator(s) that could alter barrier functionin an autocrine/paracrine manner. To investigate this possibility,the ability of TSP to stimulate this response was examined inthe presence of a protein synthesis inhibitor. Pretreatment ofmonolayers with cycloheximide (50 µg/ml, 6 h) failed to blockthe TSP-induced increment in albumin flux (0.062 ± 0.001 pmol/h,n = 7 vs. 0.073 ± 0.008 pmol/h, n = 5). Cycloheximide alone failedto increase mean (±SE) ¹⁴C-BSA flux compared with the media control (0.016 ± 0.001 pmol/h,n = 5 vs. 0.019 ± 0.001 pmol/h, n = 12, respectively). Thus, denovo protein synthesis does not appear to be necessary for theresponse to TSP.

Effect of PTK Inhibition on TSP-induced Changes in Endothelial Barrier Function

To determine whether protein tyrosine phosphorylation mediated TSP-induced changes in barrier function, TSP was presentedto monolayers in the presence of one of two PTK inhibitors (Figure3A). The mean (±SE) pretreatment baseline barrier function was0.014 ± 0.006 pmol/h (n = 53). ¹⁴C-BSA flux across EC monolayers treated with either herbimycinA (1.0 µM) or genistein (185 µM) alone was not increased comparedwith the media controls. A 6-h exposure to TSP (30 µg/ml) significantlyincreased transendothelial ¹⁴C-BSA flux compared with the media control. Pretreatment of monolayerswith either herbimycin A or genistein protected against the TSP-inducedincrement by >80% and >50%, respectively. Therefore, two structurallyand functionally dissimilar PTK inhibitors each significantlydiminished the effect of TSP in this permeability assay.

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Figure 3. Effect of PTK inhibition on TSP-induced changes in endothelial barrier function and tyrosine phosphorylation of EC proteins. (A) Vertical bars represent mean (±SE) transendothelial ¹⁴C-BSA flux in picomoles per hour immediately after 6-h exposures to TSP (30 µg/ml), genistein (50 µg/ml), herbimycin A (1.0 µM), TSP + genistein, TSP + herbimycin A, and the simultaneous media control. Herbimycin A was introduced 16 h before the standard 6-h study period. The presence of dimethylsulfoxide 0.1% was controlled for in the media controls. The pretreatment baseline is shown by the closed bar. n indicates the number of monolayers studied. *Significantly decreased compared with treatment with TSP alone at p < 0.05. (B) ECs were exposed for 1 h to vanadate (200 µM) and PAO (1.0 µM) in the absence or presence of TSP (30 µg/ml) and in the absence or presence of either herbimycin A (1.0 µM) or genistein (50 µg/ml). Herbimycin A was introduced 16 h before the 1-h study period. The ECs were lysed and processed for immunoblotting for phosphotyrosine-containing proteins. Molecular weights in kilodaltons are indicated on the left.

Effect of PTP Inhibition on TSP-induced Changes in Endothelial Barrier Function

Consistent with the suggested involvement of PTK activity in TSP-induced loss of barrier function (Figure 3), inhibition ofPTP activity enhanced the TSP effect (Figure 4). The mean (±SE)pretreatment baseline barrier function was 0.012 ± 0.001 pmol/h(n = 89). Pretreatment of monolayers with either vanadate (2.5µM) or PAO (0.1 µM) alone for 6 h did not significantly increase¹⁴C-BSA flux compared with media controls. In the presence of TSP3 µg/ml, vanadate and PAO each enhanced the TSP effect by 62 and120%, respectively (Figure 4). At a higher TSP concentration of30 µg/ml, these same two PTP inhibitors enhanced the TSP effectby 17 and 33%, respectively. The ability of these two structurallyand functionally dissimilar PTP inhibitors to enhance the TSPeffect offers further evidence that TSP influences EC barrierfunction through protein tyrosine phosphorylation.

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Figure 4. Effect of PTP inhibition on TSP-induced changes in endothelial barrier function. Vertical bars represent mean (±SE) transendothelial flux in picomoles per hour immediately after 6-h exposures to TSP (3 or 30 µg/ml), vanadate (Van) (2.5 µM), PAO (0.1 µM), TSP + Van, TSP + PAO, and the simultaneous media control (open bar). The mean (±SE) pretreatment baseline is shown by the closed bar. n indicates the number of monolayers studied. *Significantly increased compared with treatment with TSP alone at p < 0.05.

Effect of PTK Inhibition on TSP-induced Intercellular Gap Formation

On the basis of data that PTK activity is involved in the TSP-induced loss in barrier function, the role of protein tyrosinephosphorylation in opening of the paracellular pathway was assessed.Accordingly, EC monolayers exposed to TSP (30 µg/ml) ± herbimycinA (1.0 µM) were stained with fluorescein-phalloidin, an F-actin-specificreagent. By fluorescence microscopy, monolayers incubated withherbimycin A or media alone exhibited continuous transcytoplasmicactin filaments and cell-to-cell apposition without intercellulargaps (Figure 5, A and B). After exposure to TSP for 6 h, isolatedellipsoid disruptions within the F-actin lattice occurred exclusivelyat the cell-cell interface (Figure 5C). In EC monolayers preincubatedwith herbimycin A for 16 h before and throughout the 6-h exposureto TSP, no intercellular gaps could be demonstrated (Figure 5D).Therefore, PTK inhibition blocked the TSP-induced formation ofintercellular gaps in these tightly confluent EC monolayers.

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Figure 5. Effect of PTK inhibition on TSP-induced intercellular gap formation. EC monolayers grown on filters were exposed for 6 h to media or TSP (30 µg/ml) in the presence or absence of herbimycin A (1.0 µM), the latter introduced 16 h before the addition of TSP. The monolayers were fixed, rendered permeable, stained with fluorescein-phalloidin, and examined by epifluorescence microscopy. (A) Medium control; (B) herbimycin A control; (C) TSP; (D) TSP + herbimycin A. Arrows in C indicate intercellular gaps. Magnification, 750×.

Immunolocalization of Phosphotyrosines in TSP-exposed EC

Because TSP-stimulated protein tyrosine phosphorylation appears necessary for intercellular gap formation and increases inalbumin flux, we asked whether phosphoproteins localized to cell-celljunctions might be involved. When EC monolayers were exposed toTSP (20 µg/ml) for either 10 min (Figure 6B) or 1 h (Figure 6D),and then probed with FITC-conjugated antiphosphotyrosine antibody,TSP-exposed EC displayed a fluorescence signal predominately restrictedto intercellular boundaries. In addition, plaque-like structureswere evident both at intercellular boundaries and, to a lesserdegree, throughout the cell bodies. In contrast, the control cellsprovided with media alone showed only relatively weak immunostainingfor phosphotyrosine-containing proteins (Figure 6, A and C). Thesedata suggest that TSP, after exposure times as brief as 10 min,preferentially stimulates tyrosine phosphorylation of proteinsthat are either enriched to or upon phosphorylation translocateto cell-cell junctions in confluent EC monolayers.

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Figure 6. Immunolocalization of phosphotyrosine-containing proteins in TSP-exposed ECs. ECs on filters were exposed for 10 min or 1 h to media or TSP (20 µg/ml), fixed, incubated with FITC-conjugated antiphosphotyrosine antibody, and analyzed by epifluorescence microscopy. (A) Medium control, 10 min; (B) TSP, 10 min; (C) medium control, 1 h; (D) TSP, 1 h. Arrowheads in B point to phosphotyrosine signal restricted to FA-like structures, and arrows in B and D point to phosphotyrosine signal restricted to intercellular boundaries of ECs exposed to TSP. Magnification, 750×.

TSP-induced Tyrosine Phosphorylation of EC Proteins

As a first step to determine which EC proteins might be tyrosine-phosphorylated in response to TSP, extracts obtained fromEC were processed for phosphotyrosine immunoblotting. Exposureof EC to a range of TSP concentrations for varying time intervalsdemonstrated no consistent increases in protein tyrosine phosphorylationin the absence of PTP inhibition; however, in the presence ofboth PTP inhibitors, vanadate (200 µM) and PAO (1.0 µM), exogenousTSP was clearly associated with increased tyrosine phosphorylationof EC proteins (Figure 7A). This was not as evident when onlyone PTP inhibitor was present. After an exposure of 1 h in thepresence of both vanadate (200 µM) and PAO (1.0 µM), TSP concentrationsas low as 1.0 µg/ml increased the phosphotyrosine signal as comparedwith the effect seen with vanadate and PAO alone; over a TSP rangeof 1-30 µg/ml, this increase in signal appears to be concentrationdependent (Figure 7B). TSP (20 µg/ml) in the presence of bothvanadate (200 µM) and PAO (1.0 µM) increased the phosphotyrosinesignal compared with the simultaneous vanadate/PAO control afterexposure times of 1 h [Figure 8A, compare (+) and ( $-$ ) lanes].After normalization to $beta$ -tubulin, one of the phosphotyrosine-containingbands (~66 kDa) was consistently increased as early as 0.5 h.Although the bands identified by the antiphosphotyrosine antibodyincreased over time in both the TSP-exposed and vanadate/PAO controlEC, at 1 h there was a greater signal in the cells that were incubatedwith TSP (Figure 8A). When ECs were exposed to equimolar concentrationsof 3 ECM proteins other than TSP (i.e., fibronectin, vitronectin,and type I collagen), protein tyrosine phosphorylation was notincreased compared with simultaneous controls (Young, unpublishedobservations). To determine whether PTP inhibition was requiredthroughout the TSP stimulus or only before cell lysis, ECs wereexposed to TSP (30 µg/ml) or media alone in the presence of PTPinhibition with vanadate and PAO only during the final 0.25 hof the incubation (Figure 8B). Under these conditions, the foldincrease of protein tyrosine phosphorylation (~10-fold) was greaterthan the TSP-induced fold increase detected with PTP inhibitionpresent throughout the TSP exposure ~2-fold (Figure 8, A and B).

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Figure 7. Concentration-dependent effect of TSP on tyrosine phosphorylation of EC proteins in the presence of PTP inhibition. ECs were exposed for 1 h to TSP or media alone with or without vanadate (200 µM), PAO (1.0 µM), or both. Cell lysates were resolved by SDS-PAGE and transferred to polyvinylidene difluoride membranes, and the blots were probed with antiphosphotyrosine IgG. (A) Phosphotyrosine-containing proteins in extracts of ECs exposed to TSP (20 µg/ml, 1 h) or media alone in the presence and absence of vanadate, PAO, or both. Arrows indicate bands with apparent Mr of 240,000, 205,000, 185,000, 135,000, 110,000, 95,000, and 66,000. (B) Phosphotyrosine-containing proteins in EC extracts obtained from monolayers exposed for 1 h to increasing concentrations of TSP in the presence of fixed concentrations of both vanadate (200 µM) and PAO (1.0 µM). To confirm equivalent protein loading, each blot was stripped and reprobed with anti- $beta$ -tubulin antibody. Molecular weights in kilodaltons are indicated on the left. Each is a representative blot of three experiments.

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Figure 8. Temporal effect of TSP on protein tyrosine phosphorylation in ECs. (A) ECs were exposed to TSP (20 µg/ml) (+) or media alone ( $-$ ) for increasing exposure times in the presence of fixed concentrations of both vanadate (200 µM) and PAO (1.0 µM) and were processed for detection of phosphotyrosine-containing proteins by immunoblotting as described in the legend to Figure 7. (B) ECs were exposed for 1 h to TSP (30 µg/ml) (+) or media alone ( $-$ ) in the presence of vanadate and PAO only during the last 0.25 h of the 1-h incubation and were processed for phosphotyrosine immunoblotting. To indicate protein loading, each blot was stripped and reprobed with anti- $beta$ -tubulin antibody. Molecular weights in kilodaltons are indicated on the left. These are representative blots of three experiments.

Effect of PTK Inhibitors on TSP-induced Protein Tyrosine Phosphorylation

ECs exposed to TSP (30 µg/ml) in the presence of vanadate and PAO with or without either herbimycin A or genistein were processedfor phosphotyrosine immunoblotting (Figure 3B). PTK inhibitionwith either herbimycin A or genistein decreased both basal andTSP-induced tyrosine phosphorylation of EC proteins. HerbimycinA decreased both the ~135 and ~66 kDa bands by >57%, whereas genisteindecreased each band by >60%. In addition, both herbimycin A andgenistein decreased the ~95 kDa band by >97%. Thus, these twoPTK inhibitors that protected against intercellular gap formationand loss of barrier function gained entry into ECs and diminishedTSP-induced protein tyrosinephosphorylation.

Identification of Tyrosine-phosphorylated Proteins in ECs Exposed to TSP

To further assess the response of ECs to TSP, we immunoscreened for proteins that comigrated with the phosphotyrosine-containingbands with apparent Mr of 135,000, 95,000, and 66,000 (Figure8B). FAK and p120^Cas comigrated with the ~135 kDa band, $beta$ - and $gamma$ -catenin with the~95 kDa band, and paxillin with the ~66 kDa band (Young, unpublishedobservations). Lysates from EC exposed for 1 h to TSP (30 µg/ml)or media alone in the presence of vanadate and PAO for the final0.25 h of the incubation were each immunoprecipitated with anti-FAK,anti-paxillin, anti- $beta$ -catenin, anti- $gamma$ -catenin, or anti-p120^Cas antibodies. The immunoprecipitates were processed for immunoblottingwith biotinylated antiphosphotyrosine (4G10) antibody (Figure9). As a control for any discrepancy in immunoprecipitation efficiencyand/or loading of the immunoprecipitated protein, blots were strippedand reprobed with the same immunoprecipitating antibody. Underthese conditions, TSP increased tyrosine phosphorylation of FAKapproximately fivefold, paxillin approximately eightfold, $gamma$ -cateninapproximately twofold, and p120^Cas approximately threefold. The studies of $beta$ -catenin were inconclusive.Other phosphoproteins that comigrate with the ~135, ~95, and ~66kDa bands have not been excluded. In addition, other phosphotyrosine-containingproteins seen in EC exposed to TSP that migrated with an apparentMr of 240,000, 205,000, 185,000, and 110,000 have not yet beenidentified (Figures 7 and 8).

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Figure 9. Identification of tyrosine-phosphorylated proteins in ECs exposed to TSP. ECs were incubated for 1 h with TSP (30 µg/ml) (+) or media alone ( $-$ ) in the presence of vanadate (200 µM) and PAO (1.0 µM) only during the last 0.25 h of incubation. ECs were lysed and immunoprecipitated with antibodies raised against FAK, paxillin, p120^Cas, or $gamma$ -catenin. The immunoprecipitates were resolved by SDS-PAGE and transferred to polyvinylidene difluoride membranes. The blots were probed with bio-tinylated-antiphosphotyrosine (4G10) antibody, incubated with HRP-conjugated streptavidin, developed with ECL, and subjected to laser densitometry. For normalization of phosphotyrosine signal to loading of the immunoprecipitated protein, blots were stripped and reprobed with the immunoprecipitating antibodies, i.e., anti-FAK, anti-paxillin, anti-p120^Cas, or anti- $gamma$ -catenin. IP, Immunoprecipitate; IB, immunoblot; IB*, immunoblot after stripping. These blots are representative of three experiments.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

In this report, we have demonstrated that TSP influences transendothelial flux of macromolecules through a paracellular pathway,the functional state of which appears to be regulated, in part,through protein tyrosine phosphorylation. The TSP-induced incrementsin transendothelial albumin flux were dose and time dependentand could not be ascribed solely to endotoxin contamination, TGF $beta$ activation, or EC injury. TSP was effective at concentrationsas low as 1.0 µg/ml (2.2 nM). The EC response to TSP (20 µg/ml)was demonstrable at $>=$ 2 h, with further time-dependent incrementsthat were not dependent on protein synthesis. PTK inhibitors,in concentrations that blocked TSP-induced EC protein tyrosinephosphorylation, protected against TSP-induced intercellular gapformation and increments in transendothelial ¹⁴C-BSA flux. In contrast, PTP inhibition enhanced TSP-induced barrierdysfunction. The increase in phosphotyrosine immunostaining inTSP-exposed EC was initially localized to FA-like structures andintercellular boundaries and, later, almost exclusively to areasof EC-EC contact. Finally, TSP-induced protein tyrosine phosphorylationwas clearly demonstrable in the presence of PTP inhibition. Severalphosphoproteins were identified as the adherens junction componentsFAK, paxillin, $gamma$ -catenin, and p120^Cas. The concentration and time requirements for TSP-induced increasesin protein tyrosine phosphorylation were compatible with the doseand time requirements for TSP-induced changes in barrier function.Collectively these data suggest that TSP perturbs the tight regulationof EC protein tyrosine phosphorylation/dephosphorylation, whichin turn directly/indirectly opens the paracellularpathway.

That TSP induces EC protein tyrosine phosphorylation and that PTK inhibition protects against the TSP-induced responses implicatesactivation of one or more EC PTKs. TSP is a multidomain moleculethat recognizes several EC surface receptors that have been coupledto tyrosine phosphorylation events, including CD36 (Bull et al.,1994), $alpha$ _v $beta$ ₃ (Blystone et al., 1996), and IAP (CD47) (Gao et al.,1996). When EC lysates were immunoblotted with an anti-CD36 antibodythat recognizes bovine CD36, no CD36 expression was detected.Furthermore, the synthetic peptide CSVTCG that interacts withCD36 (Bull et al., 1994), failed to either simulate or block theTSP effect (Young, unpublished observations). That these EC donot express CD36, nor do they respond to the CSVTCG motif in TSP,implicates a CD36-independent, tyrosine phosphorylation-dependentTSP response. In other preliminary experiments, an RGD-containingsequence that binds to the $alpha$ _v $beta$ ₃ integrin, and a binding motifin the COOH terminus that activates IAP, KRFVVMWKK (kindly providedby Dr. W. Frazier, Washington University, St. Louis, MO), eachalso failed to simulate or block the TSP effect (Young, unpublishedobservations). It is conceivable that for certain TSP-inducedEC responses, simultaneous or serial costimulation of multiplereceptors is required. In addition, TSP may mediate its biologicaleffects on EC barrier function and protein tyrosine phosphorylationthrough an as yet undefined sequence(s) and/orreceptor(s).

The state of tyrosine phosphorylation of adherens junction proteins is central to regulating cell-cell adhesion and endothelialbarrier integrity. Growth factor activation of receptor PTKs inducestyrosine phosphorylation of adherens junction proteins and cell-celladherens junction disassembly (Hoschuetzky et al., 1994; Shibamotoet al., 1994; Esser et al., 1998; Hazan and Norton, 1998). Thephosphotyrosine-containing proteins that we have now demonstratedin ECs exposed to TSP could be immunolocalized to the intercellularboundaries. Several nonreceptor PTKs are preferentially associatedwith the plasma membrane, including members of the src family(Tsukita et al., 1991; Matsuyoshi et al., 1992; Behrens et al.,1993; Hamaguchi et al., 1993). Src transformation increases tyrosinephosphorylation of cell-cell adherens junction proteins and diminishescadherin-dependent, homophilic adhesion (Matsuyoshi et al., 1992;Volberg et al., 1992; Behrens et al., 1993; Hamaguchi et al.,1993). Interestingly, PTK inhibition with herbimycin A also protectsagainst this loss of intercellular adhesion (Matsuyoshi et al.,1992; Hamaguchi et al., 1993). Therefore, nonreceptor PTKs mayindependently or in concert with a receptor PTK mediate the ECresponse to the TSPstimulus.

That TSP-induced tyrosine phosphorylation of EC proteins was consistently observed only in the presence of PTP inhibition,and that PTP inhibition enhanced TSP-induced barrier dysfunction,implicates the participation of one or more PTPs. PTPs play acrucial role in regulating protein tyrosine phosphorylation ofadherens junctions (Volberg et al., 1992; Brady-Kalnay et al.,1995; Fuchs et al., 1996). Receptor PTP activity increases duringcontact inhibition of cultured cells in vitro (Gaits et al., 1995;Southey et al., 1995; Fuchs et al., 1996). In ECs, the activationof the receptor PTP, HPTP $beta$ , increases 12-fold as cells progressto confluence (Gaits et al., 1995). Two receptor PTPs that belongto the immunoglobulin superfamily, PTPµ (Brady-Kalnay et al.,1995) and PTP_k (Fuchs et al., 1996), each localize to cell-celladherens junctions, directly bind ZA component proteins, and participatein homophilic cell-cell adhesion. That PTP inhibition unmasksTSP-induced tyrosine phosphorylation and enhances loss of barrierfunction is compatible with these findings. In fact, others haveshown that previous PTP inhibition with vanadate is necessaryto observe tyrosine phosphorylation of EC-EC adherens junctionproteins (Lampugnani et al., 1997). In another study, microspikeformation induced by TSP became more prominent in pervanadate-treatedcells (Adams, 1995). This requirement for PTP inhibition may explainwhy tyrosine phosphorylation events in ECs have not been easilyrecognized in response to the TSPstimulus.

TSP induces tyrosine phosphorylation of multiple EC proteins with an apparent Mr of 240,000-66,000. We now have identifiedtwo substrates for TSP-induced tyrosine phosphorylation in ECsas the FA component proteins FAK and paxillin (Clark and Brugge,1995; Parsons and Parsons, 1997). These proteins participate insignaling pathways that regulate the state of FA assembly andcell-substrate adhesion. Tyrosine phosphorylation of both FAKand paxillin can occur through either ECM protein-integrin interactions(Burridge et al., 1992) and/or through Rho-A-dependent stressfiber formation and FA assembly (Chrzanowska-Wodnicka et al.,1996). Interestingly, several other established mediators of increasedvascular permeability, including bradykinin (Leeb-Lundberg etal., 1994), platelet-activating factor (Soldi et al., 1996), $alpha$ -thrombin(Schaphorst et al., 1997), and vascular endothelial growth factor(Abedi and Zachary, 1997), also stimulate tyrosine phosphorylationof FAK and paxillin. In addition, others have demonstrated thatenhanced spreading of human melanocytes in response to the TSPstimulus correlates with tyrosine phosphorylation of FAK, paxillin,and a 90-kDa protein (Gao et al., 1996). Tyrosine phosphorylationof FAK and paxillin facilitates their interactions with src homolgy-2-bearingproteins and promotes downstream signaling events. Whether TSP-inducedchanges in barrier function are mediated through these protein-proteininteractions and signaling pathways remains to bedetermined.

Two other identified substrates for TSP-induced tyrosine phosphorylation are $gamma$ -catenin (or plakoglobin) and p120^Cas. $gamma$ -Catenin, which is homologous to $beta$ -catenin, and p120^Cas are both part of the cell-cell adherens junction (ZA) complex(Kemler, 1993; Gumbiner, 1996; Barth et al., 1997). The ZA isresponsible for mediating actin-dependent, homophilic cell-celladhesion through its transmembrane receptors, the cadherins. InECs, $gamma$ -catenin and $beta$ -catenin each independently couple the EC-specific,vascular endothelial-cadherin to the actin cytoskeleton throughtheir interactions with $alpha$ -catenin (Lampugnani et al., 1995). While $beta$ -catenin associates with vascular endothelial-cadherin in newlyformed and loosely adherent EC junctions, $gamma$ -catenin predominatesin tightly confluent EC-EC junctions (Lampugnani et al., 1997).Tyrosine phosphorylation of ZA protein components reduces intercellularEC-EC adhesion (Esser et al., 1998) and disrupts the linkage betweencadherin and the actin cytoskeleton (Balsamo et al., 1995; Hazanand Norton, 1998). Tyrosine phosphorylation of $gamma$ -catenin, $beta$ -catenin,and p120^Cas induced by ligand occupancy of the epidermal growth factor receptordiminishes cell-cell adhesion through disruption of the cadherin-actincytoskeletal linkage (Hazan and Norton, 1998). Thus, tyrosinephosphorylation of $gamma$ -catenin and p120^Cas may directly contribute to TSP-induced opening of the paracellularpathway.

The relationship between TSP-induced opening of the endothelial paracellular pathway and tyrosine phosphorylation of bothFA and ZA component proteins remains to be determined. That TSPinduces tyrosine phosphorylation of proteins associated with bothadherens junctions is suggestive of intracellular cooperativitybetween both the FA and ZA. To what extent the state of assemblyof either adherens junction is influenced by the other is unclear.Recently, we have demonstrated that another counteradhesive protein,SPARC (secreted protein acidic and rich in cysteine), also inducestyrosine phosphorylation of adherens junction and possibly otherEC proteins, some of which migrate with similar molecular weights(Young et al., 1998). One could speculate that these two structurallydissimilar but functionally related counteradhesive proteins bothinduce tyrosine phosphorylation of common substrates. Whetherthese two counteradhesive proteins regulate EC-EC homophilic adhesionthrough a common tyrosine phosphorylation-dependent signalingpathway isunclear.

TSP is operative over a wide range of complex intercellular interactions. Understanding the mechanism(s) through which TSPinfluences homotypic EC-EC adhesion as well as EC shape changesand migration has implications for vasculogenesis, tissue morphogenesis,and fetal development (O'Shea et al., 1990; O'Shea and Dixit,1998), as well as angiogenesis (Taraboletti et al., 1990; Iruela-Arispeet al., 1991), within the context of wound healing (Munjal etal., 1990; DiPietro et al., 1996), tissue remodeling (Botney etal., 1992; Kuhn and Mason, 1995), and tumor cell survival (Roberts,1996). TSP also promotes leukocyte and tumor cell motility invitro (Taraboletti et al., 1987; Mansfield et al., 1990) and modulatestumor cell adhesion to ECs (Incardona et al., 1995). Therefore,this same TSP-responsive paracellular pathway might also accommodatemigrating leukocytes and/or metastatic tumor cells. TSP has beenidentified as a counteradhesive protein that disrupts cell-ECMinteractions. In this study, we have presented evidence for themodulation of EC-EC adhesion by TSP through a pathway dependenton protein tyrosinephosphorylation.

	ACKNOWLEDGMENTS

We thank Mr. Antonio Pallero for excellent technical assistance and Ms. Shirley Taylor for excellent secretarial support.This work was supported in part by the Office of Research andDevelopment, Department of Veterans Affairs (S.E.G.), the U.S.Army Medical Research and Development Command (grant DAMD17-94-J-4117)(S.E.G.), and grants DK-48373 (S.E.G.), HL-44575 (J.E.M.-U.),and HL-50061 (J.E.M.-U.) from National Institutes of Health. J.E.M.-U.is an Established Investigator of the American Heart Association(AHA-Genentech Special Awardie in Thrombosis) (grant 9640228N).B.A.Y. is a recipient of a Department of Defense AugmentationAward for Science and Engineering Research Training(AASERT).

	FOOTNOTES

Correspondingauthor.

These authors contributed equally to thismanuscript.

ABBREVIATIONS

Abbreviations used: EC, endothelial cell; FA, focal adhesion; FAK, focal adhesion kinase; IAP, integrin-associated protein; LPS, lipopolysaccharide; PAO, phenylarsine oxide; PMB, polymixin B; PTK, protein tyrosine kinase; PTP, protein tyrosine phosphatase; sTSP, stripped thrombospondin-1; TSP, thrombospondin-1; ZA, zonula adherens.

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TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERNCES

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