Caveolin-1 regulates shear stress-dependent activation of extracellular signal-regulated kinase

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Caveolin-1 regulates shear stress-dependent activation of extracellular signal-regulated kinase

Heonyong Park¹, Young-Mi Go¹, Ritesh Darji¹, Jong-Whan Choi¹, Michael P. Lisanti², Matthew C. Maland¹, and Hanjoong Jo¹

¹ Department of Pathology, University of Alabama at Birmingham, Birmingham, Alabama 35294; and ² Department of Molecular Pharmacology, Albert Einstein College of Medicine, Bronx, New York 10461

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Fluid shear stress activates a member of the mitogen-activated protein (MAP) kinase family, extracellular signal-regulatedkinase (ERK), by mechanisms dependent on cholesterol in the plasmamembrane in bovine aortic endothelial cells (BAEC). Caveolae aremicrodomains of the plasma membrane that are enriched with cholesterol,caveolin, and signaling molecules. We hypothesized that caveolin-1regulates shear activation of ERK. Because caveolin-1 is not exposedto the outside, cells were minimally permeabilized by Triton X-100(0.01%) to deliver a neutralizing, polyclonal caveolin-1 antibody(pCav-1) inside the cells. pCav-1 then bound to caveolin-1 andinhibited shear activation of ERK but not c-Jun NH₂-terminal kinase.Epitope mapping studies showed that pCav-1 binds to caveolin-1at two regions (residues 1-21 and 61-101). When the recombinantproteins containing the epitopes fused to glutathione-S-transferase(GST-Cav^1-21 or GST-Cav^61-101) were preincubated with pCav-1, only GST-Cav^61-101 reversed the inhibitory effect of the antibody on shear activationof ERK. Other antibodies, including m2234, which binds to caveolin-1residues 1-21, had no effect on shear activation of ERK. Caveolin-1residues 61-101 contain the scaffolding and oligomerization domains,suggesting that binding of pCav-1 to these regions likely disruptsthe clustering of caveolin-1 or its interaction with signalingmolecules involved in the shear-sensitive ERK pathway. We suggestthat caveolae-like domains play a critical role in the mechanosensingand/or mechanosignal transduction of the ERKpathway.

blood flow; vascular biology; atherosclerosis

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

VASCULAR ENDOTHELIAL CELLS recognize shear stress through unknown mechanosensing system(s) and respond both acutely and chronicallyby producing autocrine and paracrine factors (7). Through theseendothelial responses, shear stress controls vascular tone, vesselwall remodeling, binding of blood cells to endothelium, and hemostasis(7). Shear stress selectively and differentially regulatesexpression of many genes that are important in the pathophysiologyof vessel wall function (see Refs. 4 and 9 for reviews).Furthermore, a conserved cis-acting shear stress-response elementhas been identified in many shear-sensitive genes including platelet-derivedgrowth factor-B, intracellular adhesion molecule-1, tissue plasminogenactivator, and transforming growth factor $beta$ -1, suggesting itsbroad implication in shear-dependent regulation of gene expression(4, 9, 20, 29). An additional cis-acting element, thephorbol ester 12-O-tetradecanoylphorbol 13-acetate-responsiveelement, has been found in the monocyte chemoattractant protein-1gene (37). Shear stress also transiently activates transcriptionfactors [nuclear factor- $kappa$ B (NF- $kappa$ B), AP-1, and early growth response-1]and immediate-early response genes (c-fos, c-jun, and c-myc) thatare involved in the regulation of shear-dependent gene expression(13, 20, 21, 36, 37). Induction of specific genes byshear stress in endothelial cells is mediated by activation ofmechanosensitive signaling pathways that include at least threemembers of the mitogen-activated protein (MAP) kinase family,extracellular signal-regulated kinase (ERK1/2), c-Jun NH₂-terminalkinase (JNK), and Big MAP kinase 1 (also called ERK5) (2, 18,23, 36, 43, 47). MAP kinases are important signaling componentslinking extracellular stimuli to cellular responses such as cellgrowth, death, differentiation, and metabolic regulation (5,19).

Shear stress activates ERK in a rapid and transient manner (maximum by 5 min and returning to basal levels by 30 min of shearexposure), whereas JNK activation occurs over a much slower andprolonged time course (requiring at least 30 min and returningto basal levels after 1 day of shear exposure) (18). Shear stressactivates the two MAP kinases by distinct signaling pathways:activation of ERK is mediated by mechanisms involving G $alpha$ _i-2, proteinkinases [Src, focal adhesion kinase (FAK), and protein kinaseC- $epsilon$ ], and Ras, whereas JNK activation requires G $beta$ / $gamma$ , phosphatidylinositol-3-kinase- $gamma$ ,tyrosine kinases (Src and FAK), and Ras (11, 14, 16, 18,22, 42). How do endothelial cells ensure the specific activationof each pathway when sharing the same common signaling molecules(e.g., Src, FAK, and Ras)? A likely hypothesis is that spatialcompartmentalization of signaling molecules into microdomainsprovides the mechanism for the differential activation of ERKand JNK. In support of this hypothesis, we (28) and Rizzo etal. (30) have independently shown that the cholesterol-sensitivemicrodomains in the plasma membrane play a critical role in mechanosensitiveactivation of ERK, but not JNK, in bovine aortic endothelial cells(BAEC) and in perfused rat lung endothelium (28, 30). At presentthe underlying molecular mechanisms and morphological understandingby which cholesterol-sensitive microdomains segregate signalingmolecules and elicit selective regulation of the MAP kinases inresponse to shear stress are not known. However, caveolae andcaveolae-like domains including "raft" and "glycosphingolipidsignaling domains" are the likely candidates (1, 15, 27,30, 38).

Caveolae are noncoated micropatches of the plasma membrane with a variety of shapes (flat, invaginated, and tubular) and arefound in most cell types including endothelial cells, fibroblasts,smooth muscle cells, and adipocytes (1, 27). Caveolae serveat least two different functions: 1) transport of large and smallmolecules (transcytosis of macromolecules and potocytosis of ionsand folate) and 2) transmembrane signaling microdomains (1,27). Caveolae are enriched with cholesterol, glycosphingolipids,lipid-anchored signaling molecules, and caveolin (1, 27).

Caveolin, a 21- to 24-kDa membrane protein, is a principal component of caveolae and also binds directly to cholesterol andinteracts with such signaling molecules as G protein $alpha$ -subunits,Ras, Src family kinases, and the endothelial form of nitric oxidesynthase (eNOS) (8, 25, 27). Three members (caveolin-1,-2, and -3), including two isoforms (caveolin-1 $alpha$ and -1 $beta$ ), ofthe caveolin gene family in mammalian cells have been cloned (32,33, 40). Caveolin-1 is abundantly expressed in endothelialcells (35), whereas caveolin-3 is expressed only in muscle cells(40). The tissue distribution of caveolin-2 has been shown tobe similar to that of caveolin-1 (32). Caveolins are composedof NH₂- and COOH-terminal domains linked by a hairpinlike membrane-spanningdomain. Therefore, both the NH₂ and COOH terminals face cytoplasm(see Fig. 1 for a schematic representation; see also Ref. 27).Caveolin-1 self-oligomerizes or binds caveolin-2 to form homo-or heterooligomers (27). The NH₂-terminal domain of caveolin-1contains the oligomerization domain (residues 61-101) and thescaffolding domain (residues 81-101) (see Fig. 1 and Ref. 39).The oligomerization domain is the region involved in homooligomerizationof caveolin-1, whereas the signaling molecules present in caveolaesuch as G_i-2, Ras, Src, and eNOS bind to the scaffolding domainof caveolin-1 and are held in the inactive state (27, 39).

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Fig. 1. Construction of glutathione-S-transferase (GST)-caveolin fusion proteins. Schematic diagram shows primary structure (NH₂ and COOH terminals and membrane-spanning region) and functional domains (scaffolding domain: amino acids 82-101; oligomerization domain: amino acids 61-101) of caveolin-1 as previously proposed (25). Full-length (amino acids 1-178) and portions of caveolin-1 that were amplified by PCR and subcloned into the pGEX-4T-1 vector (29) were expressed in Escherichia coli, affinity purified using glutathione-agarose, and dialyzed against PBS.

In this study we examined the role of caveolin-1 in shear stress-dependent activation of ERK by delivering caveolin antibodiesinto mildly permeabilized endothelial cells in an attempt to blockthe shear response. Moreover, by using the recombinant glutathione-S-transferase(GST) fusion proteins containing the epitopes of the caveolin-1-recognizingcaveolin antibodies, this study determined the critical role ofthe scaffolding and oligomerization domains (residues 61-101)of caveolin-1 in shear-dependent activation ofERK.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cell culture and antibody treatment in permeabilized cells. BAEC obtained from descending thoracic aortas were maintained in a growth medium [DMEM (1 g/l glucose; Life Technologies)containing 20% fetal bovine serum (FBS; Atlanta Biologicals) withoutantibiotics] at 37°C and 5% CO₂ (17). Cells used in this studywere between passages 3 and 10. For shear stress experiments,one million cells per glass slide (75 × 38 mm; Fisher) were seededin growth medium. The next day the medium was changed to a shearmedium (phenol red-free DMEM containing 0.5% FBS and 25 mM HEPES)and incubated for 18 h. Polyclonal (pCav-1) and monoclonal caveolin-1antibodies (clones 2234, 2297, C060, and C20B) and monoclonalcaveolin-2 antibodies (clone 65) were purchased from TransductionLaboratories. A polyclonal antibody raised against canine caveolin-2was kindly provided by Dr. Kai Simons (31). BAEC were incubatedwith 0-2.5 µg/ml antibodies at 37°C in the starvation medium containing0.01% Triton X-100 for 30 min. Treated cells were then exposedto shear stress or static control in fresh, detergent-free starvationmedium. In some studies pCav-1 was preincubated for 2 h with theGST-caveolin fusion proteins containing caveolin residues 1-21(GST-Cav^1-21) or 61-101 (GST-Cav^61-101) (see Fig. 1 and Ref. 33) to block the binding of the antibodyto the epitopes of endogenous caveolin-1 in endothelial cells.The mixtures of pCav-1 antibody and GST-caveolins were then addedto BAEC in the presence of Triton X-100 and subjected to shearstress.

Shear stress studies. The glass slide containing a confluent monolayer of BAEC was assembled into a parallel plate shear chamber forming a flowchannel (220 µm high × 25 mm wide × 62 mm long) between the monolayerand a polycarbonate plate as described previously (18). Nonpulsatilelaminar shear stress was controlled by changing the flow rateof the starvation medium delivered to the cells using the constanthead flow loop or a syringe pump (KD Scientific) as described(18).

Preparation of cell lysates. After being exposed to shear stress, cells were washed in ice-cold PBS, scraped in 0.25 ml of lysis buffer [50 mM HEPES, pH7.4, 150 mM NaCl, 1 mM vanadate, 1 mM dithiothreitol (DTT), 1.0%Triton X-100, and 0.1 mM phenylmethylsulfonyl fluoride], and solubilizedfor 15 min to prepare Triton-soluble lysate as described (18).Entire solubilization procedures were performed at 4°C, and theprotein content of soluble cell lysates was measured using a Bio-RadDC assay kit (Bio-Rad).

Determination of ERK activation by Western blot analysis. Soluble lysates (10 µg each) were resolved by 10% SDS-PAGE, transferred to a polyvinylidene difluoride (PVDF) membrane (Millipore),and probed with an antibody specific to phosphorylated forms ofERK1/2 (pERK1/2) (New England Biolabs) to determine the activationstatus of the MAP kinase as described (18). As a control, thetotal amount of ERK1/2 was determined by Western blot analysisusing an ERK1 antibody that also cross-reacts with ERK2 (UBI)(18). Goat anti-rabbit IgG conjugated to alkaline phosphatasewas used as a secondary antibody, and the membrane was developedusing a method for chemiluminescent detection (18).

Immune complex assay for JNK1. Activity of JNK1 was measured by an immune complex kinase assay using an antibody specific for JNK1 (clone G151-333; Pharmingen)and c-Jun (amino acids 5-89) fused to GST (GST-c-Jun) as the substrate,as described (18). Briefly, Triton-soluble cell lysates (100µg each) were incubated with JNK1 antibody (0.25 µg) for 1 h at4°C, followed by an additional 1 h of incubation with proteinG-agarose. The immune complex was washed four times in the lysisbuffer and twice in buffer A (20 mM HEPES, pH 7.6, 20 mM MgCl₂,20 mM $beta$ -glycerophosphate, 20 mM p-nitrophenyl phosphate, 0.1 mMvanadate, and 2 mM DTT). The washed immune complexes were incubatedin 20 µl of buffer A containing GST-c-Jun (5 µg each), 20 µM ATP,and 5 µCi of [ $gamma$ -³²P]ATP for 20 min at 30°C. The reaction was terminated by boilingin 5× Laemmli sample buffer, resolved by 10% SDS-PAGE, and electrotransferredto a PVDF membrane. Autoradiographs were obtained from the driedblot, and radioactivity incorporated into GST-c-Jun was quantitatedby cutting and counting each band in a scintillationcounter.

Purification and immunoprecipitation of GST-caveolin fusion proteins. Construction of GST-fusion proteins containing the full length or fragments of caveolin-1 (see Fig. 1) from Escherichia colilysates and purification of the recombinant fusion proteins byglutathione-agarose affinity chromatography were described previously(33). For immunoprecipitation studies, 20 µg of GST-Cav (dialyzedin PBS before use) were incubated for 2 h at 4°C with 0.5 µg ofpCav-1 in PBS, followed by an additional 1 h of incubation withprotein A-agarose. Immune complexes were washed three times withthe lysis buffer, boiled in Laemmli sample buffer, resolved by12.5% SDS-PAGE, and analyzed by Coomassie blue staining and byWestern blotting using a monoclonal anti-GST antibody (SantaCruz).

Immunocytochemistry. BAEC grown on glass slides were incubated with 1 µg of pCav-1 or 1 µg of nonimmune (NI)-IgG in the presence or absence of0.01% Triton X-100 for 30 min at 37°C as described in Cell cultureand antibody treatment in permeabilized cells. Cells were washedthree times in ice-cold PBS to remove unbound antibodies and werethen fixed in 4% paraformaldehyde and 0.1% glutaraldehyde for30 min and blocked (2% BSA, 10% goat serum, and 0.1% Triton) for1 h. Bound antibodies were detected by using a secondary antibody(Cy3-conjugated goat anti-rabbit IgG) for 30 min. Cells were mountedwith Slow-Fade and examined using an Olympus fluorescence microscope.Fluorescence intensity of stained cells was quantitated by animage analysis program (ESPRIT) as described (10).

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

pCav-1 is delivered into permeabilized BAEC and binds to caveolin-1. When BAEC were incubated for 30 min with pCav-1 in the presence of 0.01% Triton X-100 (minimal permeabilization), the antibodywas detected inside virtually all treated cells (Fig. 2, B andC). Delivery of the pCav-1 antibody into the cells required thepresence of the detergent, because the antibody was not detectedin cells incubated without Triton X-100 (Fig. 2E). When NI-IgGwas used as a control in Triton-permeabilized cells, the fluorescentsignal was very faint, indicating that the IgG did not bind tightlyto the cells and was mostly removed by extensive washing (Fig.2D). The staining of pCav-1 showed a punctate pattern (Fig. 2C),which is consistent with its reported intracellular localizationin the plasma membrane and Golgi apparatus (33). The characteristicpunctate staining pattern of pCav-1 was also observed when BAECwere fixed first and subsequently permeabilized with the use ofa high concentration of Triton X-100 (0.1%) before cells wereincubated with pCav-1 followed by the secondary antibody (Fig.2A, positive control).

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Fig. 2. Delivery of polyclonal caveolin-1 antibody (pCav-1) into permeabilized bovine aortic endothelial cells (BAEC). A: positive control. BAEC were first fixed in paraformaldehyde and glutaraldehyde, highly permeabilized (0.1% Triton X-100 for 30 min), and blocked for 1 h before being incubated with pCav-1. B-E: unlike control shown in A, cells were not fixed and highly permeabilized before antibody was added. Instead, cells were incubated with 1 µg/ml pCav-1 (B, C, and E) or nonimmune (NI)-IgG (D) in presence (B, C, and D) or absence (E) of 0.01% Triton X-100 for 30 min at 37°C. Cells were then washed in PBS and fixed in paraformaldehyde and glutaraldehyde. pCav-1 and NI-IgG were identified by incubation with Cy3-conjugated goat anti-rabbit IgG for 30 min. Fluorescence micrographs (A and B: original magnification, ×500; C-E: original magnification, ×2,5000; C is a higher magnification of B) are representative of at least 3 independent experiments.

To estimate what percentage of total caveolin-1 is bound to the pCav-1 antibody in minimally permeabilized cells, its stainingintensity was compared with that of the positive control groupby quantitative fluorescence microscopy. Assuming that the fluorescenceintensity of pCav-1 staining in positive control cells (prefixedand highly permeabilized cells, Fig. 2A) is 100% (total immunoreactivecaveolin-1), 6.8 ± 0.4% (n = 99) of total caveolin-1 bound tothe antibody in minimally permeabilized cells (compare Fig. 2,A and B). These results show that pCav-1 was delivered insidevirtually all minimally permeabilized cells and also suggest thatit bound to a fraction of the total caveolin-1.

To confirm the binding of pCav-1 to caveolin-1 in permeabilized cells, BAEC were incubated with the antibody in the presenceof Triton for increasing periods of time and washed with PBS.Cell lysates were then incubated with protein A-agarose to retrievethe pCav-1-caveolin-1 complex. Western blot analysis showed thatthe immune complex contained both the heavy chain of pCav-1 (pCav-1IgG-H) and caveolin-1 only when cells were incubated with pCav-1and Triton for 30 min (Fig. 3). Taken together, the results shownin Figs. 2 and 3 confirm that the pCav-1 antibody was deliveredto the cells and bound to caveolin-1 in minimally permeabilizedBAEC.

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Fig. 3. Binding of pCav-1 to caveolin-1 in permeabilized BAEC. BAEC were treated with pCav-1 (2.5 µg/ml) in presence of 0.01% Triton X-100 for up to 30 min at 37°C. Cells were then washed with PBS and lysed in a buffer containing 1% Triton X-100. Cell lysates were incubated with protein A-agarose to immunoprecipitate the antibody-caveolin-1 complex. Top: immune complexes were resolved by 10% SDS-PAGE, transferred to a polyvinylidene difluoride membrane, cut in half, and analyzed by Western blots with a goat anti-rabbit antibody (top of membrane) to identify pCav-1 delivered into cells. Bottom of membrane was probed with a caveolin-1 antibody (m2297) and subsequently with a goat-anti-mouse antibody. Note that the heavy chain of pCav-1 (IgG-H at ~55 kDa) and caveolin-1 (Cav-1 at 22-24 kDa) were immunoprecipitated only from cells that were incubated for 30 min with antibody and Triton X-100. Results are representative of 3 independent experiments.

pCav-1 inhibits shear stress-dependent activation of ERK, but not JNK, in Triton-permeabilized BAEC. To investigate whether the pCav-1 antibody inhibits shear-dependent activation of ERK, cells were pretreated with the antibodyin the presence of Triton before being subjected to shear stress.As we showed previously (28), permeabilization of BAEC by lowconcentrations of Triton has no significant effect on shear-dependentactivation of ERK (Fig. 4, A and C). However, when cells wereincubated with pCav-1 in the presence of Triton (minimally permeabilized),shear stress-dependent activation of ERK was inhibited in an antibodyconcentration-dependent manner, whereas NI-IgG had no effect (Fig.4, A and C). The inhibitory effect of pCav-1 on the shear activationof ERK was not observed if cells were not Triton permeabilized(Fig. 4B). Although pCav-1 appeared to have a small effect instatic controls of nonpermeabilized cells in some studies, itseffect was not statistically significant (Fig. 4, B and C).

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Fig. 4. pCav-1 inhibits shear-dependent activation of extracellular signal-regulated kinase (ERK). BAEC were incubated with increasing amounts of pCav-1 or NI-IgG in presence (A) or absence (B) of 0.01% Triton X-100 for 30 min at 37°C. Cells were then subjected to static control or shear stress (10 dyn/cm² for 5 min) in fresh shear medium without Triton. Cell lysates were analyzed by Western blots with antibodies specific to total ERK1/2 or phospho-ERK1/2 (pERK1/2). C: data for line graph are means ± SE (n = 3) obtained from densitometric quantitation of pERK1 bands. Ab, antibody. *P < 0.05.

Our previous report (28) showed that removal of cholesterol from the plasma membrane selectively inhibits shear-dependentactivation of ERK without affecting that of JNK. This findingsuggested that the cholesterol-sensitive, caveolae-like domainsspecifically mediate the shear-sensitive ERK pathway, but notJNK. This hypothesis was further tested in this study by determiningwhether pCav-1 inhibits shear-dependent activation of JNK. Tothis end, we treated BAEC with pCav-1 in the presence of Tritonbefore exposing cells to static conditions or shear stress. Consistentwith our previous report (28), Triton permeabilization of BAECdid not alter basal or shear-dependent activation of JNK (Fig.5). Furthermore, treatment of cells with pCav-1 or NI-IgG hadno effect on shear-dependent activation of JNK. Together, thecurrent and previous findings (28) show that shear-dependentactivation of JNK is regulated by mechanisms independent of caveolin-1and plasma membrane cholesterol.

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Fig. 5. pCav-1 has no effect on shear-dependent activation of c-Jun NH₂-terminal kinase (JNK). BAEC were pretreated without or with pCav-1 (2.5 µg/ml) or NI-IgG (2.5 µg/ml) and 0.01% Triton X-100 for 30 min, followed by exposure to static control or shear stress (10 dyn/cm² for 1 h) and preparation of cell lysates. JNK activity was determined by phosphorylation of GST-cJun using immunoprecipitated JNK1. Top: results of Western blot obtained using a JNK antibody (JNK blot) showing that similar amounts of JNK1 were immunoprecipitated in each lane. A representative autoradiograph shows phosphorylation of GST-cJun. Bottom: radioactivity of each band was quantitated by scintillation counting, and means + SE (n = 3) are shown on bar graph.

The specific effect of pCav-1 on shear-dependent activation of ERK. To determine whether caveolin-1 antibodies other than pCav-1 could also block ERK activation in response to shear stress,we screened additional caveolin-1 antibodies. For this study,cells were incubated with three monoclonal antibodies specificto caveolin-1, m2297 (the epitope 61-71 residues, a part of theoligomerization domain), m2234 (the epitope 1-21 residues), andC20B (an antibody raised against the whole molecule), in minimallypermeabilized cells as described in Fig. 3. The pCav-1 antibodyand NI-IgG were also used as positive and negative controls, respectively.First, the ability of various caveolin-1 antibodies to bind caveolin-1under our minimally permeabilized conditions for 30 min was determinedby immunoprecipitation. For this study, minimally permeabilizedand antibody-treated cells were lysed in 60 mM octylglucosidebuffer (1 h at 4°C), and protein G-agarose was added to the celllysates. Immunoprecipitates were subsequently probed by Westernblot using the m2297 antibody as shown in Fig. 6A. To aid in quantifyingthe amount of caveolin-1 immunoprecipitated by each antibody,we directly used an aliquot of the lysate in the Western blotstudies. As shown in Fig. 6A, the m2234 and pCav-1 antibodiesimmunoprecipitated 30 ± 2% (n = 3) and 2.7 ± 0.2% (n = 5) of totalcaveolin-1, respectively. These results suggest that both m2234and pCav-1 bind to the native form of caveolin-1 and are consistentwith previous reports (26, 33). In contrast, the m2297 andmC20B antibodies and NI-IgG did not immunoprecipitate any significantamount of caveolin-1 from cell lysate (Fig 6A). However, m2297and mC20B work well in Western blot analysis (see Figs. 3 and6 as well as unpublished results from Transduction Lab describedin DISCUSSION), suggesting that these antibodies recognize denatured,but not native, caveolin-1.

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Fig. 6. Specificity of caveolin-1 antibodies on shear-dependent activation of ERK. BAEC were incubated without (none) or with 2.5 µg/ml caveolin-1 antibodies (m2297, m2234, C20B, or pCav-1) or NI in presence of 0.01% Triton X-100 for 30 min. A: to determine amount of caveolin-1 that can be immunoprecipitated by each antibody, cells were lysed in $beta$ -octylglucoside (60 mM), and lysates (200 µg each) were used for immunoprecipitation with protein G-agarose for 1 h at 4°C. Each immunoprecipitate was analyzed by Western blot analysis with m2297. Also, lysate (10 µg) was used to determine total amount of caveolin-1. B: after treatment with caveolin antibodies and minimum permeabilization, cells were exposed to static control ( $-$ ) or shear stress (+). Activation of ERK was then determined by Western blot analysis with a pERK antibody (pERK1/2) and quantitated densitometrically as described in Fig. 3. Data in bar graph are means ± SE (n = 3). *P < 0.05.

Next, the effects of each antibody on shear stress-dependent activation of ERK were determined. As shown in Fig. 6B, onlypCav-1 inhibited shear activation of ERK, whereas m2297, m2234,mC20B, and NI-IgG did not have any significant effect on eitherthe basal or shear-dependent activation of ERK. Because m2297and mC20B could not immunoprecipitate appreciable amounts of caveolin-1(Fig. 6A), the effects of these antibodies on shear activationof ERK may be due to their inability to bind caveolin-1 in minimallypermeabilized BAEC. However, it is interesting to note the remarkabledifference between the two antibodies (m2234 and pCav-1) thatare capable of immunoprecipitating caveolin-1. Whereas m2234 bound30% of total caveolin-1 (Fig. 6A), it did not have any effecton the shear activation of ERK (Fig. 6B). In contrast, pCav-1immunoprecipitated 3% of total caveolin-1 (Fig. 6A) while inhibitingthe shear-dependent activation of ERK by 89% of control [Fig.6B, compare lane 2 (544 ± 72% of static control) with lane 12(153 ± 6.9% of static control), n = 3 each]. This result demonstratesthat the effect of Cav-1 antibodies on the shear activation ofERK is not related simply to the affinity or the amount of caveolin-1bound to antibodies. In addition, the m2234 (epitope 1-21 residues)result shows that the pCav-1 antibody effect on shear activationof ERK may not be explained by caveolin residues 1-21, at leastnotalone.

Epitope mapping of pCav-1. The pCav-1 antibody was raised against the NH₂-terminal domain (1-101) of caveolin-1, but its epitopes have not been determined.To determine the amino acid residues of caveolin-1 that are recognizedby pCav-1 in a nondenatured state, we used the recombinant GSTfusion proteins containing various fragments of caveolin-1 inimmunoprecipitation studies. The recombinant GST-caveolins wereproduced in E. coli and purified by glutathione-agarose, and itspurity was determined by protein staining (Fig. 7A). When pCav-1was added to various GST-caveolins, only the fusion proteins containingeither residues 1-21 or 61-101 were immunoprecipitated (Fig. 7B).In contrast, the m2234 antibody immunoprecipitated the fusionproteins containing residues 1-21 but not residues 61-101 (Fig.7C). The epitope 1-21 that recognizes m2234 in a nondenaturedstate is the same as that previously reported using denaturedand reduced caveolin-1 in Western blot analysis (33).

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Fig. 7. Epitope mapping of caveolin-1 antibodies. Full-length (1-178) and portions (amino acid residue numbers shown above each lane) of caveolin-1 were recombinantly expressed as GST-fusion proteins as described in Fig. 1. A: Coomassie blue staining of purified caveolin fusion proteins. B and C: GST-caveolin fusion proteins were incubated with either pCav-1 (B) or a monoclonal caveolin-1 antibody (m2234) (C) overnight at 4°C and subsequently with Protein A- or G-agarose for 1 h. Washed immunoprecipitates (IP) were then analyzed by Western blot analysis using an antibody specific to GST ( $alpha$ GST). Note that pCav1 recognizes 2 epitopes within caveolin-1 residues 1-21 and 61-101, whereas m2234 binds to 1-21.

The inhibitory effect of pCav-1 can be prevented by preabsorption with the recombinant fusion protein GST-Cav^61-101. The study of epitope mapping of pCav-1 (Fig. 7) showed that two epitopes in caveolin-1 bind to pCav-1: 1) one at residues1-21, which is at the NH₂ terminus of the caveolin-1 $alpha$ isoform,and 2) the other at residues 61-101, spanning both the oligomerizationdomain (residues 61-101) and the scaffolding domain (residues81-101). To determine whether one or both epitopes could blockthe effect of pCav-1, we preincubated the antibody with GST-Cav^1-21, GST-Cav^61-101, or GST alone before adding the mixtures of antibodies and fusionproteins to permeabilized cells. After cells were exposed to staticcontrol or shear stress, activation of ERK was measured. As shownin Figs. 4 and 6, treatment of minimally permeabilized cells withpCav-1 inhibited shear-dependent activation of ERK (Fig. 8, comparelanes 1 and 2 with lanes 3 and 4). However, the inhibitory effectof pCav-1 completely reversed if the antibody was preincubatedwith GST-Cav^61-101 (Fig. 8, compare lanes 3 and 4 with lanes 9 and 10). In contrast,GST-Cav^1-21 or GST alone did not reverse the inhibitory effect of the pCav-1antibody (Fig. 8, lanes 4-7). Although in some studies treatmentof cells with GST-Cav^61-101 plus pCav-1 appeared to have a small effect on basal ERK activity(Fig. 8, lane 9), this effect was not statistically significant(n = 3). Furthermore, GST-caveolins or GST alone had no effectin the absence of the antibody on control or shear-dependent activationof ERK (Fig. 8, compare lanes 11 and 12 with lanes 13-18). Theseresults show that the peptide 61-101 of caveolin-1 is the essentialregion that mediates the inhibitory effect of pCav-1 on shear-dependentactivation of ERK.

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Fig. 8. Residues 61-101 of caveolin-1 prevent the inhibitory effect of pCav-1 on shear-dependent activation of ERK. A: pCav-1 (2.5 µg/ml) was preincubated for 2 h without or with 1 µg/ml GST-Cav^1-21 (1-21) and GST-Cav^61-101 (61-101) or GST alone. Mixtures of pCav-1 and GST-fusion proteins were then added to BAEC in presence of Triton as described in Fig. 3. As a control (lanes 1 and 2), cells were incubated only with Triton X-100 without antibody. In some studies (lanes 13-18), BAEC were incubated with GST-fusion proteins (1-21 or 61-101) or GST alone with Triton but in absence of pCav-1. After minimum permeabilization and antibody treatment, cells were exposed to shear stress (10 dyn/cm² for 5 min), and ERK activity was determined by Western blot using antibodies specific for pERK1/2 and total ERK (A) as described in Fig. 3. Representative Western blots with total ERK and pERK antibody, respectively, are shown. B: bar graphs represent means ± SE (n = 3) of densitometric quantitation of pERK1 bands. *P < 0.05.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The current study demonstrates that shear stress-dependent activation of ERK is inhibited by an antibody to caveolin-1, pCav-1,in Triton-permeabilized BAEC. In this study we have establisheda unique method to minimally permeabilize cells using a low concentrationof Triton X-100. Using this method, we were able to show thatpCav-1 can be delivered to virtually all BAEC and that the antibodybound to 3-7% of total caveolin-1 as determined by immunohistochemistryor immunoprecipitation (Figs. 2, 3, and 6A). Although only a smallfraction of caveolin-1 was bound by the pCav-1 antibody, it wasenough to inhibit shear stress-dependent activation of ERK by65-90% of control in >12 different experiments. This finding raisesthe interesting possibility that endothelial cells may containdifferent pools of caveolin-1, one of which readily binds to thepCav-1 antibody and plays a crucial role in the mechanosensitiveactivation of ERK. Furthermore, the mechanisms by which the pCav-1antibody inhibits shear-dependent activation of ERK involve theamino acid residues 61-101 of caveolin-1. These results suggestthat the scaffolding and oligomerization domains (residues 61-101)of caveolin-1 are critical in regulating the mechanosensitiveactivation ofERK.

Caveolin-1 is composed of 178 amino acids, and its topology is thought to resemble a hairpinlike structure with its membrane-spanningdomain (residues 102-134) flanked by the NH₂ terminus (residues1-101) and COOH terminus (residues 134-178), both of which facethe cytoplasm (27). Caveolin-1 forms oligomers through its oligomerizationdomain (residues 61-101) and the COOH terminus (39) and bindsdirectly with many signaling molecules such as heterotrimericG proteins, Ras, Src family kinases, and eNOS through the scaffoldingdomain (residues 81-101) (27). These caveolin-binding signalingmolecules have been proposed to form signal transduction unitsin the inactive state within caveolae-like structures, ready tobe activated by specific stimuli (27). The sequestration ofpreassembled signaling units may provide the mechanisms responsiblefor signaling specificity and efficiency in response to specificstimuli. Most caveolin-binding signaling proteins contain thetwo related motifs ( $Phi$ X $Phi$ XXXX $Phi$ and $Phi$ XXXX $Phi$ XX $Phi$ , where $Phi$ is the aromaticamino acid Trp, Phe, or Tyr) that bind to the scaffolding domainof caveolin-1 (38).

What is the mechanism by which pCav-1 inhibits activation of ERK in response to shear stress? Although pCav-1 binds to thetwo caveolin-1 epitopes (residues 1-21 and 61-101), only the additionof the competing fusion protein GST-Cav^61-101 prevents the inhibitory effect of pCav-1 on shear activationof ERK (Fig. 8). A simple interpretation of this finding is thatthe binding of pCav-1 to the residues 61-101 of caveolin-1 disruptsclustering of caveolin-1 (oligomerization domain at the residues61-101) or the interaction between the scaffolding domain (residues81-101) and signaling molecules (e.g., G_i-2, Src, and Ras) thatare upstream regulators of the flow-sensitive ERK pathway. Currentliterature provides strong support for the possibility that bindingof pCav-1 to the scaffolding domain would compete with the caveolin-bindingsignaling molecules and displace them from caveolin-1. This disruptionwould then prevent activation of the ERK pathway in response toshear stress. It was recently found that the scaffolding domainis both necessary and sufficient for membrane attachment of caveolin-1(34). This provides an additional possibility that pCav-1 maydisrupt attachment of caveolin-1 to membrane, resulting in itsinability to mediate the mechanosensitive activation of ERK pathway.At present, we cannot exclude other possibilities, including thepossibility that the binding of the pCav-1 antibody to caveolin-1interferes with trafficking of cholesterol between caveolae andintracellular compartments such as endoplasmic reticulum (1).The exact mechanisms underlying the specific effect of pCav-1await furtherstudies.

Caveolin-1 binds to itself as well as caveolin-2 to form homo- or heterooligomers (6, 31). Therefore, the inhibitoryeffect of pCav-1 on shear activation of ERK may involve caveolin-2directly or indirectly. It is not clear, however, whether BAECexpress caveolin-2. Unlike caveolin-1, the amino acid sequencesof caveolin-2 show species-specific (human vs. canine) differences(31, 32). Two caveolin-2 antibodies are currently available:one is specific for human caveolin-2 (Transduction Lab) and theother for the canine form (31). However, both antibodies failedto recognize caveolin-2 by either immunoprecipitation or Westernblot analysis in BAEC, whereas the mouse and canine antibodiesrecognized caveolin-2 expressed in RSV-3T3 cells (provided asa positive control by Transduction Lab) and Madin-Darby caninekidney cells, respectively (data not shown). Caveolin-2 antibodiesrecognizing the bovine form are not yet available to our knowledge.Although both caveolin-2 antibodies had no effect on the shearactivation of ERK (results not shown), these studies need to beevaluated further when bovine-specific caveolin-2 antibodies becomeavailable.

Collectively, our current and previous (28) findings as well as the report by Schnitzer and colleagues (30) suggest thatthe cholesterol- and caveolin-sensitive platforms in the plasmamembrane such as caveolae-like domains are responsible for mediatingthe activation of ERK in response to shear stress. These findingshave implications in not only the mechanisms responsible for spatialsequestration of signaling units but also the elusive mechanosensor(s)that senses the changes in shear stress. Several candidates havebeen proposed as the potential mechanosensor, including the caveolaestructure itself, G proteins, G protein-coupled receptors, integrins-cytoskeleton(tensegrity theory), and ion channels (3, 7, 12, 30,44). It is interesting to note that many of these candidates,including caveolae, G protein-coupled receptors, G proteins, andintegrins, have been shown to interact with caveolin-1 (3,27, 44, 45, 46). Recently integrins, transmembrane glycoproteinsthat act as adhesion receptors for extracellular matrix, havebeen reported as caveolin-binding molecules (45, 46). Severallines of evidence provide support for the potential importanceof caveolin-integrin interaction in the shear-dependent ERK pathway:1) integrin-dependent cell adhesion is required for activationof ERK (41), 2) $alpha$ _v $beta$ ₃- and $beta$ ₁-integrins and FAK are involvedin the mediation of shear-dependent ERK activation (14, 22),and 3) caveolin-1 binds to $beta$ ₁-integrins and plays a critical rolein integrin-dependent activation of ERK and cell adhesion (45,46).

The minimal permeabilization method developed in this study using a non-cholesterol-specific detergent could be used as ageneral technique to deliver membrane-impermeable macro- or micromolecules(i.e., peptides, antibodies, oligonucleotides, etc.) inside thecells. This could be especially useful as an alternative to otherwildly used membrane-permeabilizing agents such as digitonin andfilipin, which work by chelating membrane cholesterol, therebypotentially interfering with caveolae-dependent cellular functions(28).

In summary, we report that the scaffolding and/or oligomerization domain of caveolin-1 plays an essential role in shear stress-dependentactivation of ERK. On the basis of our current and previous (28)findings, we propose that the shear-sensitive signaling moleculesthat regulate the ERK pathway are assembled in caveolae-like domainsby binding to the scaffolding domain of caveolin-1 in the inactivestate. Changes in shear stress level may then specifically triggerrapid, organized, and compartmentalized signaling cascades toactivate ERK, but not other pathways. This spatial compartmentalizationmodel provides a plausible mechanism by which shear stress differentiallyactivates MAP kinases and other mechanosensitive responses inendothelialcells.

	ACKNOWLEDGEMENTS

We thank Dr. Kai Simons for providing a canine caveolin-2 antibody and Dr. V. Darley-Usmar for critically reading thismanuscript.

	FOOTNOTES

This work was supported by National Heart, Lung, and Blood Institute First Award HL-53601, National Aeronautics and SpaceAdministration Grant NAG2-1348, American Heart Association (AHA)Grant-In-Aid AL-G-960035, and a University of Alabama Health ServicesFoundation-General Endowment Fund Grant (to H. Jo); a postdoctoralfellowship from AHA-Southeast Consortium (to H. Park); and NationalCancer Institute Grant R01-CA-80250 and grants from the CharlesE. Culpeper Foundation, the G. Harold and Leila Y. Mathers CharitableFoundation, and the Sidney Kimmel Foundation for Cancer Research(to M. P.Lisanti).

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate thisfact.

Address for reprint requests and other correspondence: H. Jo, Univ. of Alabama at Birmingham, Dept. of Pathology, G019C Volker Hall, Birmingham, AL 35294 (E-mail: Jo{at}path.uab.edu).

Received 21 July 1999; accepted in final form 24 November 1999.

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