Inhibition of endothelial cell survival and angiogenesis by protein kinase A (original) (raw)

Integrin α5β1 promotes endothelial cell survival in vitro and in vivo. Antagonists of α5β1 and fibronectin inhibit growth factor and tumor-induced angiogenesis (17, 19). Because integrins have been shown to promote cell survival, we examined the roles of α5β1 and fibronectin in endothelial cell survival. Endothelial cells (HUVECs) cultured on poly-L-lysine (which mediates nonspecific cell attachment to the substratum) and fibronectin substrates were analyzed for the binding of annexin V, a Ca2+-dependent phospholipid-binding protein that binds to apoptotic cells with exposed phosphatidyl serine (29). HUVECs attached to fibronectin bind little annexin V, whereas over 85% of cells on poly-L-lysine–coated plates bound annexin V (Figure 1a, P = 0.01). Additionally, lysates from HUVECs cultured in suspension or on poly-L-lysine and fibronectin were immunoblotted for PARP, an enzyme involved in DNA repair that is cleaved by caspase-3 during the early stages of apoptosis to produce 85-kDa and 2-kDa fragments, resulting in loss of normal PARP function (30, 31). Cells in suspension or attached to poly-L-lysine displayed significant PARP cleavage, while cells attached to fibronectin showed little PARP cleavage (Figure 1b, P = 0.006). Similarly, attachment to fibronectin, but not poly-L-lysine, protects HUVECs from DNA fragmentation associated with apoptosis (Figure 1c, P = 0.0001). These studies indicate that fibronectin attachment promotes the survival of proliferating endothelial cells.

Fibronectin and integrin α5β1 support endothelial cell survival. (a–c) HUVEFigure 1

Fibronectin and integrin α5β1 support endothelial cell survival. (ac) HUVECs were maintained in suspension (SUS) or on fibronectin-coated (Fn) or poly-L-lysine–coated (PLL) plates. (a) The percentage of annexin V–positive cells on poly-L-lysine– or fibronectin-coated dishes was determined at regular intervals from 0 to 8 hours. (b) Cell lysates prepared after 4 hours of attachment were immunoblotted to detect intact (116 kDa) and cleaved PARP (85 kDa). The ratio of intact to cleaved PARP was determined by densitometry. Cl., cleaved. (c) Soluble DNA extracted from cells attached to poly-L-lysine or fibronectin was electrophoresed on 1.6% agarose gels. Relative DNA cleavage was determined by densitometry. (df) HUVECs were plated on fibronectin, anti-α5β1, or control Ab-coated plates. (d) The percentage of annexin V–positive cells was determined from 0 to 8 hours. (e) Cell lysates were immunoblotted to detect intact and cleaved PARP. (f) DNA fragmentation was evaluated as in c. cIgG, control immunoglobulin.

To determine if integrin α5β1 is the fibronectin receptor supporting HUVEC survival in vitro, HUVECs were cultured on surfaces coated with anti-α5β1 or control Ab’s. Immobilized anti-integrin Ab’s cluster integrins, thereby acting as agonists (6, 32). Cells attached to surfaces coated with Ab’s directed against α5β1 bound little annexin (Figure 1d, P = 0.001) and thus remained viable. In contrast, more than 75% of cells attached to control Ab’s were annexin positive. Cells attached to α5β1 Ab-coated surfaces also showed significantly less PARP cleavage (Figure 1e, P = 0.007) and DNA fragmentation (Figure 1f, P = 0.003) than cells attached to control Ab’s. These results indicate that α5β1 promotes endothelial cell survival.

Antagonists of integrin α5β1 block angiogenesis in vivo but have no effect on unstimulated blood vessels (17). To determine if these antagonists induce endothelial cell apoptosis during angiogenesis in vivo, CAMs were stimulated with bFGF, treated with saline, function-blocking anti-α5β1 Ab’s, and isotype-matched control Ab’s, and then analyzed for markers of apoptosis. Intravenous injection of fluorescently labeled annexin V demonstrated that α5β1 antagonists induce endothelial cell apoptosis in vivo. Anti-α5β1 Ab’s, but not saline or control Ab’s, induced annexin V staining of blood vessels in living CAMs, indicating that α5β1 regulates survival in vivo of proliferating endothelial cells (Figure 2a). In fact, vessels in anti–α5β1-treated CAMs bound eight times more annexin V than control-treated CAMs (Figure 2b, P = 0.015). These anti-α5β1 Ab’s were shown previously to react with α5β1 on chicken endothelial cells and to block its function in vitro and in vivo (17). Because α5β1 is only expressed at significant levels on proliferating endothelial cells (17), α5β1 function-blocking Ab’s target proliferating endothelial cells. Because peptide and small molecule antagonists of α5β1 also inhibit angiogenesis (17) and induce apoptosis (not shown), Ab-mediated complement activation is not likely to play a significant role in this apoptosis induction. Thus, these results suggest that integrin α5β1 antagonists induce endothelial cell apoptosis in vivo.

Integrin α5β1 supports endothelial cell survival during angiogenesis in vivFigure 2

Integrin α5β1 supports endothelial cell survival during angiogenesis in vivo. (a) CAMs were stimulated with bFGF or saline and then treated for 24 hours with saline, anti-α5β1, and control Ab’s. CAMs were then injected with 50 μl FITC-annexin V, harvested 2 hours later, and analyzed directly by confocal microscopy. (b) Green pixels (annexin V positive) present per optical section were quantified. (c) CAMs treated as in a were cryosectioned and immunostained with anti–cleaved caspase-3 (anti-cl.csp3) (green) and anti-vWF (red). Cleaved caspase-3–positive blood vessels are yellow (arrows). (d) CAMs treated as in a were cryosectioned and immunostained with anti-vWF (red) and for DNA fragmentation (TUNEL staining, green). Arrows indicate blood vessels. Yellow structures are apoptotic blood vessels. (e) Soluble DNA isolated from CAMs treated as in a was electrophoresed on 1.6% agarose gels. Molecular-weight markers are 1-kb DNA ladders. Relative DNA cleavage was determined by densitometry. (f) Individual cells isolated from CAMs treated as in a were stained with FITC-annexin V.

To determine further whether α5β1 antagonists cause apoptosis in vivo, sections of CAMs were analyzed for the expression of cleaved caspase-3 in blood vessels (Figure 2c, P = 0.01). Cleavage of caspase-3 into 17- and 12-kDa fragments is an indication of caspase-3 activation; the amount of cleaved caspase-3 is a quantitative index of apoptosis induction. Ab’s directed against mammalian caspases cross-react with avian caspases, because avian caspases exhibit 65% overall sequence identity and 100% activation domain sequence identity with mammalian caspases (33). Treatment with either α5β1 or αvβ3 antagonists induces caspase-3 cleavage (green) in blood vessels (red) in growth factor–stimulated CAMs. Antagonists of α5β1 but not control Ab’s also induce DNA fragmentation in bFGF-stimulated endothelial cells, as evaluated by TUNEL staining (Figure 2d) and by analysis of DNA fragmentation of agarose gels (Figure 2e, P = 0.003). Furthermore, isolated cells from CAMs treated with α5β1 and αvβ3 function-blocking Ab’s bound significantly more FITC-annexin V than in cells from control CAMs (Figure 2f, P = 0.0002 and 0.003, respectively). These studies definitively show that α5β1 antagonists induce endothelial cell apoptosis during angiogenesis.

Unligated integrin α5β1 induces apoptosis in adherent endothelial cells. To determine how α5β1 antagonists interfere with cell survival during angiogenesis, proliferating HUVECs in complete culture medium were plated on poly-L-lysine–, fibronectin-, vitronectin-, or collagen-coated culture plates in the presence of Ab antagonists of integrins α5β1, αvβ3, or α2β1 for 24 hours. Cells were then stained with FITC-annexin V. While fibronectin and vitronectin promote the survival of proliferating endothelial cells (Figure 3, a and c), collagen does not (ref. 34; data not shown). Integrin antagonists that block cell attachment to the substratum (Figure 3, b and d) induce apoptosis, or anoikis, in endothelial cells (Figure 3, a and c). For example, antagonists of α5β1 induce apoptosis on fibronectin (Figure 3a, P = 0.001), while antagonists of αvβ3 induce apoptosis on vitronectin (Figure 3c, P = 0.02) by blocking cell attachment to the substratum.

Unligated integrin α5β1 regulates endothelial cell survival. HUVECs were plFigure 3

Unligated integrin α5β1 regulates endothelial cell survival. HUVECs were plated on poly-L-lysine–coated, fibronectin-coated (a and b), or vitronectin-coated (c and d) culture plates in culture medium (med) or culture medium containing anti-α5β1, anti-αvβ3, anti-α2β1 Ab’s. After 1 hour, cell attachment was determined (b and d). After 24 hours, the percentage of FITC-annexin V–positive (a and c) cells was determined. (e) HUVECs plated on vitronectin-coated plates in the presence of function-blocking anti-α5β1 or control Ab’s were collected at regular intervals from 0 to 8 hours and PARP cleavage assessed by Western blotting. Relative PARP cleavage levels were determined by densitometry.

In vivo, however, anoikis induced by loss of attachment to the ECM is unlikely to occur because endothelial cells are attached to multiple matrix proteins through multiple integrins at any one time. Therefore, we also examined the ability of integrin antagonists to induce apoptosis in cells that remain attached through other integrins. In fact, α5β1 antagonists induce apoptosis of cells on vitronectin (Figure 3c, P = 0.05) without affecting their attachment to vitronectin (Figure 3d). Anti-α5β1, but not control Ab’s, also induce PARP cleavage in HUVECs plated on vitronectin substrates (Figure 3e, P = 0.003). Thus, unligated α5β1 inhibits endothelial cell survival on provisional matrix proteins such as fibronectin and vitronectin. These studies indicate that integrin α5β1 provides critical survival signals to proliferating endothelial cells such as those participating in angiogenesis. These studies indicate that integrin α5β1 can directly and indirectly regulate survival of proliferating endothelial cells.

Unligated integrin α5β1 activates a caspase-8–mediated apoptosis pathway in vitro and in vivo. To determine the nature of the cell death pathway induced by α5β1 antagonists, endothelial cells were plated on ECM protein–coated culture plates in the presence of integrin antagonists and caspase inhibitors or vehicle control (0.33% DMSO). Cell death induced by anti-α5β1 Ab’s was blocked by caspase-3 inhibitors, whether the cells were attached to fibronectin (P = 0.0005, Figure 4a) or vitronectin (P = 0.02, Figure 4b). Cell attachment to poly-L-lysine rapidly activated caspases-3 and -8 while attachment to vitronectin did not (Figure 4, c and d). Anti-α5β1 Ab’s but not control Ab’s also activated caspase-3 and -8 (P = 0.0001 and P = 0.002, respectively) in cells attached to vitronectin (Figure 4, c and d) and fibronectin (not shown). Caspase-3 cleavage was also readily detected in cells treated with anti-α5β1 but not control Ab’s (P = 0.01, Figure 4e). In contrast, caspase-9 cleavage was not detected in cells treated with α5β1 antagonists (Figure 4f). These studies show that integrin α5β1 antagonists induce a proapoptotic pathway in proliferating endothelial cells that results from activation of initiator caspases (8) rather than stress caspase (9) pathways. These results also indicate that blocking α5β1 ligation induces caspase-8– and -3–mediated death even when cells are still attached to provisional matrix ligands through other integrins.

Unligated integrin α5β1 induces caspase-3 and -8, but not -9, activation. HFigure 4

Unligated integrin α5β1 induces caspase-3 and -8, but not -9, activation. HUVECs were plated on (a) fibronectin-, (b) vitronectin-, or (a and b) poly-L-lysine–coated culture plates in the presence of anti-α5β1 Ab’s and 50 μM z-DEVD-fmk (caspase-3) or z-IETD-fmk (caspase-8) inhibitors or vehicle control (0.33% DMSO) for 24 hours. The percentage of annexin V–positive cells was then determined. inhib, inhibitor. (c and d) Caspase-3 and -8 activities were determined in HUVECs plated on vitronectin-coated or poly-L-lysine–coated plates in the presence of culture medium, anti-α5β1, or control Ab’s. (e) Cell lysates were immunoblotted with anti–caspase-3 and anti–cleaved caspase-3 Ab’s. Relative caspase-3 cleavage was determined by densitometry. (f) Cell lysates were immunoblotted with anti–caspase-9 and anti–cleaved caspase-9 Ab’s.

Our studies show that integrin-mediated survival depends on suppression of caspase-3 and -8 activity in vitro. As α5β1 antagonists block angiogenesis in vivo, these antagonists may induce caspase-3 and -8 activation in vivo. CAMs stimulated with bFGF were treated with saline, vehicle control (DMSO), caspase-3 or -8 inhibitors, and anti-integrin Ab’s in the presence or absence of caspase inhibitors. Angiogenesis was inhibited by anti-α5β1 Ab’s (Figure 5, a–d); this inhibition was partially reversed by cell-permeable caspase-3 inhibitors (P = 0.04, Figure 5a) and fully reversed by caspase-8 inhibitors (P = 0.05, Figure 5c). Caspase-3 inhibitors partially blocked caspase-3 activity in vivo (Figure 5b), while caspase-8 inhibitors completely blocked its activity in vivo (Figure 5d). Furthermore, caspase-3 and -8 inhibitors prevented in vivo endothelial cell DNA fragmentation induced by α5β1 inhibition (Figure 5e). Caspase-9 inhibitors had little effect on angiogenesis (not shown). Caspase inhibitors alone had no effect on angiogenesis or on unstimulated CAMs. These results indicate that α5β1 antagonists activate caspases-8 and -3 in vivo, thereby inhibiting angiogenesis.

Integrin antagonists induce caspase-3– and -8–dependent apoptosis in vivo.Figure 5

Integrin antagonists induce caspase-3– and -8–dependent apoptosis in vivo. (ad) CAMs stimulated with saline or bFGF were treated with 2.5% DMSO (vehicle control), anti-α5β1, or anti-α5β1 with 500 μM caspase-3 (a and b) or caspase-8 (c and d) inhibitors. (a and c) Blood vessel branch points were quantified after 48 hours. (b and d) Caspase-3 and -8 cleavage was evaluated by Western blotting with (b) anti–cleaved caspase-3 or (d) anti–cleaved caspase-8 Ab’s and anti-actin Ab’s. (e) Cryosections of CAMs treated as in ad were immunostained for vWF expression (red) and to detect DNA fragmentation (TUNEL staining, green). Arrows indicate blood vessels. Apoptotic vessels appear yellow.

Unligated integrins induce PKA-dependent apoptosis. Integrin ligation activates signaling pathways that promote cell migration, proliferation, and survival. Typically, integrin-mediated signaling is characterized by increases in tyrosine phosphorylation of signaling intermediates such as focal adhesion kinase, src, and ERK family members. However, integrin ligation also suppresses the activation of at least one kinase, PKA (19). Importantly, we found that integrin ligation suppresses PKA activation, while antagonists of integrins activate this enzyme (Figure 6a). Notably, antagonists of integrin α5β1 activate endothelial cell PKA whether endothelial cells are plated on fibronectin or on vitronectin (Figure 6a). Therefore, we investigated the contribution of PKA to integrin-mediated cell death. We found that a pharmacological inhibitor of PKA, HA1004, substantially suppressed the apoptosis induced by integrin antagonists anti-αvβ3 (P = 0.05) or anti-α5β1 (P = 0.05) in cells attached to vitronectin, as detected by annexin V binding to intact cells (Figure 6b). PKA inhibitors also blocked caspase-3 cleavage induced by anti-α5β1 (P = 0.002, Figure 6c). Expression of dnPKA, but not a control transgene (GFP), also prevented integrin antagonist–induced cell death (P = 0.004; Figure 7, a and b). More than 80% of cells expressed the transgene, which was also detected by Western blotting (Figure 7d). These studies indicate that both direct (anoikis) and indirect integrin antagonist–mediated cell death is PKA dependent.

Unligated α5β1-mediated death is PKA dependent. (a) PKA activity was measurFigure 6

Unligated α5β1-mediated death is PKA dependent. (a) PKA activity was measured in HUVECs attached to poly-L-lysine, fibronectin, or vitronectin in the presence or absence of integrin antagonists. (b) HUVECs were plated on vitronectin-coated or poly-L-lysine–coated culture plates in the presence or absence of anti-α5β1 or anti-αvβ3 Ab’s, a selective PKA inhibitor (1 μM HA1004), or anti-integrin Ab’s in combination with 1 μM HA1004. After 24 hours, the percentage of FITC-annexin–positive cells was determined. (c) Cell lysates from b were immunoblotted with anti–caspase-3 and anti–cleaved caspase-3 Ab’s. Relative caspase-3 cleavage was determined by densitometry.

PKA negatively regulates cell survival. (a and b) HUVECs transfected with GFigure 7

PKA negatively regulates cell survival. (a and b) HUVECs transfected with GFP (–) or a dnPKA (+) were plated on (a) fibronectin-coated, (b) vitronectin-coated, or poly-L-lysine–coated plates in the absence or presence of anti-α5β1, anti-αvβ3, or anti-α2β1. After 24 hours, the percentage of annexin V–positive cells was determined. (c) HUVECs treated with culture medium or dibutyryl cAMP (250 μM) and HUVECs transfected with GFP or the catalytic subunit of PKA (PKAcat) were plated on vitronectin-, or poly-L-lysine–coated plates. After 24 hours, the percentage of annexin V–positive cells was determined. (d) Expression of transgenes was detected by Western blotting cell lysates with anti-GFP or anti-V5.

PKA activation induces endothelial cell apoptosis in vitro and in vivo. Our studies show that inhibition of PKA suppresses integrin antagonist–induced cell death. To determine whether activation of PKA directly induces endothelial cell death, endothelial cells were treated with dibutyryl cAMP or were transiently transfected with the active, catalytic subunit of PKA. Both cAMP and expression of the catalytic subunit of PKA significantly induce apoptosis (P = 0.009 and P = 0.003, respectively) in endothelial cells in vitro (Figure 7c). Thus, PKA directly induces apoptosis in endothelial cells.

To determine whether PKA plays a role in the negative regulation of angiogenesis in vivo, bFGF-stimulated CAMs were transfected with expression plasmids encoding GFP and dnPKA and treated with α5β1 Ab’s. While α5β1 antagonists block angiogenesis (Figure 8a, P = 0.004), dnPKA reverses this inhibition (Figure 8a, P = 0.02). Expression of dnPKA also prevents α5β1 antagonist–induced DNA fragmentation in vivo as detected by TUNEL staining (Figure 8b) and inhibits activation of caspase-3 and -8 in vivo (Figure 8c). Since integrin antagonists induce PKA-dependent apoptosis in vivo, direct activation of PKA may also inhibit angiogenesis. Expression of the PKA catalytic subunit during angiogenesis in vivo completely suppresses angiogenesis (P = 0.0005), as does exposure to cAMP (P = 0.001, Figure 8d). VEGF-stimulated angiogenesis is also inhibited by activation of PKA (data not shown). This inhibition results from apoptosis induction, because it is accompanied by DNA fragmentation detected by TUNEL staining (Figure 8e) and caspase-3 cleavage in vivo (Figure 8f). The expression of transgenes could be demonstrated in endothelial cells in vivo by immunohistochemical staining for the presence of His-tagged proteins (Figure 8g). Thus, activation of PKA by integrin antagonists, by cAMP, or by expression of the catalytic subunit of PKA induces endothelial cell apoptosis and inhibits angiogenesis.

PKA inhibits angiogenesis by inducing apoptosis. (a) CAMs stimulated with bFigure 8

PKA inhibits angiogenesis by inducing apoptosis. (a) CAMs stimulated with bFGF were transfected 24 hours later by placing 4 μg pcDNA/V5/His dnPKA or N1-GFP expression plasmid on CAMs. CAMs were treated on the same day with saline or anti-α5β1 Ab’s and were harvested 48 hours later. Blood vessel branch points were quantified. (b) Cryosections of CAMs from a were immunostained with anti-vWF (red) and were stained to detect fragmented DNA by the TUNEL method (green). Arrows indicate blood vessels. Apoptotic blood vessels appear yellow. (c) Western blots of lysates prepared from CAMs treated as in a were immunoblotted with anti–cleaved caspase-3 and anti–cleaved caspase –8, as well as anti-actin as a loading control. (d) CAMs stimulated with bFGF were treated with saline or 250 μM cAMP or were transfected by placing 4 μg pcDNA/V5/His PKAcat or N1-GFP expression plasmid on stimulated CAMs. Blood vessel branch points were quantified 48 hours later. (e) Cryosections of CAMs from d were immunostained with anti-vWF (red) and were stained to detect fragmented DNA by the TUNEL method (green). Arrows indicate blood vessels. Apoptotic blood vessels appear yellow. (f) Detergent lysates prepared from freshly excised CAMs from d were immunoblotted for expression of cleaved caspase-3 and actin as a loading control. (g) Cryosections of CAMs from a and d were immunostained with anti-pentaHis (red) to detect expression of His-tagged transgenes in the transfected CAM tissue. Sections were counterstained with DAPI. Arrows indicate blood vessels.

These studies demonstrate that the unligated integrin α5β1 induces endothelial cell apoptosis in vivo in a PKA-dependent manner, thereby inhibiting angiogenesis. These studies demonstrate that activation of PKA by unligated integrins is an essential step in the induction of apoptosis. Importantly, our studies demonstrate that direct activation of PKA in vivo induces endothelial cell apoptosis and inhibition of angiogenesis.