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J Thorac Cardiovasc Surg 2007;133:1137-1146
© 2007 The American Association for Thoracic Surgery

Cardiopulmonary Support and Physiology

Endothelin-1 accentuates the proatherosclerotic effects associated with C-reactive protein

^a Heart Transplant Program, Toronto General Hospital, University Health Network, University of Toronto, Toronto, Ontario, Canada
^b Division of Cardiac Surgery, University of Toronto, Toronto, Ontario, Canada
^c Division of Cardiology, University of Toronto, Toronto, Ontario, Canada.

Read at the Eighty-sixth Annual Meeting of The American Association for Thoracic Surgery, Philadelphia, Pa, April 29-May 3, 2006.

Received for publication April 28, 2006; revisions received October 18, 2006; accepted for publication November 1, 2006.

^_* Address for reprints: Vivek Rao, MD, PhD, FRCS, Alfredo and Teresa DeGasperis Chair in Heart Failure Surgery, 4N-464, Toronto General Hospital, 200 Elizabeth Street, Toronto, Ontario, M5G 2C4, Canada (Email: vivek.rao{at}uhn.on.ca).

	Abstract

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Objectives: The proinflammatory marker C-reactive protein has been demonstrated to play a role in the development of atherosclerosis. Endothelin-1 and nitric oxide homeostasis is crucial for normal vasomotor function, limiting inflammatory activation and maintaining a nonthrombogenic endothelial surface. In addition to its vasoactive properties, endothelin-1 is also an inflammatory cytokine. We have previously demonstrated that C-reactive protein impairs endothelial cell nitric oxide production. Protein kinase C, an important signal transducer within the cell, is involved in several cellular responses to external stimuli. We therefore sought to determine whether endothelin-1 exposure modulates C-reactive protein’s effects on nitric oxide production via protein kinase C.

Methods: Endothelial cells were incubated with C-reactive protein (200 µg), endothelin-1 (100 nM), C-reactive protein + endothelin-1, or phosphate-buffered saline solution (control) for 24 hours. After exposure, endothelial nitric oxide synthase expression was determined in addition to total nitric oxide production and protein kinase C translocation and activity.

Results: Endothelial nitric oxide synthase protein expression was reduced following incubation with C-reactive protein and endothelin-1 treatment compared with baseline by 40% and 45%, respectively (P = .04); however, no additive effects were seen with coincubation. C-reactive protein produced a 47% decrease in nitric oxide production compared with control. Coincubation with endothelin-1 resulted in a synergistic 70% reduction in nitric oxide production (P = .001). C-reactive protein exposure inhibited translocation of protein kinase C compared with control (P = .01). Furthermore, coincubation of C-reactive protein with endothelin-1 led to a synergistic inhibition of protein kinase C translocation (P = .01). C-reactive protein exposure reduced protein kinase C activity by 40% compared with control (P = .02), although coincubation with endothelin-1 had a synergistic reduction in activity (P = .02).

Conclusions: Our results indicate that endothelin-1 exposure accentuated C-reactive protein’s impairment of endothelial nitric oxide production via synergistic inhibition of protein kinase C translocation and activity. Our investigations suggest that endothelin-1 inhibition and protein kinase C stimulation may provide a novel therapeutic strategy to improve vascular nitric oxide homeostasis and mitigate the proatherosclerotic effects of C-reactive protein.

	Introduction

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Endothelial dysfunction, an initiator of atherosclerosis, is manifested by altered nitric oxide (NO) and endothelin-1 (ET-1) homeostasis. Impaired NO release precedes the development of atherosclerosis and serves to reinforce vascular pathology once established. ET-1 is one of the most potent endogenous vasoconstrictors¹ and mediates a host of responses including endothelial dysfunction, vasomotor contraction, leukocyte activation, and cellular proliferation.^2,3 Diminished production of NO and exaggerated release of ET-1 are believed to be key initiators of endothelial injury.³ Impaired NO homeostasis, a hallmark of endothelial dysfunction, not only reflects the degree of endothelial cell injury but also is an active component of the atherosclerotic process. Reduced NO release results in heightened endothelial cell thrombogenicity, loss of inflammatory cell inhibition, and altered vasomotor function. The deleterious effects of NO impairment finally culminate in the development of atherosclerosis. Several investigators have demonstrated that ET-1 adversely affects endothelial function as well as outcomes following cardiac surgery.^3-7 We have previously shown that ET-1 results in endothelial dysfunction following cardiac transplantation and antagonism with bosentan abrogated this effect.⁵ Recent evidence suggests that elevated levels of ET-1 may impair NO production.^8,9 However, the mechanisms by which elevated levels of ET-1 reduce NO production in endothelial cells have yet to be determined. Therefore, the injured endothelial cell has altered ET-1 and NO homeostasis, resulting in vasomotor impairment, immune activation, and atherosclerosis.

Accumulating evidence supports the concept that inflammation plays a central role in the genesis of atherosclerosis and its complications.^10,11 Chronic inflammation results in endothelial dysfunction and facilitates the interactions between modified lipoproteins, monocyte-derived macrophages, T cells, and the normal cellular elements of the arterial wall (Figure 1). ^10,11 This inflammatory process ultimately leads to the development and progression of atherosclerosis.^10,11 The inflammatory marker C-reactive protein (CRP) has been shown to predict myocardial infarction, stroke, and vascular death in a variety of settings.^10-20 This acute-phase reactant has also been demonstrated to predict future coronary events and also to portend the vulnerability of an atherosclerotic lesion and the likelihood of plaque rupture.^{10-13,15,17-20} CRP augments the production of key inflammatory cytokines such as interleukin-6 and directly impairs NO homeostasis.²¹ Verma and colleagues²¹ demonstrated that CRP is not only a risk factor but also an active player in atherosclerosis by impairing NO production, resulting in endothelial dysfunction with its associated negative consequences. The mechanisms underlying this impairment in NO production remain unknown. Furthermore, whether ET-1 enhances the potential proatherosclerotic effects of CRP remains unclear.

View larger version (47K): [in this window] [in a new window]   Figure 1. A, Normal vascular NO homeostasis. B, Chronic inflammation results in endothelial dysfunction and facilitates the interactions between modified lipoproteins, monocyte-derived macrophages, T cells, and the normal cellular elements of the arterial wall, resulting in decreased NO production leading to impaired endothelial function and vasoconstriction. These same factors also increase ET-1 production, further promoting vasoconstriction and vasomotor impairment. C, Our hypothesis that CRP alters PKC activity leading to NO impairment.

	Materials and Methods

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Endothelial Cell Cultures
Human saphenous vein endothelial cells (HSVECs) were cultured in 10-cm diameter dishes at 37°C and 5% CO₂ in medium MCDB-131 (VEC Technologies, Rensselaer, NY) containing 10% fetal bovine serum, 100 U/mL penicillin, and 100 mg/mL streptomycin. Cells passaged 2 to 4 times and aged between 14 and 30 days from the time of primary culture were used for this study. We examined the effects of our interventions on eNOS expression, NO production, isoform-specific PKC translocation, and PKC activity. Cells were treated with CRP (25 µg/mL, Calbiochem, San Diego, Calif), 100 nM of ET-1 (Sigma, Oakville, Ontario, Canada), ET-1 + CRP, or phosphate-buffered saline solution (control, n = 12 per group) for 24 hours. ET-1 antagonism was achieved with the use of bosentan 10 µM (courtesy of Actelion Pharmaceuticals Ltd, Allschwil, Switzerland). We employed 2 PKC antagonists with different mechanisms of action, calphostin C (200 nM) and chelerythrine (1 µM; Sigma). Chelerythrine inhibits the adenosine triphosphate binding site, whereas calphostin C interferes with the lipid cofactor-binding site of PKC. The PKC agonist phorbol 12-myristate 13-acetate (PMA; 10 nM; Sigma) was used to stimulate PKC activity. The concentrations of these agents have been previously validated and published by our laboratory.²⁴

NO Production
Cell culture supernatants were collected following treatment. NO production was detected spectrophotometrically by measuring its degradation products, nitrite and nitrate. Total nitrite was quantified after the reduction of all nitrates with nitrate reductase. After the conversion of nitrate to nitrite, total nitrite was determined spectrophotometrically at 540 µm by using the Griess reaction. Total nitrite concentration was calculated from a standard curve and expressed as µmol/L per milligram protein. The amount of NO produced was normalized against total cellular protein and assessed using the Bradford method.²⁵

Protein Expression
Western immunoblotting was performed using chemiluminescent detection and protein-specific monoclonal antibodies for eNOS (BD Biosciences, Mississauga, Ontario, Canada). Samples were separated using sodium dodecylsulfate-polyacrylamide gel electrophoresis. Gels were then transferred to polyvinylidene fluoride membranes. Comparisons between groups were performed using densitometric analysis (BioRad, Hercules, Calif) corrected for ß-actin expression.

PKC Translocation/Activity
Determination of isoform-specific PKC translocation was performed by analysis of cytosolic and membrane fractions of HSVEC to calculate a membrane-to-cytosolic (M/C) ratio using Western blot analysis. Purity of the cytosolic and membrane fractions was determined by confirming the absence of membrane bound Ca-ATPase (cytosolic) or ß-actin (membrane). Our preliminary studies indicated that only the , , , , and PKC isoforms are present in this cell population. Therefore, each blot was stained with these isoform-specific antibodies.

For measurement of PKC activity, a commercially available PKC assay kit (Calbiochem) was used to determine protein-adjusted activity. Activity was determined colorimetrically at 490 nm and is displayed as arbitrary units per mg of protein (U/mg).

Statistical Analysis
All results are presented as means ± SD. Statistical comparisons were made by analysis of variance followed by Dunn’s multiple contrast test to identify differences between various treatments. Exact P values are provided for each comparison. Statistical analysis was performed with the SAS statistical software program version 8.2 (SAS Institute, Inc, Cary, NC).

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

 
CRP and ET-1 Attenuate NO Release
Treatment with CRP resulted in a 47% decrease in NO production compared with control (Figure 1, A). Exposure to ET-1 also reduced NO production (P = .001), although coincubation with CRP led to a further 70% reduction in NO release (P = .001; Figure 2, A). Bosentan treatment was effective in attenuating the effects of ET-1 on NO production; however, bosentan did not mitigate the effects of CRP. HSVEC exposed to bosentan alone demonstrated a significant increase in NO production by approximately 20% (P = .001).

View larger version (29K): [in this window] [in a new window]   Figure 2. A, NO production in HSVECs following treatment. The presence of CRP and ET-1 significantly reduced NO production. Coincubation of CRP with ET-1 resulted in a greater decrease in NO release. Bosentan treatment prevented ET-1-induced impairment in NO release but did not prevent the effects of CRP. B, Quantitative Western blot analysis following 24-hour exposure demonstrated that CRP, ET-1, and CRP + ET-1 exposure downregulated eNOS protein expression compared with control. Treatment of HSVEC with bosentan abrogated ET-1 inhibition of eNOS protein expression while having no effect on CRP-induced dowregulation.

PKC Isoforms
We assessed our cell cultures for the presence of several PKC isoforms (, ß, , , , , , ). We found the presence of only , , , , and isoforms in our HSVECs. No significant differences in PKC and PKC M/C ratios (translocation to the membrane) were seen between groups. PKC, , and isoforms demonstrated significant changes following treatment (Figure 3, A, B, C).

View larger version (43K): [in this window] [in a new window]   Figure 3. A, PKC translocation. Top, Western blot of PKC expression in the cytosolic fractions (C) and membrane fractions (M) following treatment. Bottom, Quantitative Western blot analysis of PKC translocation. No differences were seen after CRP treatment, although ET-1 exposure resulted in a significant PKC translocation to the membrane compared with control. Coincubation of CRP with ET-1 resulted in a further increase in PKC translocation. B, PKC translocation. Top, Western blot of PKC expression in the cytosolic fractions (C) and membrane fractions (M) following treatment. Bottom, Quantitative Western blot analysis of PKC translocation. PKC was significantly translocated to the membrane following both CRP and ET-1 treatment compared with control. Coincubation demonstrated PKC translocation that was significantly greater than that of CRP alone but similar to ET-1 exposed cells. C, PKC translocation. Top, Western blot of PKC expression in the cytosolic fractions (C) and membrane fractions (M) following treatment. Bottom, Quantitative Western blot analysis of PKC translocation. Exposure of HSVECs to CRP and ET-1 caused a significant lowering of PKC M/C ratio. Coincubation of CRP with ET-1 led to further decrease in PKC M/C ratio.

PKC inhibition resulted in a significantly reduced M/C ratio for PKC and PKC in control and in treated cells (CRP, ET, and CRP + ET; Table 2). PKC translocation was impaired following PKC inhibition only in the control groups (P < .05). PKC activation resulted in significantly greater translocation to the membrane of all PKC isoforms in all our treatment groups except for PKC in the CRP + ET group (Table 2).

PKC Activity
Determination of PKC translocation does not necessarily correlate with cellular PKC activity, and therefore we measured direct overall PKC activity. Endothelial cells treated with CRP or ET-1 displayed a significant reduction in PKC activity (P = .01; Figure 4). A greater reduction was seen following coincubation of CRP with ET-1 (Figure 4). Bosentan treatment blocked the ET-1-induced effect but also resulted in enhanced PKC activity (P < .05; Table 1). However, bosentan did not abrogate the CRP-induced effects. As expected, HSVEC treated with calphostin C and chelerythrine demonstrated reduced PKC activity. No further effect of ET-1 on CRP was seen. PMA exposure increased PKC activity and abrogated both CRP- and ET-1-induced effects.

View larger version (16K): [in this window] [in a new window]   Figure 4. HSVEC PKC activity. CRP and ET-1 caused a significant decrease in PKC activity compared with control with a further reduction seen following coincubation.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

We have made the following observations outlined in Figure 5:

1 CRP attenuates NO production and downregulates eNOS protein expression.

2 ET-1 accentuates the CRP-induced reduction in NO release with no further downregulation of eNOS expression.

3 CRP appears to selectively stimulate PKC translocation while inhibiting translocation with a further reduction in PKC translocation when coincubated with ET-1.

4 CRP inhibits PKC activity with a further decrease seen following ET-1 coincubation.

5 Bosentan can maintain cellular NO production following ET-1 exposure but does not prevent CRP-induced impairment.

6 PKC inhibition leads to a severe reduction in cellular NO production with no further reduction observed with simultaneous exposure to CRP or ET-1.

7 PKC stimulation with PMA significantly increases cellular NO production and is capable of completely reversing the inhibitory effects of both CRP and ET-1 exposure.

View larger version (47K): [in this window] [in a new window]   Figure 5. A, B, Human endothelial cell exposed to CRP or ET-1 results in decreased NO production by reducing PKC activity and translocation leading to eNOS downregulation. C, The concomitant exposure of ET-1 with CRP further reduces endothelial cell NO release by enhancing PKC inhibition and increased eNOS downregulation.

Our results are consistent with the studies by Verma and colleagues²¹ and Dong and associates,⁸ which demonstrated that elevated CRP and ET-1 levels result in downregulation of eNOS protein expression in endothelial cells. We demonstrated that CRP-induced NO dysregulation was partly caused by changes in eNOS protein expression. eNOS protein expression was downregulated following both CRP and ET-1 treatment. In contrast to NO production, no further reduction in eNOS expression was seen with coincubation. The greater impairment in NO production seen with coincubation may be a result of decreased eNOS activity. Decreased eNOS activity may be caused by changes in regulatory kinase activity such as PKC.

Our study demonstrated that NO production is regulated by PKC. NO bioavailability is impaired following PKC inhibition, and PKC activation led to NO release. Further evidence that PKC is a player in both CRP- and ET-1-induced NO impairment is that concomitant exposure of CRP or ET-1 with PKC inhibition did not lead to a greater reduction in NO bioavailability as would be anticipated if they acted in a PKC-independent fashion. The simultaneous exposure of our endothelial cells to PMA and CRP or ET-1 resulted in increased NO production similar to exposure to PMA alone. Our data support the hypothesis that CRP and ET-1 decrease NO production through PKC inhibition. eNOS protein expression was also regulated by PKC. We found that PKC antagonism downregulated eNOS protein expression, although PKC agonists upregulated eNOS protein expression. In addition, concomitant exposure of HSVECs to CRP or ET-1 with PMA resulted in upregulation of eNOS to a level similar to PMA alone, further demonstrating that CRP- and ET-1-induced alterations in eNOS expression is PKC dependent and is fully reversible by direct PKC stimulation.

The differential roles of PKC on NO production have been observed in various animal models.^26-28 Matsubara and colleagues²⁶ in bovine aortic cells found that PKC activation decreases NO production, although Partovian and coworkers²⁷ found that PKC activation increases NO formation. Partovian and associates²⁷ found that PKC activation increases eNOS activity in the vasculature, indicating that PKC regulation of eNOS is tissue and species dependent. Therefore, depending on species and cell type, PKC inhibition or activation can lead to NO impairment. In our study, using human endothelial cells, we demonstrated that PKC inhibition, likely the lambda isoform, decreases eNOS protein expression and NO production.

Effects of CRP and ET-1 on PKC Translocation and Activity
To determine which isoforms were involved in NO regulation, we evaluated isoform-specific translocation. Our study revealed that both CRP and ET-1 exposure resulted in membrane translocation of the epsilon isoforms, although the M/C ratio of the lambda isoform was reduced, suggesting inhibited translocation. Coincubation of CRP with ET-1 led to a greater increase in PKC translocation and further reduced PKC translocation. Because translocation does not always correlate with activity, we measured PKC activity in our cell cultures. We determined that cellular PKC activity is reduced following both CRP and ET-1 exposure, suggesting that inhibition of PKC activity is the likely mechanism by which CRP and ET-1 impairs NO production.

Our data revealed that ET-1 coincubated with CRP resulted in the greatest reduction in PKC activity, which corroborates the effect of ET-1 on CRP-induced NO impairment. The inhibition of eNOS protein expression was similar in all treatment groups; therefore, differences in NO production were caused by changes in eNOS activity. We speculate that eNOS activity is regulated by specific PKC isoforms. The results of our studies suggest that CRP and ET-1 reduces PKC translocation and overall PKC activity, leading to decreased eNOS activity and impaired NO production.

ET-1 has been extensively studied and found to typically increase PKC translocation in various cell types.^22,23,29-32 Dlugosz and colleagues²² demonstrated that ET-1 exposure results in PKC and PKC translocation in mesangial cells. McNair and associates’³¹ data showed that PKC is activated by ET-1 exposure in coronary smooth muscle. Our findings are consistent with previous results demonstrating PKC and PKC translocation following ET-1 exposure. Our observation that ET-1 reduces PKC translocation in human endothelial cells is a novel finding. We speculate that unlike lower levels of ET-1, which normally results in G protein S activation leading to PKC translocation, higher levels of ET-1 also activate G protein I, which leads to PKC inhibition. Further studies are required to demonstrate the mechanisms behind ET-1-induced PKC inhibition.

Effects of ET-1 Antagonism
Our study also sought to determine whether endothelin blockade with bosentan can prevent ET-1- and CRP-induced impairment in NO homeostasis. The beneficial effects of ET-1 antagonism have previously been observed following ischemia and reperfusion and in cardiac transplantation.^5,33-35 We have previously demonstrated that bosentan enhances endothelial protection during cardiac allograft storage.⁵ In atherosclerotic mice, Barton and coworkers³⁵ also showed that ET-1 blockade restores NO-mediated endothelial function. Li and associates³⁶ have demonstrated that ET-1 antagonism may attenuate CRP-induced endothelial dysfunction. They showed that ET-1 blockade reduces CRP-induced upregulation of lectinlike oxidized low-density lipoprotein receptor-1.³⁶ Our study examined the effect of ET-1 antagonism on CRP-induced impairment of NO homeostasis. However, ET-1 antagonism does not appear to preserve NO production following CRP exposure. When bosentan was given to the CRP + ET groups, the incremental deleterious effect of ET-1 on NO production was eliminated. In our experiments, bosentan failed to inhibit CRP’s effect on eNOS expression; however, it completely abrogated ET-1-induced downregulation. Bosentan exposure resulted in increased PKC activity as well as greater PKC translocation compared with CRP, ET-1, and control. Bosentan’s effects seem to further support the position that PKC is the key isoform involved in NO regulation. In support of this conclusion is the fact that bosentan results in increased NO production although only increases PKC translocation and PKC activity.

The present study demonstrates a potential mechanism behind CRP- and ET-1-induced injury and suggests possible therapeutic strategies. Although bosentan treatment was beneficial in reducing ET-1 injury as well as eliminating the added effect of ET-1 on CRP’s proatherosclerotic effect, it was unable to block CRP-induced endothelial cell injury assessed by decreased NO production. Bosentan may be beneficial in those patients who have both elevated CRP and ET-1 levels, such as patients having cardiac transplant or heart failure. Caution must be taken with bosentan, as we previously found that administration of bosentan can result in severe vasodilation and hypotension, rendering its clinical use problematic. Similarly, despite widespread evidence that ET-1 levels are elevated in congestive heart failure, large randomized clinical trials such as The ENABLE trials (Endothelin Antagonist Bosentan for Lowering Cardiac Events in Heart Failure) also demonstrated a higher rate of sudden death, potentially due to hypotension-related arrhythmias. Therefore, care must be taken with the use of ET-1 antagonism, especially in patients with heart failure. Hence, determining the mechanism of benefit for ET-1 blockade may permit the development of novel targeted therapies without the side effects associated with a nonselective antagonist. The effects of CRP are not mitigated by endothelin antagonism alone. We suggest that PKC modulation may be the optimal strategy to reduce the atherosclerotic burden in patients with elevated acute phase reactants such as CRP and ET-1. The results of these investigations have obvious clinical implications for patients with acute coronary syndrome, post–coronary artery bypass graft patency, and transplant vasculopathy. Further studies are required to assess the potential benefits of PKC modulation in preventing endothelial dysfunction.

	Footnotes

 
Supported by the Heart and Stroke Foundation of Ontario (Grant # NA 5868), the Canadian Institutes for Health Research, the Thoracic Surgery Foundation for Research and Education, the Tailored Advanced Collaborative Training in Cardiovascular Science for Research Fellows, and the Physician Services Incorporated Foundation Grant for Research Fellows. D.R. is a Research Fellow of the TSFRE, PSI and TACTICS; V.R. is a CIHR New Investigator.

Manuscript accepted for the C. Walton Lillehei Resident Forum Session at the Annual Meeting of the American Association for Thoracic Surgery.

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