Abstract

Angiotensin converting enzyme inhibitors (ACE-I) are known to affect the endothelial function decreasing the formation of the potent vasoconstrictor angiotensin II and increasing the bioavailability of the vasodilators bradykinin and nitric oxide. In order to test the potential differences among the class of ACE-I, we have evaluated their effects on endothelin-1 and nitric oxide availability, and on reactive oxygen species generation in human vascular endothelial cells (HUVECs) obtained from umbilical cord veins. HUVECs were cultured in the presence of either sulfhydryl-containing ACE-I (zofenoprilat or captopril) or nonsulfhydryl-containing ACE-I (enalaprilat or lisinopril). After 24 hours, all ACE-I reduced endothelin-1 secretion and increased nitric oxide production. However, zofenoprilat ( 42% after 8 hours of incubation) was more effective ( ) than enalaprilat ( 25%), lisinopril ( 21%), and captopril ( 30%) in reducing endothelin-1 secretion. Similarly, zofenoprilat (+110% after 8 hours of incubation) was more effective ( ) than enalaprilat (+64%), lisinopril (+63%), and captopril (+65%) in increasing nitrite plus nitrate production. The effect of ACE-I on the nitric oxide availability and on endothelin-1 secretion is mediated by the activation of bradykinin receptor being reverted, at least in part, by a specific antagonist. Zofenoprilat and, to a lesser extent, captopril also blunted tumour necrosis factor (TNF) -stimulated production of reactive oxygen species and decreased TNF -stimulated glutathione consumption in endothelial cells. In conclusion, structural differences among the class of ACE-I play a role in their interaction with mediators that influence the homeostasis of the endothelium. The marked antioxidant effects exerted by zofenoprilat due to its sulphydryl group and lipophilia seem to be responsible for its greater endothelium protective activity.

1. Introduction

Angiotensin converting enzyme (ACE), also known as kininase II, is a bivalent dipeptidyl carboxyl metallopeptidase present both as a membrane-bound form in epithelial, neuroepithelial, and endothelial cells, including the vascular ones, and as a soluble form in different body fluid, including blood [1]. Due to its ability to cleave the C-terminal dipeptide from a number of peptides, ACE can either convert the inactive decapeptide angiotensin I to the active octapeptide angiotensin II or inactivate kinins [1]. Thus, ACE strategically modulates the balance between the vasoconstrictive and salt-retentive renin-angiotensin system and the vasodilatory and natriuretic kallikrein-kinin one [1]. As a consequence, after the initial use as antihypertensive drugs [2], ACE-inhibitors (ACE-Is) rapidly became a fundamental tool also in treating congestive heart failure, left ventricular dysfunction after myocardial infarction, diabetic and nondiabetic nephropathies [24].

Despite of the successful use in all of the above conditions, the mechanisms responsible for the vascular benefits exerted by ACE-I are not fully understood. ACE-I are able to improve both endothelium-dependent [5] and endothelium-independent [6] vascular relaxation. However, the endothelial effects of ACE-I are not only dependent on decrease of angiotensin II formation and increase of bradykinin bioavailability [2, 5, 6]. In this regard, it has been suggested that the vascular action of ACE-I could be also related to their ability to reduce production of endothelin-1 (ET-1) [7], one of the most potent vasoconstrictor [8], through an increased nitric oxide (NO) production [7, 9] leading to a down-regulation of ET-1 gene expression [9].

In this regard, sulfhydryl containing ACE-I can act as antioxidants by scavenging superoxide anion [10] as well as nonsuperoxide radicals [11]. Since unscavenged superoxide anion quenches NO to give the pro-oxidant compound peroxynitrite [12], which is unable to down-regulate (or even up-regulates) ET-1 gene expression, sulfhydryl containing ACE-I could be particularly effective in decreasing ET-1 secretion by cultured HUVECs in increasing NO production [13].

To address this topic, we compared the effects of zofenoprilat and captopril, that are, two sulfhydryls containing ACE-I, with those of enalaprilat and lisinopril, two nonsulfhydryls containing ACE-I, on ET-1 secretion and NO production by human vascular endothelial cells (HUVECs). In addition, to assess the ACE-I antioxidant properties, their effects on intracellular content of the endogenous free radical scavenger reduced glutathione (GSH) [14, 15] and the generation of reactive oxygen species were also evaluated.

2. Materials and Methods

2.1. Cells

HUVECs were harvested from fresh human umbilical cord veins cultured until the third passageas previously described [7, 16, 17]. The purity of the endothelial cell monolayer was confirmed by their cobblestone morphological pattern and by cell staining with a monoclonal antibody specific for von Willebrand factor [17]. Newly confluent cells in culture medium were lifted with trypsinization; the trypsin was inhibited with 20% foetal calf serum, and cells were washed in culture medium. After 10 minutes of centrifugation (1100 rpm, C), the supernatant was removed and HUVECs were resuspended in culture medium (3 mL) and then used for the experiments.

HUVECs were incubated either with zofenoprilat (the active form of zofenopril), or enalaprilat (the active form of enalapril), or lisinopril or captopril for various times up to 24 hours. The above experiments were repeated in the presence of either bradykinin, or , that is, a bradykinin receptor antagonist, or , that is, a bradykinin receptor antagonist. Finally, experiments were also repeated in the presence of the NO synthase competitive inhibitor -nitro-L-arginine methyl ester (L-NA).

Zofenoprilat was obtained from Menarini Ricerche SpA, Firenze, Italy. Angiotensin II was purchased by Clinalfa (Laufelfingen, Switzerland). The other reagents were purchased by Sigma (St Louis, Mo, US). If it is not otherwise specified, all the tested substances have been added to culture medium to a final concentration of , a concentration that fully inhibited the human recombinant ACE for all the antagonists under study [18].

2.2. Endothelin-1

The peptide was assayed as previously described [16]. In brief, the culture medium derived from each well was centrifuged at 3.000 rpm for 10 minutes. The supernatant was subsequently freeze-dried, reconstituted in starting high performance liquid chromatography buffer, injected onto columns (Pharmacia, Uppsala, Sweden), and eluted over 70 minutes using a linear gradient of 15–75% acetonitrile/0.1% trifluoroacetic acid in water. Fractions were collected each minute and evaporated before reconstitution in assay buffer (50 mmol/L phosphate buffer, pH 7.4, containing 0.9% NaCl, 0.05% , and 0.5% bovine serum albumin). Endothelin-1 immunoreactivity was then assayed on reconstituted samples by a sensitive radioimmunoassay (Peninsula Laboratories, Belmont, Calif, USA). Interassay and intra-assay variations were <10%. Cross-reactivity of the ET-1 antibody with endothelin-2 and endothelin-3 was <7%, according to the supplier.

2.3. Nitric Oxide

NO production by HUVECs was assessed by evaluating the concentration of NO metabolite ( ), that is, nitrite plus nitrate, in culture medium. Briefly, concentrations were evaluated by colorimetric detection of nitrite after conversion of all sample nitrate to nitrite (Assay Design Inc., Ann Arbor, Mich, USA) as previously described [7].

2.4. Measurements of Intracellular Glutathione Redox Status and Oxidative Stress

Intracellular glutathione (GSH) concentration was measured according to the method previously described by our group [15]. In brief, HUVECs were firstly diluted in 1 mL isotonic saline + HCl (10 mmol/L) and then lysed in acetone, thawed four times, and centrifuged for 15 minutes at C. Supernatants were deproteinized with 10% 5-sulfosalicylic acid and used for total GSH determination, that is, glutathione (GSH) + GSH disulphide (GSSG), by the enzymatic method described by Anderson [19]. For GSSG determination, 0.1 mL deproteinized supernatants were treated with 2 μL 2-vinylpyridine, neutralized with triethanolamine at a final pH of 6.5 and assayed after 1 hour incubation. Then, endothelial cell GSH content was calculated by subtracting GSSG from total intracellular GSH concentrations.

Intracellular oxidative stress was measured at baseline and after incubation with tumour necrosis factor (TNF)α according to Wu and Juurlink’s method [14]. In brief, cultured HUVECs were loaded with the permeable agent 5-(6)-carboxy- - -dichlorodihydrofluorescein (DCHF) ester for 60 minutes. In the presence of intracellular esterases permeable DCHF ester is converted to its impermeable counterpart. This latter is oxidized to the fluorescent DCF by strong oxidants such as hydroxyl radicals [15, 20]. Then, intracellular oxidative stress was quantified by monitoring DCF content in HUVECs with fluorimeter with excitation at 495 nm and emission at 525 and expressed as percent of control.

2.5. Statistical Analysis

Changes in migration were analyzed by ANOVA followed by Bonferroni’s test. Multiple comparisons were analyzed by ANOVA followed by post hoc analysis to adjust the significance level. Statistical significance was considered as . Data are given as the mean ±SD of four experiments.

3. Results

3.1. ACE-I Counteracts Endothelin-1 Secretion by HUVEC: Evidence of Different Pathway

All tested ACE-I at reduced spontaneous ET-1 secretion by HUVECs to a level which was similar to that induced by bradykinin (see Figure 1(a)). Preincubation with the bradykinin receptor antagonist but not the bradykinin receptor antagonist both at abolished the inhibitory effect of ACE-I on ET-1 secretion by HUVECs (see Figures 1(b)–1(f)). These data suggested that bradykinin receptor stimulation was involved in the inhibitory effect of the four tested ACE-Is on ET-1 secretion. Although all the four tested drugs counteracted spontaneous ET-1 secretion by HUVECs, zofenoprilat was more effective than the other ACE-I in this setting. In addition, the inhibitory effect of zofenoprilat on ET-1 secretion was only partially counteracted by bradykinin receptor inhibition (see Figure 1(c)). This finding indicated that bradykinin receptor stimulation does not represent the only pathway involved in the inhibitory effect of zofenoprilat on ET-1 production by HUVECs.

3.2. Increased NO Availability Is Responsible for the Inhibitory Effect of ACE-I on Endothelin-1 Secretion by HUVECs

All tested ACE-I at and bradykinin at significantly increased spontaneous concentrations in culture medium (see Figure 2(a)). ACE-I and bradykinin related changes in concentrations were counteracted by previous incubation of HUVECs with the bradykinin receptor antagonist at (see Figures 2(b)–2(f)) while the bradykinin receptor antagonist at was completely ineffective in this setting (see Figures 2(b)–2(f)). The preincubation of HUVECs with the NO synthase inhibitor L-NA at completely abolished the effects of ACE-I and bradykinin on production (see Figures 2(b)–2(f)). In addition, L-NA also counteracted the inhibitory effect of ACE-I on ET-1 production (see Figures 1(b)–1(f)). These data suggest that increased NO production plays a pivotal role in the inhibitory effect of ACE-I on endothelin-1 secretion by HUVECs.Although all four tested ACE-I were effective in increasing concentrations in culture medium, this effect was more evident in the presence of zofenoprilat (see Figure 2(a)). In addition, bradykinin receptor inhibition was only partially effective in counteracting zofenoprilat-induced increment of concentrations in culture medium (see Figure 2(c)).

3.3. ACE-I Reduces Intracellular Oxidative Stress and Increases GSH Content

HUVECs preincubation with of zofenoprilat and captopril, but not with enalaprilat and lisinopril, was resulted in a significant decrease of TNFα-stimulated generation of reactive oxygen species (see Figure 3(a)). Although both sulfhydryls containing ACE-I reduced TNFα-stimulated reactive oxygen species generation in cultured HUVECs, zofenoprilat was more effective than captopril in this setting (see Figure 3(a)). In keeping with this, zofenoprilat but not captopril, lisinopril, and enalaprilat significantly protected HUVECs against the GSH decrease observed after incubation with TNFα (see Figure 3(b)).

4. Discussion

The ability of ACE-I to counteract ET-1 production by endothelial cells [7, 9] has been proposed as a relevant contributor to the well-known vascular protective effects exerted by ACE-inhibition [7, 21]. Indeed, although tonic ET-1 production by endothelial cells physiologically contributes to vascular tone [21, 22], this peptide has per se all the biological potential to contribute to the onset and progression of atherosclerotic vascular damage [8, 21]. The current report provides evidence that ACE-I, tested at concentrations that fully inhibited the ACE, do not share in common similar efficacy in counteracting ET-1 release from vascular endothelial cells. Indeed, we found that zofenoprilat was more effective than captopril, lisinopril, and enalaprilat in reducing ET-1 secretion from cultured HUVECs. In addition, our data demonstrate that different intracellular pathways are involved in the inhibitory effects of the four tested ACE-Is on ET-1 secretion. In this context, it has been previously demonstrated that the inhibitory effect of ACE-I on ET-1 production by HUVECs is due to a bradykinin receptor-mediated increase in NO production by HUVECs [9].

As known, oxygen derived free radical can inactivate NO [12]. In turn, NO represents a barrier against oxidants such as unscavenged superoxide anion [23]. Thus, it is reasonable to speculate that the greater effects observed with zofenoprilat in reducing ET-1 secretion and increasing NO production by cultured HUVECs might have been due to its antioxidant properties [11, 24]. In keeping with this, zofenoprilat and at lesser extent captopril, but not lisinopril and enalaprilat, were able to decrease generation of reactive oxygen species induced by TNFα in HUVECs. Further, zofenoprilat but not the two nonsulfhydryl containing ACE-I lisinopril and enalaprilat blunted the GSH decrease in HUVECs induced by TNFα. Since sulfhydryls containing ACE-I are supposed to act as antioxidants as the endogenous free radical scavenger GSH [2, 10, 11], both these findings suggest that the sulfhydryl group can be the responsible for the effect of zofenoprilat in reducing ET-1 production, that is, because of sulfhydryl-related scavenging capability and the consequent decrease in NO inactivation by endogenous oxidants. In agreement with this hypothesis, Cominacini et al. [24] demonstrated that zofenoprilat, but not enalapril, protected the intracellular proinflammatory pleiotropic mediator nuclear factor κB against oxidant-induced activation and was able to spare GSH from consumption induced by oxLDL. Likewise, sulfhydrylic ACE-Is have been reported to protect cultured endothelial cells against the damage induced by both superoxide and nonsuperoxide radicals [11] and to decrease LDL susceptibility to oxidation in hypertensive patients [25, 26].

However, the presence of a sulphydryl group in zofenoprilat molecule does not completely explain our findings. Indeed, the other sulfhydryl containing ACE-I tested in our study, captopril, was mildly but not significantly more effective than lisinopril and enalaprilat in our tests. These data agree with previous findings obtained in leucocytes and endothelial cells, demonstrating that captopril poorly scavenged newly generated superoxide anion [27, 28]. In this regard, zofenoprilat displays higher lipophilicity than captopril, suggesting it could exert more pronounced intracellular effects [18]. Worth mentioning in this regard, the recent evidence by Soardo et al. [29] demonstrating a stronger inhibitory effect of zofenoprilat on alcohol-induced ET-1 production by endothelial cells in comparison to carvedilol, a beta adrenoceptor blocker with known antioxidant activity [30].

In conclusion, the sulfhydryl containing ACE-I zofenoprilat, that is, the active drug of the prodrug zofenopril [18], was more effective than the nonsulfhydryl containing ACE-I lisinopril and enalapril and the sulfhydryl containing one captopril in reducing ET-1 secretion by cultured HUVECs and improving NO bioavailability. These findings likely reflect different antioxidant power between the four tested ACE-Is. Since both increased ET-1 production and decreased NO bioavailability are deeply involved in the pathophysiology of atherosclerosis [22], reciprocal changes in ET-1 and NO production by the vascular endothelium could contribute to the benefits deriving from clinical use of ACE inhibitors [2]. The presence of a sulfhydryl group confers to ACE inhibitors some ancillary properties, such as greater protection against LDL oxidation [26] and nuclear factor κB activations [24], scavenging of superoxide anion [10] and nonsuperoxide radical [11], and, as demonstrated in this study, more pronounced favourable effects on ET-1/NO balance in vascular endothelial cells. Whether or not these endothelial effects of zofenoprilat could contribute to the observed cardiovascular benefits deriving from zofenopril treatment [31] remains to be elucidated.

Acknowledgment

The authors thank Miss Maria Greco for her secretarial assistance.