Quercetin reduces inflammatory responses in LPS-stimulated cardiomyoblasts.

Flavonoids possess several biological and pharmacological activities. Quercetin (Q), a naturally occurring flavonoid, has been shown to downregulate inflammatory responses and provide cardioprotection. However, the mechanisms behind the anti-inflammatory properties of Q in cardiac cells are poorly understood. In inflammation, nitric oxide (NO) acts as a proinflammatory mediator and is synthesized by inducible nitric oxide synthase (iNOS) in response to pro-inflammatory agents such as lipopolysaccharide (LPS), a causative agent in myocardial depression during sepsis. In the present study, we evaluated the protective effect of Q on rat cardiac dysfunction during sepsis induced by LPS. Pretreatment of H9c2 cardiomyoblasts with Q inhibited LPS-induced iNOS expression and NO production and counteracted oxidative stress caused by the unregulated NO production that leads to the generation of peroxynitrite and other reactive nitrogen species. In addition, Q pretreatment significantly counteracted apoptosis cell death as measured by immunoblotting of the cleaved caspase 3 and caspase 3 activity. Q also inhibited the LPS-induced phosphorylation of the stress-activated protein kinases (JNK/SAPK) and p38 MAP kinase that are involved in the inhibition of cell growth as well as the induction of apoptosis. In conclusion, these results suggest that Q might serve as a valuable protective agent in cardiovascular inflammatory diseases.

1. Introduction

Systemic bacterial infection is associated with multiorgan dysfunctions including heart failure, which is the main cause of morbidity and mortality in septic patients [1, 2]. Lipopolysaccharides (LPSs), a major constituent of bacterial outer membrane, have been demonstrated to play a critical role in the initiation of the pathophysiological cascades [3-5]. Under septic conditions, excessive LPS activates numerous types of cells upon recognition by toll-like receptor 4 (TLR-4) resulting in enhanced production of proinflammatory cytokines that contribute to myocardial dysfunction [6-8]. Recent studies have shown that cardiomyoblasts express TLR-4 through which LPS has direct adverse effect on cardiomyocyte physiology [9, 10]. Activation of TLR-4 by LPS triggers NF-κB signaling and results in decreased cardiomyocyte contractility and substantial expressions of proinflammatory cytokines such as intercellular adhesion molecule-1 (ICAM-1) [11, 12], tumor necrosis factor-α (TNF-α) [13, 14], and inducible nitric oxide synthase (iNOS) [13]. The increased expression of iNOS, especially in noninflammatory cells, may have deleterious effects [15-17]. Potential subcellular mechanisms involved in these harmful consequences include excessive direct reactions of NO with a wide variety of proteins and enzymes including reactions with amino, thiol (SH), diazo, and tyrosyl groups, and with heme and Fe2+ or sulfur centers [18]. Moreover, unregulated NO production, also associated with oxidative stress, can result in the generation of peroxynitrite and other reactive nitrogen species (RNS) that alter protein function via nitration and oxidation reactions [16, 19, 20]. It has been demonstrated that reducing systemic inflammatory response could improve myocardial function [21]. Activation of multiple stress signaling processes such as oxidative stress and mitogen-activated protein kinases (MAPKs) plays pivotal roles in the pathogenesis of septic cardiac dysfunction [22]. While activation of ERK1/2 MAP-kinase has been identified to enhance cell growth and migration, the stress-activated protein kinases JNK/SAPK and p38 MAP-kinase are involved in the inhibition of cell growth as well as the induction of apoptosis [23].

Quercetin (Q) is a flavonoid and more specifically a flavonol that possesses a broad range of pharmacological properties, including anti-inflammatory effects [24], antiproliferative effects [25], and protective effects against oxidative stress [26]. Foods rich in quercetin include apples, black and green tea, onions, red wine, red grapes, citrus fruit, broccoli and other leafy green vegetables, cherries, and a number of berries including raspberries and cranberries [27]. Normally, human quercetin plasma concentrations are in the nanomolar range, but after quercetin intake, they may reach the micromolar range [28, 29]. A recent study demonstrated that low to moderate oral dose of quercetin for two weeks increased plasma quercetin concentrations dose-dependently in healthy individuals [30], confirming its bioavailability. In a previous study, we have demonstrated that Q is uptaken by the cardiomyoblast H9c2 cell line and counteracts cardiac oxidative stress via both its well-known antioxidant activity and through the modulation of two key fundamental protein kinases involved in prosurvival signaling pathways, Akt and ERK1/2 [31]. Moreover, we have shown that Q is able to strongly upregulate different antioxidant and phase 2 enzymes in neonatal rat cardiomyocytes demonstrating its indirect antioxidant activity [32].

In this paper, we evaluated the anti-inflammatory effects of Q in cardiac cells, focusing on the possible mechanisms by which this polyphenol counteracts LPS-induced inflammatory responses.

2. Materials and Methods

2.1. Materials

PhosSTOP was purchased from Roche Diagnostics (Mannheim, Germany). CelLytic M, 2′,7′-dichlorodihydrofluorescein diacetate (DCFH-DA), mammalian protease inhibitor mixture, DMEM, fetal bovine serum (FBS), penicillin, streptomycin, L-glutamine, acetyl-Asp-Glu-Val-Asp-7-amido-4-methylcoumarin (Ac-DEVD-AMC), quercetin, and all other chemicals of the highest analytical grade were purchased from Sigma Chemical (St. Louis, MO).

2.2. Cell Cultures

Rat embryonic heart-derived myogenic cell line H9c2 (European Collection of Cell Cultures Salisbury, UK) was grown in DMEM supplemented with 10% heat-inactivated FBS, penicillin (100 U/mL), streptomycin (100 mg/mL), and L-glutamine (2 mM) in a humidified incubator with 5% CO2 at 37°C. Cells were split 1 to 4 at subconfluence (80%). H9c2 cells were seeded at a density of 5 × 104 cells/cm2 72 hours prior to treatments.

2.3. Measurement of Nitric Oxide Production

Released nitrite, a stable product of NO in aqueous medium, was measured using the Griess Reagent System (Promega, Madison, WI, USA). Briefly, H9c2 cells were treated with 30 μM Q for 2 hours prior to stimulation with 10 μg/mL LPS for 24 hours. At the end of this time period, the culture medium was mixed with an equal volume of sulfanilamide solution (1% in 5% phosphoric acid) and of N-1-naphtylethylenediamine dihydrochloride solution (0.1% in water). The absorbance was measured at 540 nm. Nitrite concentrations were determined from a calibration curve of standard 0.1 M sodium nitrite concentrations 0.5–25 μM against absorbance.

2.4. Detection of Intracellular Reactive Oxygen Species

The formation of ROS was evaluated using a fluorescent probe, DCFH-DA, as described by Wang and Joseph [33]. Briefly, H9c2 cells were pretreated with 30 μM Q for 24 h and then incubated with 5 μM DCFH-DA in PBS for 30 min. After DCFH-DA removal, the cells were stimulated with 10 μg/mL LPS for different periods (0.5–24 hours). Cell fluorescence was measured using 485 nm excitation and 535 nm emission with a microplate spectrofluorometer (VICTOR3 V Multilabel Counter, Perkin-Elmer, Wellesley, MA). Intracellular antioxidant activity was expressed as percentage of control cells.

2.5. Caspase-3 Activity Assay

The activity of caspase-3 was measured by hydrolysis of Ac-DEVD-AMC by caspase-3, resulting in the release of the fluorescent 7-amino-4-methylcoumarin moiety (AMC) [34]. H9c2 cells were treated with 30 μM Q for 2 hours prior to stimulation with 10 μg/mL LPS for different periods (0.5–24 hours). Cells were lysated in lysis buffer (50 mM Tris, 0.1% Triton X-100, 150 mM NaCl, 2 mM EGTA/EDTA, 1 mM sodium pyrophosphate, 10 mg/mL phenylmethylsulfonyl fluoride, 1 mM sodium vanadate, 50 mM sodium fluoride, and 1 mg/mL aprotinin) and then centrifuged 5 min at 5,000 g and the supernatant was added to the assay buffer (100 mM HEPES pH 7.0, 5 mM dithiothreitol, 0.1% CHAPS, 10% sucrose, and 0.15 mM Ac-DEVD-AMC). The specific cleavage of the fluorogenic peptide Ac-DEVDA-MC was monitored following AMC cleavage at 370 nm excitation and 455 nm emission. One unit is defined as the amount of enzyme activity cleaving 1.0 nmol of substrate per minute at 25°C under the conditions described.

2.6. Western Immunoblotting

H9c2 cells were treated with 30 μM Q and after 2 hours were stimulated with 10 μg/mL LPS for different periods (0.5–24 hours). Cells were washed with ice-cold PBS and proteins extracted with CelLytic M cell lysis reagent with mammalian protease inhibitor mixture (1 : 100 dilution) and PhosSTOP. Proteins were boiled at 98°C for 3 min in loading buffer (62.5 mM Tris, pH 6.8 containing 2% SDS, 5% 2-mercaptoethanol, 10% glycerol, and 0.0025% bromophenol blue). Protein extracts were separated by SDS-PAGE (20 μg/lane) and then transferred onto nitrocellulose membrane (Hybond-C; GE Healthcare, Buckinghamshire, UK) at 110 V for 90 min using Tris-glycine buffer. Membranes were then incubated in a blocking buffer containing 5% (w/v) skimmed milk and incubated with anti-NOS2, anti-phospho SAPK/JNK (Thr183/Tyr185), anti-SAPK/JNK, anti-phospho p38 MAPK, anti-p38 MAPK (Cell Signaling Technology, Beverly, MA), and anti-β-actin (Sigma), overnight at 4°C on a three-dimensional rocking table. The blots were then incubated with goat anti-rabbit IgG conjugated to horseradish peroxidase for 60 min at room temperature. The results were visualized by chemiluminescence using ECL advance reagent according to the manufacturer's protocol (GE Healthcare). Semiquantitative analysis of specific immunolabeled bands was performed using a Fluor S image analyzer (Bio-Rad, Hercules, CA, USA).

2.7. Protein Concentration

The protein concentration of the cell lysates was determined by the Bio-Rad Bradford protein assay (Bio-Rad Laboratories).

2.8. Statistics

Each experiment was performed at least three times, and all values are represented as means ± SD. One-way analysis of variance (ANOVA) was used to compare differences among groups followed by Bonferroni's test (Prism 5, GraphPad Software Inc., San Diego, CA, USA). Values of P < 0.05 were considered as statistically significant.

3. Results

3.1. Effect of Q on iNOS Expression and NO Production

The first aim of the study was to identify the effect of LPS treatment on iNOS expression (Figure 1). LPS treatment (10 μg/mL) of H9c2 cells for 0.5 hours did not influence iNOS protein expression. On the contrary, LPS stimulation for 2 and 24 hours was able to significantly induce iNOS. In particular, LPS increased the enzyme protein expression in a time-dependent manner (r = 0.9888, P < 0.05). Treatment with 30 μM Q alone for 2 hours had no effect on iNOS protein expression, while pretreatment with Q, prior to LPS exposure, was able to significantly reduce iNOS protein expression at each LPS stimulation time.

Figure 1

Effect of Q on iNOS expression in LPS-stimulated H9c2 cells. Cells were pretreated with 30 μM Q for 2 hours before stimulation with 10 μg/mL LPS. After the indicated time points, cells were harvested and lysed. Crude homogenates (20 μg) were immunoblotted with an antibody that detects endogenous levels of iNOS (NOS2). Equal loading was verified with an anti-β-actin antibody. Densitometric analysis of the protein bands was performed using Bio-Rad Quantity One 1-D Analysis software. Each column represents the mean ± SD of three independent experiments. Data were analyzed by one-way ANOVA followed by Bonferroni's test. *P < 0.05 compared to Control; °P < 0.05 compared to the corresponding LPS exposure times.

We next evaluated total nitrite release as an indicator of NO production (Figure 2). As at 24 hours LPS stimulation had the strongest effect on iNOS protein expression, we used this time to stimulate H9c2. In agreement with the previous results, LPS significantly increased the release of NO in the culture medium, 30 μM Q alone did not influence NO production, and pretreatment with 30 μM Q before LPS stimulation significantly reduced NO production to level comparable to control cells.

Figure 2

Effect of Q on NO production in LPS-stimulated H9c2 cells. Cells were pretreated with 30 μM Q for 2 hours before stimulation with 10 μg/mL LPS for 24 hours. After the treatment, the culture medium was collected for NO assay. The concentration of NO was determined by the Griess reagent using NaNO2 as standard. Each column represents the mean ± SD of three independent experiments. Data were analyzed by one-way ANOVA followed by Bonferroni's test. *P < 0.05 compared to Control; °P < 0.05 compared to LPS.

3.2. Effect of Q on Intracellular ROS Production

To verify if the increase in RNS was accompanied by a concomitant increase in ROS production, we evaluated intracellular ROS accumulation in H9c2 cells stimulated with LPS for different periods in the presence or the absence of 30 μM Q (Figure 3). Intracellular ROS levels were significantly increased in cells stimulated with LPS for 24 hours compared to control cells, as indicated by the increase in DCF fluorescence. However, the increase in DCF fluorescence was significantly decreased by Q pretreatment suggesting that Q was capable of reducing intracellular ROS accumulation following LPS stimulation.

Figure 3

Effect of Q on intracellular ROS production in LPS-stimulated H9c2 cells. Cells were pretreated with 30 μM Q for 2 hours before stimulation with 10 μg/mL LPS. After 24 h intracellular ROS were measured using the peroxide-sensitive fluorescent probe DCHF-DA. Each column represents the mean ± SD of three independent experiments. Data were analyzed by one-way ANOVA followed by Bonferroni's test. *P < 0.05 compared to Control; °P < 0.05 compared to LPS.

3.3. Effect of Q on LPS-Induced Apoptosis in H9c2 Cells

Q demonstrated antiapoptotic effects in different cell types, therefore, we next investigated whether Q protects cardiomyoblasts from LPS-induced apoptosis. H9c2 cells were pretreated with 30 μM Q before exposure to 10 μg/mL LPS for different exposure times and cleaved caspase 3 protein expression (Figure 4) and caspase 3 activity (Figure 5) were evaluated. Immunoblot analyses showed that stimulation with LPS for 24 hours induced a significant cleavage of caspase 3 in respect to control cells, while 0.5 and 2 hours LPS exposure times had no effect on cleaved caspase 3. Pretreatment with Q before LPS stimulation was able to strongly reduce cleavage of caspase 3 to level comparable to control cells. Q alone did not modify caspase 3 cleavage. These data were confirmed by caspase 3 activity assay. Only 24 hours LPS stimulation was able to significantly increase caspase 3 activity and pretreatment with Q significantly reduced caspase 3 activity to level comparable to control cells, demonstrating the antiapoptotic effect of Q against LPS-induced damage.

Figure 4

Effect of Q on cleaved caspase 3 protein expression in LPS-stimulated H9c2 cells. Cells were pretreated with 30 μM Q for 2 hours before stimulation with 10 μg/mL LPS. At the indicated time points, cells were harvested and lysed. Crude homogenates (20 μg) were immunoblotted with an antibody that detects endogenous levels of cleaved caspase 3. Equal loading was verified with an anti-β-actin antibody. Densitometric analysis of the protein bands was performed using Bio-Rad Quantity One 1-D Analysis software. Each column represents the mean ± SD of three independent experiments. Data were analyzed by one-way ANOVA followed by Bonferroni's test. *P < 0.05 compared to Control; °P < 0.05 compared to the corresponding LPS exposure times.

Figure 5

Effect of Q on caspase 3 activity in LPS-stimulated H9c2 cells. Cells were pretreated with 30 μM Q for 2 hours before stimulation with 10 μg/mL LPS. At the indicated time points, caspase 3 activity was measured spectrofluorimetrically in cell lysates as reported in Section 2. Each column represents the mean ± SD of three independent experiments. Data were analyzed by one-way ANOVA followed by Bonferroni's test. *P < 0.05 compared to Control; °P < 0.05 compared to the corresponding LPS exposure times.

3.4. Effect of Q on LPS Activation of MAPK in H9c2 Cells

To better clarify the mechanisms behind Q protection against LPS induced apoptosis, we investigated the role of Q in the modulation of two fundamental proapoptotic signaling pathways in H9c2 cells: JNK and p38 MAPK. H9c2 cells were pretreated with 30 μM Q before exposure to 10 μg/mL LPS for different exposure times and cell lysates were analyzed by immunoblotting with anti-phospho-p38 and anti-p38 antibodies (Figure 6) or anti-phospho-JNK and anti-JNK antibodies (Figure 7). LPS treatment for 0.5 and 2 hours significantly activated p38 MAPK as measured by phospho/total p38 ratio, with the highest increase at 0.5 hours. At the longest exposure time p38, MAPK was no longer activated as phospho/total p38 ratio was comparable to control cells. Q was able to significantly inhibit p38 MAPK activation. LPS treatment for 0.5 hours significantly activated JNK as measured by phospho/total JNK ratio, while after 2 and 24 hours LPS stimulation did not influence JNK phosphorylation. Q was able to significantly reduce JNK activation after 0.5 hours LPS exposure time at level comparable to control cells.

Figure 6

Effect of Q on p38 MAPK activation in LPS-stimulated H9c2 cells. Cells were pretreated with 30 μM Q for 2 hours before stimulation with 10 μg/mL LPS. At the indicated time points, cells were harvested and lysed. Crude homogenates (20 μg) were immunoblotted with anti-phospho-p38 and anti-p38 antibodies. Equal loading was verified with an anti-β-actin antibody. Densitometric analysis of the protein bands was performed using Bio-Rad Quantity One 1-D Analysis software. Each column represents the mean ± SD of three independent experiments. Data were analyzed by one-way ANOVA followed by Bonferroni's test. *P < 0.05 compared to Control; °P < 0.05 compared to the corresponding LPS exposure time.

Figure 7

Effect of Q on JNK activation in LPS-stimulated H9c2 cells. Cells were pretreated with 30 μM Q for 2 hours before stimulation with 10 μg/mL LPS. At the indicated time points, cells were harvested and lysed. Crude homogenates (20 μg) were immunoblotted with anti-phospho-JNK and anti-JNK antibodies. Equal loading was verified with an anti-β-actin antibody. Densitometric analysis of the protein bands was performed using Bio-Rad Quantity One 1-D Analysis software. Each column represents the mean ± SD of three independent experiments. Data were analyzed by one-way ANOVA followed by Bonferroni's test. *P < 0.05 compared to Control; °P < 0.05 compared to the corresponding LPS exposure time.

4. Discussion

In this study, we have evaluated the anti-inflammatory role of Q in H9c2 cells demonstrating that this polyphenol attenuated LPS-induced inflammatory events inhibiting iNOS induction, reducing NO production and oxidative stress, and counteracting apoptosis through the modulation of two key protein kinases p38 MAPK and JNK.

A range of clinical conditions are associated with a dysregulation of inflammatory responses. Although the most common of these is sepsis, high concentrations of cytokines are also generated by ischemia-reperfusion, trauma, acute rejection, antigen-specific immune responses, and different acute inflammatory states [35]. Several studies suggest a beneficial effect for cardiac dysfunction through inhibition of cardiac inflammatory processes in sepsis [13].

LPS of Gram-negative bacteria has been recognized as a causative agent in myocardial depression during sepsis [36]. It has been shown that the inflammatory responses induced by LPS in cardiomyocytes are characterized by an increased production of ROS which leads to the activation of transcription factors and intracellular signaling pathways and to the induction of inflammatory mediators, including TNF-α, ICAM-1, and iNOS. All of these mediators may be involved in the depression of cardiac function [13, 37, 38]. In the cardiovascular system, NO produced by iNOS is a major pathophysiologic mediator of septic shock [39] and has been shown to mediate the negative inotropic effects of cytokines [40]. In agreement with previous studies, performed using cardiomyocytes stimulated with LPS for at least 20 h [41, 42], we demonstrated that iNOS protein expression and NO production were significantly increased in LPS-stimulated H9c2. On the contrary, a study of Chen et al. [43] demonstrated an increase in iNOS mRNA level while NO production was not influenced by a 4 h LPS stimulation in rat cardiomyoblasts. This discrepancy could be ascribed to the lower LPS exposure time that is probably too short to significantly increase NO in the culture medium. In our study, Q treatment was able to significantly reduce both iNOS expression and NO production.

As NO may react with ROS such as the superoxide radical to yield the highly reactive oxidant species peroxynitrite, leading to more aggressive oxidative and nitrosative stress [44], we evaluated the intracellular ROS production in LPS-stimulated H9c2 cells. As expected, LPS significantly increased intracellular ROS level while Q pretreatment was able to reduce this production to level comparable to control cells. We previously demonstrated the ability of Q to reduce oxidative stress in H9c2 cells [31] and in rat cardiomyocytes [32] through both a direct and indirect antioxidant mechanisms.

The action of NO has been related to the induction of programmed cell death, or apoptosis, in various cells [45]. The capacity of NO to induce apoptosis was first appreciated by Albina et al. [46], who showed that NO caused apoptosis in macrophages. Many reports suggest that during the ischemia-reperfusion event, NO mediates tissue injury [47, 48]. Moreover, induction of iNOS by cytokines in primary rat cardiac myocytes was associated with an increased myocytes apoptosis, which was ameliorated by the administration of an inhibitor of NO synthase, which blocked the expression of iNOS in response to cytokines [45]. These results suggest that NO is markedly involved in cardiomyopathy, which leads to the contribution of impaired cardiac function. Our results demonstrated that Q was able to counteract LPS-induced apoptosis by inhibiting caspase-3 activation and significantly reducing caspase-3 activity. Different studies have demonstrated that the mechanism underlying the cytoprotection of Q may be mediated by inhibition of NF-κB activation [44, 49, 50], which controls the expression of inflammatory mediators [51]. A crucial step in the activation of NF-κB is the degradation of IκBa [52]. LPS stimulates the canonical NF-κB activation pathway through degradation of IκBa and phosphorylation of NFκB p65 subunit [53, 54], NF-κB p65 subsequently translocates from the cytoplasm to the nucleus and, in turn, triggers a large amount of genes encoded for inflammatory mediators [54].

The mitogen-activated protein kinase (MAPK) family, including extracellular signal-regulated c-Jun N-terminal kinases 1 and 2 (JNK) and p38 MAP kinases, plays an important role in cell fate decisions and has been implicated in death/survival signaling in cardiac myocytes [55]. Evidence also indicates that ROS contribute to LPS-stimulated MAPKs signaling pathways in myocardial cells [13]. These findings are in line with the crucial role of MAPKs signaling and oxidative stress in sepsis-induced myocardial contractile dysfunction [13, 37, 38]. Data reported in this paper demonstrated that LPS stimulation activates both p38 MAPK and JNK. In particular, JNK activation was quick and transient and after 2 h LPS stimulation JNK phosphorylation was comparable to control cells, while p38 MAPK activation lasted for at least 2 h. Our data are in agreement with the results of Peng et al. [56] that demonstrated an immediate and transient increase in p38 MAPK activation after LPS stimulation, which was followed by TNF-α production in the myocardium and the inhibition of p38 MAPK activation improved cardiac function and survival during endotoxemia in mice. Activation of JNK signal transduction cascades has been implicated in the regulation of hypertrophic and apoptotic responses in the myocardium [57]. Peng et al. [58] showed that LPS increases JNK activation in cultured cardiomyocytes. It has been demonstrated that the activation of JNK/SAPK is crucial for NO toxicity in H9c2 cardiac muscle cells [59], moreover, Liu et al. [60] observed that incubation of LPS-treated myocardial cells with the JNK1/2 inhibitor SP600125 resulted in marked inhibition of LPS-induced phosphorylation of IκB, degradation of IκB and upregulation of TNF-α, leading to myocardial apoptotic responses.

Q pretreatment was able to reduce the activation of the two kinases to values comparable to control cells, demonstrating that the antiapoptotic effect of Q could be also mediated by the modulation of p38 MAPK and JNK whose detrimental role in sepsis has been largely demonstrated.

In conclusion, Q inhibited iNOS induction in LPS-stimulated H9c2 cells in a time-dependent manner, reduced NO production, and counteracted LPS-induced apoptosis. This protective effect might be mediated by the suppression of the activation of p38 MAPK and JNK. Therefore, these results suggest that Q might serve as a valuable protective agent in cardiovascular and inflammatory diseases.