Disturbances in nitric oxide synthase (NOS) and cyclooxygenase (COX) isozyme systems, manifested by the excessive NO and prostaglandin (PGE 2) generation, are well-recognized features of gastric mucosal inflammatory responses to H. pylori infection. In this study, we report that H. pylori LPS-induced enhancement in gastric mucosal inducible (i) iNOS expression and COX-2 activation was accompanied by the impairment in constitutive (c) cNOS phosphorylation, up-regulation in the inhibitory κB kinase- β (IKK β) activation and the increase in the transcriptional factor, NF- κB, nuclear translocation. Further, we show that abrogation of cNOS control over NF- κB activation has lead to induction of iNOS expression and COX-2 activation through S-nitrosylation. Moreover, we demonstrate that the modulatory effect of peptide hormone, ghrelin, on the LPS-induced changes was reflected in the increase in Src/Akt-dependent cNOS activation through phosphorylation and the suppression of IKK- β activity through cNOS-mediated IKK- β protein S-nitrosylation. As a result, ghrelin exerted the inhibitory effect on NF- κB nuclear translocation, thus causing the repression of iNOS gene induction and the inhibition in COX-2 activation through iNOS-dependent S-nitrosylation. Our findings point to cNOS activation as a pivotal element in the signaling cascade by which ghrelin exerts modulatory control over proinflammatory events triggered in gastric mucosa by H. pylori infection.
Infection with Helicobacter pylori is a primary factor in the etiology of gastric disease, and the excessive nitric oxide (NO) and prostaglandin (PGE2) generation along with up-regulation in proinflammatory cytokine production, are well-documented features of H. pylori-induced gastritis as well as characterize gastric mucosal inflammatory responses to H. pylori lipopolysaccharide (LPS) [1-4]. While NO and PGE2 generated by the constitutive (c) nitric oxide synthase (cNOS) and cyclooxygenase-1 (COX-1) enzymes are responsible for maintaining normal physiological functions, and are recognized as essential elements of gastric mucosal defense mechanism, the overexpression of inducible (i) iNOS and cyclooxygenase-2 (COX-2) has been intimately implicated as the promoting event in H. pylori-associated chronic gastritis and gastric cancer [2,4-6].
A growing body of evidence, moreover, supports the existence of a functional and signaling relationship between NO generated by NOS isozyme system, and the formation of PGE2 synthesized from arachidonic acid by the action of COX systems [7-10]. The cross-talk between the products of NOS and COX pathways is supported by the studies indicating that stimulation of NO production through iNOS induction leads to COX enzymes activation and the increase in PGE2 generation, whereas NOS gene deletion or inhibition of NOS enzymes with pharmacological agents results in a decrease in PGE2 formation [9-12]. The role of cNOS in the iNOS-dependent COX-2 activation has also been suggested [10,13], and we have reported that the disturbances in NO and PGE2 generation elicited by H. pylori LPS are reflected in the massive up-regulation of iNOS and COX-2 activity, and the suppression in Src/Aktdependent cNOS activation [14-16].
Investigations into LPS-induced signaling events underlying the expression of proinflammatory mediators indicate that H. pylori LPS, like LPS of other Gram-negative bacteria, is known to trigger the activation of tolllike receptor-4 (TLR-4), which through downstream effectors leads to activation of transcriptional factors involved in iNOS and COX-2 gene induction [10,12,17,18]. While the induction of iNOS gene expression in response to LPS involves activation of transcriptional factor NF- κB [8,10,19], the role of NF-κB in the transcriptional control of COX-2 expression is less apparent and remains controversial [17,18,20]. Depending on the cell type, the regulation of COX-2 expression has been attributed to transcriptional factors, NF-κB, activator protein-1 (AP-1), cAMP response element biding protein (CREB), and CCATT/enhancer binding protein (C/EBP), as well as kinases of MAPK and PKC family [10,12,18, 20,21]. Moreover, up-regulation in COX-2 activation has been linked to posttranslational modification of the enzyme protein through S-nitrosylation via LPS-elicited induction in iNOS expression [9,10]. Indeed, as demonstrated recently, the induction in iNOS expression by H. pylori LPS leads to COX-2 S-nitrosylation that results in an excessive PGE2 generation [
In this study, we investigated further the role of cNOS in the signaling cascade of H. pylori LPS-induced expression of iNOS and COX-2 in gastric mucosal cells. Our results demonstrate that the LPS-induced abrogation of cNOS control over NF-κB activation results in the induction of iNOS expression and leads to COX-2 activation through S-nitrosylation. Moreover, our results show that peptide hormone, ghrelin, recognized for its modulatory control over NOS and COX enzyme systems [16,22-25], suppresses these untoward consequences of the LPS through up-regulation in cNOS activation that interferes with NF-κB nuclear translocation, thus causing the repression of iNOS gene induction and the inhibition of COX-2 activation through iNOS-dependent S-nitrosylation.
The cells were collected form the mucosa of freshly dissected rat stomachs with a blunt spatula, and suspended in five volumes of ice-cold Dulbecco’s modified (Gibco) Eagle’s minimal essential medium (DMEM), supplemented with fungizone (50 µg/ml), penicillin (50 U/ml), streptomycin (50 µg/ml), and 10% fetal calf serum. The cells were then gently dispersed by trituration with a syringe, settled by centrifugation, and following rinsing resuspended in the medium to a concentration of 2 × 107 cell/ml [
Nitric oxide synthase activities of cNOS and iNOS enzymes in the gastric mucosal cells were measured by monitoring the conversion of L-[3H] arginine to L-[3H] citrulline using NOS-detect kit (Stratagene). The cells from the control and experimental treatments were homogenized in a sample buffer containing either 10 mM EDTA (for Ca2+-independent iNOS) or 6 mM CaCl2 (for Ca2+- depenedent cNOS), and centrifuged. The aliquots of the resulting supernatant were incubated for 30 min at 25˚C in the presence of 50 µCi/ml of L-[3H] arginine, 10 mM NAPDH, 5 µM tetrahydrobiopterin, and 50 mM Tis-HCl buffer, pH 7.4, in a final volume of 250 µl. Following addition of stop buffer and Dowex-50 W (Na+) resin, the mixtures were transferred to spin cups, centrifuged and the formed L-[3H] citrulline contained in the flow through was quantified by scintillation counting [
The cyclooxygenase activity of COX-1 and COX-2 isoforms in gastric mucosal cells was measured with the COX Activity Assay Kit (Cayman) by monitoring the appearance of oxidized TMPD at 590 nm [
The aliquots of gastric mucosal cell suspension from the control and various experimental conditions were settled by centrifugation at 1500 × g for 5 min, rinsed with phosphate-β uffered saline, and lysed by incubation for 10 min on ice in the lysis buffer, containing 10 mM HEPES, pH 7.9, 10 mM KCl, 0.1 mM EDTA, 0.5% Nonidet P-40, 1 mM dithiothreitol, and 0.5 mM PMSF [
2.5. IκB Kinase Activity Assay To measure the IKK-β activity we utilized the ELISAbased detection kit, K-LISATM (Calbiochem). The GSTIκB-α 50-amino acid peptide that includes the Ser32 and Ser36 of IκB-α phosphorylation sites was used as a substrate [
A biotin switch procedure was employed to assess IKK-β and COX-2 protein S-nitrosylation [28,29]. The gastric mucosal cells were treated with ghrelin (0.5 µg/ml), or Akt inhibitor, SH-5 (20 µM) + ghrelin (0.5 µg/ml), and incubated in the presence of 100 ng/ml of H. pylori LPS. Following centrifugation at 500 × g for 5 min, the recovered cells were lysed in 0.2 ml of HEN lysis buffer (250 mM HEPES, 1 mM EDTA, 0.1 mM neocuprin, pH 7.7), and the unnitrosylated thiol groups were blocked with S-methyl methanethiosulfonate reagent at 50˚C for 20 min [
The mucosal cells from the control and experimental treatments were collected by centrifugation and resuspended for 30 min in ice-cold lysis buffer (20 mM TrisHCl, pH 7.4, 150 mM NaCl, 10% glycerol, 1% Triton X- 100, 2 mM EDTA, 1 mM sodium orthovanadate, 4 mM sodium pyrophosphate, 1 mM PMSF, and 1 mM NaF), containing 1 µg/ml leupeptin and 1 µg/ml pepstatin [
All experiments were carried out using duplicate sampling, and the results are expressed as means ± SD. Analysis of variance (ANOVA) and nonparametric KruskalWallis tests were used to determine significance. Any difference detected was evaluated by means of post hoc Bonferroni test, and the significance level was set at P < 0.05.
Infection of gastric mucosa by H. pylori in humans or stimulation of gastric mucosal cells with H. pylori LPS elicits a rapid proinflammatory reaction characterized by the excessive NO and PGE2 generation caused by the disturbances in NOS and COX isozyme systems [1-4,16]. Hence, to further ascertain the nature of the disturbances, we first assessed the time course of protein expression and the activity of NOS and COX isozyme systems in rat gastric mucosal cells exposed to H. pylori LPS. The results revealed that the LPS (100 ng/ml) elicited a significant induction in COX-2 (
pression of COX-1 (
Moreover, we established that preincubation of gastric mucosal cells with peptide hormone, ghrelin, lead to a concentration-dependent suppression of the LPS-induced COX-2 (
tion at Ser1179 (
Hence, to provide further leads as to the requirements for iNOS-dependent up-regulation in COX-2 activation by H. pylori LPS, the mucosal cells prior to incubation with ghrelin were pretreated with the inhibitors of cNOS phosphorylation, an Akt inhibitor, SH-5 and Src inhibitor, PP2, and assayed for COX-2 and iNOS activity. As shown in
of NF-κB activation, while showing no inhibitory effect on the LPS-induced expression of COX-2 protein, caused a marked inhibition in the LPS-induced expression of iNOS protein (
Therefore, to understand the mechanism underlying up-regulation in COX-2 activation, we examined the effect of ghrelin on the LPS-induced NF-κB activation. As NF-κB activation requires degradation of the inhibitory protein IκB-α that leads to translocation of p65 component of NF-κB from the cytoplasm to nucleus [30 -33], we exposed the gastric mucosal cells to H. pylori LPS in the absence or presence of ghrelin, and the cell lysates were analyzed for IκB-α level, while the nuclear extracts were assessed for p65 NF-κB. The results of immunoblots analysis revealed that, the LPS effect was manifested by a distinct reduction in IκB-α protein level and a marked increase of p65 in the nuclear extract (
Next, we analyzed the influence of ghrelin on H. pylori LPS-induced changes in the activity of IKK-β, a key enzyme of NF-κB activation pathway that controls the extent of IκB-α phosphorylation and its proteasomal degradation. The results revealed that ghrelin exerted a profound countering effect on the LPS-induced up-regulation in gastric mucosal cell IKK-β activity (
Moreover, the effect of ghrelin on LPS-induced upregulation in IKK-β activity was subject to suppression by the inhibitors of Src/Akt pathway, PP2 and SH-5. A significant decrease in the countering effect of ghrelin on the LPS-induced up-regulation in IKK-β activity was also attained in the presence of cNOS inhibitor, LNAME, while the inhibitor of NF-κB activation, PPM-18, and iNOS inhibitor, 1400 W, had no effect. This indicates that the countering effect of ghrelin on H. pylori LPSinduced up-regulation in gastric mucosal IKK-β activation, and the suppression of COX-2 and iNOS enzymes,
occurs with the involvement of Src/Akt-mediated cNOS activation, and shows dependence on NO generated by the cNOS system.
Consequently, to reveal further the role of NO generated by cNOS isozyme system in the regulation of the LPS-induced IKK-β and COX-2 activation, we assessed the effect of nitrosothiols reducing agent, ascorbate. While preincubation with ascorbate produced no discernible effect on the extent of the LPS-induced IKK-β activation, a marked decrease was observed in the LPS-induced COX-2 activation (
induction and hence leads to the inhibition of COX-2 activation through iNOS-dependent S-nitrosylation.
Colonization of gastric mucosa by H. pylori in humans or stimulation of gastric mucosal cells with H. pylori LPS is known to elicit a cascade of inflammatory responses resulting in the release of proinflammatory mediators that increase the risk of gastric disease [2,4-6,14]. Primary among these mediators, is up-regulation in proinflammatory cytokine production and the excessive generation of NO and PGE2 [2,4,14,16]. While the NO and PGE2 generated by the constitutive cNOS and COX-1 enzyme systems are deemed essential for the maintenance of normal housekeeping functions, the overexpression of inducible iNOS and COX-2 isozymes, and consequent increase in NO and PGE2 production, are considered of major importance in defining the extent of gastric mucosal inflammatory involvement [4,5,16]. The signaling events underlying the induction of iNOS and COX-2 enzymes by bacterial LPS involves the stimulation of TLR-4, which then through a series of downstream effectors triggers the activation of transcriptional factors that exert control over iNOS and COX-2 gene expression [10,17,18,34,35]. Principal among the factors implicated in the regulation of inflammatory responses to H. pylori, is the nuclear transcriptional factor, NF-κB [34-36]. While the induction of iNOS gene by LPS has been convincingly linked to NF-κB activation [10,19, 26,30], the role of NF-κB in COX-2 gene expression remains less apparent [17,18,20]. Hence, in the present study we assessed the relationship between H. pylori LPS-induced NF-κB activation, iNOS gene induction, and COX-2 activation.
Our data, obtained with rat gastric mucosal cells, revealed that the LPS-elicited enhancement in the expression of iNOS COX-2 is accompanied by the impairment in cNOS phosphorylation, up-regulation in IKK-β activation, and the increase in NF-κB nuclear translocation. Further, we demonstrated that abrogation of cNOS control over NF-κB activation and its nuclear translocation leads to induction in iNOS expression, and COX-2 activation through S-nitrosylation. Moreover, we showed that ghrelin modulates the LPS-induced changes by exerting the inhibitory effect on NF-κB nuclear translocation, thus causing repression of iNOS gene and the inhibition of COX-2 activation through iNOS-dependent Snitrosylation. Indeed, examination of gastric mucosal cell expression of COX and NOS proteins and the activity of the individual isozymes demonstrated that H. pylori LPS-induced enhancement in iNOS and COX-2 enzymatic activities was associated with the induction in iNOS and COX-2 protein levels. The LPS, however, had no apparent effect on the expression of COX-1 and cNOS proteins, and COX-1 activity, while the activity of cNOS showed a marked decrease. Furthermore, assessment of the effect of peptide hormone, ghrelin, revealed that the induced increase in cNOS phosphorylation at Ser1179 was associated with a significant up-regulation in cNOS activity, inhibition of iNOS expression, and the suppression in COX-2 activity without affecting its protein expression. These findings are thus in concordance with the rapidly accumulating literature data attesting to a central role of ghrelin in modulation of gastric mucosal inflammatory responses to H. pylori colonization [14-16, 22-25], as well as point to cNOS activation through phosphorylation as a pivotal element of ghrelin signaling cascade.
The mechanism that underlies the regulation of NOS system by ghrelin involves the receptor (GHSR1a)- mediated activation of heterotrimeric G protein-dependent pathway that results in signal propagation through a multiple network of protein kinases, including that of Src/ Akt cascade that controls the process of cNOS activation [14,15,24,37,38]. Indeed, we found that in keeping with the documented involvement of Src/Akt in posttranslational cNOS activation through phosphorylation at Ser1179 [37,38], the countering effect of ghrelin on the LPS-induced up-regulation in COX-2 and iNOS activation was susceptible to suppression by Akt inhibitor, SH- 5, as well as Src inhibitor, PP2. Moreover, the LPS-induced increase in COX-2 and iNOS activity displayed susceptibility to PPM-18 and Bay 11-7082, the inhibitors of NF-κB activation with different mechanism of action [39,40]. However, while this inhibitory effect on iNOS activity was also reflected in a marked suppression in the expression of iNOS protein, neither PM-18 nor Bay 11-7082 affected the LPS-induced expression of COX-2 protein. Hence, considering the fact that PPM-18 is a potent blocker of NF-κB binding to its nuclear promoter response elements [
Indeed, our studies confirmed an important role for ghrelin in the inhibition of NF-κB activation in response to H. pylori LPS-induced up-regulation in iNOS expression. NF-κB is a rapid transcriptional activator that is held in the cytoplasm of resting cells bound to a family of inhibitory IκB proteins. Upon stimulation by LPS or TNF-α, IκB undergoes phosphorylation at two critical serine residues by the an IκB kinase (IKK) complex, which targets IκB for degradation through the ubiquitinproteasomal pathway and leads to nuclear translocation of NF-κB, its biding to promoter response elements, and activation of the target gene transcription [30-34]. In concordance with this classical pathway of NF-κB activation [35,41], we have shown that the effect of H. pylori LPS was manifested by a distinct reduction in the inhibitory protein, IκB-α and a marked increase in p65 NF- κB nuclear translocation, whereas in the presence of ghrelin, the extent of the LPS-induced IκB-α degradation and the nuclear translocation of NF-κB decreased significantly. Moreover, we found that countering effect of ghrelin on the LPS-induced up-regulation in gastric mucosal cell IKK-b activity was subject to suppression by the inhibitors of Src/Akt pathway, PP2 and SH-5. A significant decrease in the effectiveness of ghrelin to counter the LPS-induced IKK-b activation was also observed in the presence of cNOS inhibitor, L-NAME, while the inhibitor of NF-κB activation, PPM-18, and iNOS inhibitor, 1400W, had no effect. From this, we inferred that the countering effect of ghrelin on H. pylori LPS-induced up-regulation in gastric mucosal IKK-b activation, as well as COX-2 and iNOS enzyme suppression, occurs with the involvement of Src/Akt-mediated cNOS activation, and shows dependence on NO generated by the cNOS. In this connection, it is pertinent to reiterate that signaling through Src/Akt pathway is known to occupy a central stage in the receptor (GHSR1a)-mediated responses to ghrelin stimulation [14,15, 24,38]. Deserving equally insightful consideration in furthering our understanding the signaling pathways of ghrelin are the reports indicating that the activity of IKK-β complex as well as that of COX-2 protein may also be regulated through S-nitrosylation [9,10,33,42- 44].
Indeed, as demonstrated recently, the induction in iNOS expression by LPS leads to COX-2 S-nitrosylation that result in an excessive PGE2 generation [9,10,16], and S-nitrosylation of a specific cysteine residue within the activation loop of IKK-β by endogenous NO donors eerts the inhibitory effect on the extent of IκB-α degradation, and hence affects the nuclear translocation of NF- κB [33,42,44]. Hence, to examine further the role of cNOS in the regulation of H. pylori LPS-induced IKK-β and COX-2 activation by ghrelin, we assessed the effect of nitrosothiol reducing agent, ascorbate. While preincubation with ascorbate produced no discernible effect on the extent of the LPS-induced IKK-β activation, a marked decrease was observed in the LPS-induced COX- 2 activity. Moreover, ascorbate elicited an amplification in the inhibitory effect of ghrelin on COX-2 activity and produced a significant relieve in the inhibitory effect of ghrelin on the LPS-induced IKK-β activity. Therefore, consistent with our findings, the regulation of IKK-β activity as well as the activation of COX-2 appears to be intimately linked to the events of S-nitrosylation by NO generated by the cNOS system. This contention is supported further by the results of biotin switch assay [28, 29]. Western blot analysis of COX-2 and IKK-β protein S-nitrosylation patterns revealed that gastric mucosal cells exposed to the LPS alone showed a marked increase in COX-2 S-nitrosylation, while the countering effect of ghrelin on the LPS-induced up-regulation in IKK-β activity was manifested by an increase in the kinase Snitrosylation as well as the substantial loss in COX-2
S-nitrosylation. Moreover, the induced by ghrelin increase in IKK-β S-nitrosylation was susceptible to suppression by Akt inhibitor, SH-5, which also caused the reversal of the countering effect of ghrelin on the LPSinduced COX-2 S-nitrosylation. Thus, our findings lend further support to increasingly apparent assertion that cNOS activation through Src/Akt-mediated phosphorylation is a pivotal element in the signaling cascade by which ghrelin exerts the modulatory control over proinflammatory events triggered in gastric mucosa by H. pylori infection [14-16,24,26,41].
Together, the data provided in our study demonstrate that H. pylori LPS-induced abrogation of cNOS control over NF-κB activation leads to the induction of iNOS expression that triggers up-regulation COX-2 activation through S-nitrosylation that results in an excessive PGE2 generation (