Endogenous nitric oxide inhibits the synthesis of cyclooxygenase products and interleukin-6 by rat Kupffer cells

Stadler, J.; Silvio, Mauricio Di; Curran, Ronald; Jordan, Mark L.; Simmons, Richard L.; Billiar, Timothy R.

doi:10.1002/jlb.53.2.165

Cited by 239 publications

(111 citation statements)

References 34 publications

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“…Salvemini et al (34) have shown that injection of iNOS inhibitors into a rodent air pouch model (carrageenan-induced) blocked both iNOS and COX-2 activity in areas of inflammation. Our studies, in contrast, are similar to the studies by Stadler et al (35) and Swierkosz et al (36) that indicate that endogenous NO inhibits the synthesis of COX products as observed in rodent Kupffer cells and macrophages, respectively. This controversy may be due to the tissue-specific expression of NOS/COX-2 in various cell types, the difference in the pathophysiology of normal and OA-affected chondrocytes, and the influence of various other mediators in the microenvironment of the cartilage that may influence the production of NO and PGE 2 .…”

Section: Discussionsupporting

confidence: 93%

Superinduction of cyclooxygenase-2 activity in human osteoarthritis-affected cartilage. Influence of nitric oxide.

Amin¹,

Attur²,

Patel³

et al. 1997

J. Clin. Invest.

355

285

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Cartilage specimens from osteoarthritis (OA)-affected patients spontaneously released PGE 2 at 48 h in ex vivo culture at levels at least 50-fold higher than in normal cartilage and 18-fold higher than in normal cartilage ϩ cytokines ϩ endotoxin. The superinduction of PGE 2 production coincides with the upregulation of cyclooxygenase-2 (COX-2) in OA-affected cartilage. Production of both nitric oxide (NO) and PGE 2 by OA cartilage explants is regulated at the level of transcription and translation. Dexamethasone inhibited only the spontaneously released PGE 2 production, and not NO, in OA-affected cartilage. The NO synthase inhibitor H N G -monomethyl-L -arginine monoacetate inhibited OA cartilage NO production by Ͼ 90%, but augmented significantly (twofold) the spontaneous production of PGE 2 in the same explants. Similarly, addition of exogenous NO donors to OA cartilage significantly inhibited PGE 2 production. Cytokine ϩ endotoxin stimulation of OA explants increased PGE 2 production above the spontaneous release. Addition of L -NMMA further augmented cytokine-induced PGE 2 production by at least fourfold. Inhibition of PGE 2 by COX-2 inhibitors (dexamethasone or indomethacin) or addition of exogenous PGE 2 did not significantly affect the spontaneous NO production. These data indicate that human OA-affected cartilage in ex vivo conditions shows ( a ) superinduction of PGE 2 due to upregulation of COX-2, and ( b ) spontaneous release of NO that acts as an autacoid to attenuate the production of the COX-2 products such as PGE 2 . These studies, together with others, also suggest that PGE 2 may be differentially regulated in normal and OA-affected chondrocytes. ( J. Clin. Invest. 1997. 99:1231-1237.)

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Section: Discussionsupporting

confidence: 93%

Superinduction of cyclooxygenase-2 activity in human osteoarthritis-affected cartilage. Influence of nitric oxide.

Amin¹,

Attur²,

Patel³

et al. 1997

J. Clin. Invest.

355

285

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“…27 The co-induction of COX-2 and iNOS has also been observed in studies in vitro of rat vascular smooth muscle cells, 28,29 glomerular mesangial cells, 7 murine macrophages, 30 rat islets of Langerhans, 31 human endothelial cells, 32 articular chondrocytes, 33 and rabbit hepatocytes 34 incubated with endotoxin and/or cytokines but not in similar studies of human fetal cell fibroblasts 6 or bovine aortic endothelial cells. 35 Proinflammatory cytokines known to be synthesized and released by T lymphocytes and macrophages during cardiac allograft rejection are probably responsible for induction of COX-2 in this situation.…”

Section: Discussionmentioning

confidence: 86%

“…In cultured bovine endothelial cells, NO or NO donor drugs have been shown to inhibit PGI 2 release by bradykinin (COX-1) 39 and to inhibit COX-2 induction and activity in rat Kupffer cells. 34 In contrast, however, NO and NO donor drugs have been shown to stimulate COX-1 and COX-2 activity in endotoxin-activated murine macrophages 6 and in vascular smooth muscle cells 28 and human endothelial cells. 39,40 Similarly, in the hydronephrotic model of renal inflammation, 22 in air-pouchinduced inflammation, 24 there is evidence that NO augments the activity of COX-1 and COX-2, leading to enhanced synthesis of prostaglandins.…”

Section: Discussionmentioning

confidence: 99%

Upregulation of COX-2 During Cardiac Allograft Rejection

Yang

Szabolcs

et al. 2000

Circulation

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Background-The hypothesis that cyclooxygenase-2 (COX-2) is involved in the myocardial inflammatory response during cardiac allograft rejection was investigated using a rat heterotopic abdominal cardiac transplantation model. Methods and Results-COX-2 mRNA and protein in the myocardium of rejecting cardiac allografts were significantly elevated 3 to 5 days after transplantation compared with syngeneic controls (nϭ3, PϽ0.05). COX-2 upregulation paralleled in time and extent the upregulation of iNOS mRNA, protein, and enzyme activity in this model. COX-2 immunostaining was prominent in macrophages infiltrating the rejecting allografts and in damaged cardiac myocytes. Prostaglandin (PG) levels in rejecting allografts were also higher than in native hearts. Because NO has been reported to modulate PG synthesis by COX-2, additional transplants were performed using animals treated with a selective COX-2 inhibitor (SC-58125) and a selective inhibitor of the inducible nitric oxide synthase (iNOS) N-aminomethyl-L-lysine. At posttransplant day 5, inhibitor administration resulted in a significant reduction of COX-2 mRNA expression (3764Ϯ337 versus 5110Ϯ141 arbitrary units, nϭ3, PϽ0.05) and iNOS enzymatic activity (1.7Ϯ0.4 versus 22.8Ϯ14.4 nmol/mg protein, nϭ3, PϽ0.01) compared with vehicle-treated allogeneic transplants. Allograft survival in treated animals was increased modestly from 5.4 to 6.4 days (PϽ0.05). However, apoptosis of cardiac myocytes (TUNNEL method) was only marginally reduced relative to vehicle controls in treated graft recipients. The intensity of allograft rejection was also similar in the treated and untreated allografts. Conclusions-The data indicates that COX-2 expression is enhanced in parallel with iNOS in the myocardium during cardiac allograft rejection. (Circulation. 2000;101:430-438.)

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“…Several studies have indicated that in murine and human models these upper level fluxes of NO can be achieved in tissue. Inhibition of P450 and COX-2 have provided evidence that locally, high levels of NO can be achieved by inflamed liver cells [90][91][92] . Nitric oxide mediated inhibition of P450 may have important consequence under inflammatory conditions 93, 94 .…”

Section: The Concentration Range Of Endogenously Generated Nitric Oxidementioning

confidence: 99%

The chemical biology of nitric oxide: Implications in cellular signaling

Thomas¹,

Ridnour²,

Isenberg³

et al. 2008

Free Radical Biology and Medicine

826

710

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Nitric oxide (NO) has earned the reputation of being a signaling mediator with many diverse and often opposing biological activities. The diversity in response to this simple diatomic molecule comes from the enormous variety of chemical reactions and biological properties associated with it. In the last few years, the importance of steady state NO concentrations have emerged as a key determinant of its biological function. Precise cellular responses are differentially regulated by specific NO concentration. We propose 5 basic distinct concentration levels of NO activity; cGMP mediated processes ([NO] <1-30 nM; Akt phosphorylation ([NO] = 30-100 nM); stabilization of HIF-1α ([NO] = 100-300 nM); phosphorylation of p53 ([NO] > 400 nM) and nitrosative stress (1 µM). In general, lower NO concentrations promote cell survival and proliferation, while higher levels favor cell cycle arrest, apoptosis, and senescence. Free radical interactions will also influence NO signaling. One of the consequences of reactive oxygen species (ROS) generation is to reduce NO concentrations. This antagonizes the signaling of nitric oxide and in some cases results in converting a cell cycle arrest profile to a cell survival one. The resulting reactive nitrogen species (RNS) that are generated from these reactions can also have biological effects and increase oxidative and nitrosative stress responses. A number of factors determine the formation of NO and its concentration, such as diffusion, consumption, and substrate availability which are referred to as Kinetic Determinants for Molecular Target Interactions. These are the chemical and biochemical parameters that shape cellular responses to NO. Herein we discuss signal transduction and the chemical biology of NO in terms of the direct and indirect reactions.

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Endogenous nitric oxide inhibits the synthesis of cyclooxygenase products and interleukin-6 by rat Kupffer cells

Cited by 239 publications

References 34 publications

Superinduction of cyclooxygenase-2 activity in human osteoarthritis-affected cartilage. Influence of nitric oxide.

Superinduction of cyclooxygenase-2 activity in human osteoarthritis-affected cartilage. Influence of nitric oxide.

Upregulation of COX-2 During Cardiac Allograft Rejection

The chemical biology of nitric oxide: Implications in cellular signaling

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