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The Journal of Neuroscience, August 20, 2003, 23(20):7470-7478
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The Involvement of Glucose Metabolism in the Regulation of Inducible Nitric Oxide Synthase Gene Expression in Glial Cells: Possible Role of Glucose-6-Phosphate Dehydrogenase and CCAAT/Enhancing Binding Protein
Je-Seong Won,1,2 Yeong-Bin Im,1 Lyndon Key,1 Inderjit Singh,1 andAvtar K. Singh2,3 Departments of 1Pediatrics and 2Pathology, Medical University of South Carolina, Charleston, South Carolina 29425, and 3Laboratory Medicine Service, Ralph Johnson Veterans Affairs Medical Center, Charleston, South Carolina 29425
Abstract
Top
Abstract
Introduction
In rat glial cells the lipopolysaccharide (LPS)-induced inducible nitric oxide synthase (iNOS) gene expression was enhanced by extracellular glucose concentration in a dose-dependent manner. On the other hand, 2-deoxy-D-glucose decreased the LPS-induced iNOS gene expression even in the presence of glucose (6 gm/l), suggesting that glucose metabolism is linked to the regulation of iNOS gene expression. The intracellular NADPH/NADP+ directly correlated with the extracellular glucose concentration, and the reduction of NADPH generation via a block of glucose-6-phosphate dehydrogenase (G6PD) by treatment with dehydroepiandrosterone or the antisense DNA oligomer of G6PD mRNA resulted in the inhibition of iNOS gene expression. Gel shift assays showed that CAAT/enhancing binding protein (C/EBP), rather than AP-1 or NF-B, correlated better with a glucose-dependent increase in iNOS gene expression. The induction of C/EBP DNA binding activity by LPS and glucose was attributable mainly to the increase in C/EBP-
protein. The cotransfection with wild-type C/EBP-
Key words: C/EBP; astrocytes; glucose; G6PD; iNOS; NADPH; NF-
Introduction
Clinical studies have suggested that mortality and morbidity are increased in stroke patients with high plasma glucose levels (Candelise et al., 1985). Consistent with these observations, acute hyperglycemia is detrimental when ischemia is followed by reperfusion in focal ischemia animal models (Nedergaard, 1987
To understand how hyperglycemia or hypoglycemia affects ischemia-mediated outcomes, we hypothesized that extracellular glucose may affect brain damage by the regulation of the inducible or immunological isoform of nitric oxide (NO) synthase (iNOS) gene expression, because iNOS has been known to be involved in the mechanisms of cerebral ischemic insult (Iadecola, 1999
In contrast to neuronal and endothelial NOS, iNOS is regulated mainly at the transcriptional level (Nathan, 1992
(IFN-
In the present study we examined the influence of glucose on the induction of iNOS gene expression in glial cells and also sought to determine the transcriptional factors and signaling mechanisms involved in glucose-mediated upregulation of iNOS gene expression. We report that extracellular glucose upregulated the LPS-induced expression of iNOS in a dose-dependent manner, whereas 2-deoxy-D-glucose decreased the LPS-induced iNOS expression. This increase in iNOS expression was mediated by the transactivation of C/EBP-
Materials and Methods
Isolation and maintenance of primary rat astrocytes and C6 rat glioma cells. Astrocytes were prepared from rat cerebral tissue as described by McCarthy and de Vellis (1980Assay for NO production and induction of iNOS enzyme. C6 rat glioma cells and astrocytes were cultured in 12-well plastic tissue culture plates. After the appropriate treatment the production of NO was determined by an assay of the culture supernatant for nitrite (Green et al., 1982
Western blot analysis. The protein concentration of samples was determined with the detergent-compatible protein assay reagent (Bio-Rad Laboratories, Hercules, CA) by using bovine serum albumin (BSA) as the standard. Samples were boiled for 3 min with 0.1 volume of 10%
-mercaptoethanol and 0.5% bromophenol blue mix. Then 50 µg of total cellular protein and 10 µg of nuclear extract or membrane protein or cytoplasmic protein were resolved by electrophoresis in 8 or 12% polyacrylamide gels, electrotransferred to polyvinylidene difluoride (PVDF) filter, and blocked with PVDF buffer [I-Block (Tropix, Bedford, MA), 10 mM Trizma base, pH 7.4, 1% Tween 20, and 150 mM NaCl]. After incubation with antiserum against iNOS (1:1000; 610432, BD PharMingen, San Diego, CA), hRas (1:1000; sc-520), RhoA (1:1000; sc-179), C/EBP-
Isolation of total RNA and Northern blot assay. C6 rat glioma cells were cultured in six-well plastic tissue culture plates. After the appropriate treatment the total cellular RNA was extracted by the use of a rapid guanidine thiocyanate water-saturated phenol/chloroform extraction procedure and by subsequent precipitation with acidic sodium acetate. Total RNA (5 µg) was denatured and electrophoresed on 1% agaroseformaldehyde gels and transferred onto nylon Hybond-N hybridization membrane sheets (Amersham Biosciences). After UV cross-linking, the membranes were prehybridized at 68°C in prehybridization buffer (5x SSC, 50% formamide, 0.02% SDS, 0.1% sodium N-lauroyl sarcosine, and 2% blocking reagent). The digoxigenin (DIG)-labeled iNOS probes were added to the prehybridization buffer and incubated overnight. The iNOS probe was generated by in vitro transcription from partial rat iNOS cDNA (1-893 bp), which was generated by reverse transcriptase-PCR, using primers (5'-ATG GCT TGC CCC TGG AAG TTT CTC T-3' and 5'-AGC GGC CAT AGC GGG GCT T-3') from total RNA from C6 rat glioma cells and subsequent cloning to an EcoRV site on pBluescript II KS+ (Stratagene, La Jolla, CA). The membranes were washed three times in 2x SSC and 0.1% SDS at room temperature and in 0.1x SSC and 0.1% SDS at 68°C. After the membranes were equilibrated in maleic acid buffer (100 mM maleic acid and 150 mM NaCl, pH 7.5), the membranes were blocked in maleic acid buffer containing 1% blocking reagent (Roche Molecular Biochemicals, Indianapolis, IN). The chemiluminescent autoradiography detection was performed as suggested by the manufacturer (Roche Molecular Biochemicals), using an alkaline phosphataseconjugated anti-DIG Fab fragment (Roche Molecular Biochemicals) and CSPD [disodium 3-(4-methoxyspiro {1,2-dioxetane-3,2'-(5'-chloro) tricyclo [3.3.1.1 3,7]decan}-4-yl) phenyl phosphate (Roche Molecular Biochemicals)].
Nuclear extraction. Nuclear extracts from C6 cells and astrocytes (1 x 10 7 cells) were prepared by using a previously published method (Dignam et al., 1983
Extraction of membrane and cytoplasmic fraction. C6 rat glioma cells were cultured in 60 mm plastic tissue culture dishes. After the appropriate treatment the cells were washed with ice-cold PBS and collected by scraping. After centrifugation at 1500 x g for 3 min the cells were subjected to sonication in (in mM) 10 HEPES, pH 7.9, 10 KCl, 2 MgCl2, and 0.5 dithiothreitol plus protease inhibitor mixture (Sigma) and were centrifuged at 150,000 x g for 30 min at 4°C. The pellet (membrane fraction) or supernatant (cytosolic fraction) was dissolved in 50 µl of 1x or an equal volume of 2x SDS sample loading buffer (0.125 M Trizma base, 4% w/v SDS, 20% glycerol), respectively.
Gel shift assay (electrophoretic mobility shift assay). Nuclear proteins (10 µg) were used for the electrophoretic mobility shift assay for the detection of AP-1, NF-
0.3 pmol of AP-1 (Santa Cruz Biotechnology) or NF-
Knockdown of G6PD by using antisense DNA oligomer. For the transfection the C6 rat glioma cells were cultured on 24-well plates. At 80% of confluency the G6PD antisense DNA oligomer (5'-AAG-CCA-CCTGCT-CTG-CCA-TG-3'), which has an equivalent location to -1 to
Plasmid constructs and site-directed mutagenesis. Expression vector coding wild-type mouse C/EBP-
C/EBP-2 was constructed by a megaprimer method (Barik, 1996
Transient transfections and reporter gene assay. C6 rat glioma cells (3 x 10 5 cells/well) were cultured in six-well plates for 36 hr before transfection. Transfection was performed with 2 µg of reporter gene (pGL3/-3.2iNOS or pGL3/-3.2iNOS
Biochemical assay. NADPH and NADP+ were measured as described previously (Zhang et al. 2000). In brief, the absorbance at 340 nm of these separate fractions (A1, A2, and A3) was measured. A1 was the untreated cell extract. A2 was the cell extract treated with a glucose-6-phosphate dehydrogenase (G6PD) and glucose-6-phosphate to convert all of the NADP+ to NADPH; then the absorbance was measured. A3 was the cell extract treated with a glutathione reductase and oxidized glutathione to convert all of the NADPH to NADP+; then the absorbance was measured. Absorbance A1 - A3 was reflective of NADPH content, and absorbance A2 - A1 was reflective of NADP+ content of the extract.
For the quantification of intracellular ATP level, C6 cells were plated in 12-well plastic plates. After appropriate treatment the cells were washed with cold PBS and then treated with boiling 200 µl of 100 mM Tris, pH 7.75, and 4 mM EDTA and further boiled for 2 min. After centrifugation at 1000 x g for 60 sec the ATP levels of the supernatant were measured by an ATP bioluminescence assay kit (Roche Molecular Biochemicals) according to the manufacturer's instruction.
For the quantification of lactate dehydrogenase (LDH) release the C6 cells were plated in 12-well plastic plates. After appropriate treatment the medium was collected in a 1.5 ml microcentrifuge tube. After centrifugation at 250 x g the LDH activity was measured by using an LDH activity detection kit (Roche Molecular Biochemicals).
For the cell viability assay, 1/20 volume of MTT reagent (5 mg/ml; Sigma) was added to cell media. At 2 hr after the incubation the cells were washed with PBS and dissolved in isopropanol, including 0.1N HCl. The cell viability was measured at an optical density of 570 nm by SpectraMax 190 (Molecular Devices).
For the measurement of cellular glutathione the cells (3 x 10 6) were pelleted and resuspended in 5% metaphosphoric acid. After homogenization by Teflon pestle the lysate was centrifuged at 3000 x g for 10 min. The glutathione level in the supernatant was measured by a kit provided by Calbiochem (La Jolla, CA).
Statistical analysis. All values shown in the figures are expressed as the means ± SEM of n determinations, obtained from at least three independent experiments. The results were examined by one- and two-way ANOVA; then individual group means were compared with the Bonferroni test. A p value <0.05 was considered significant.
Results
The extracellular glucose regulates LPS-induced NO production and iNOS gene expression
Previous studies report the role of insulin (Zhu and Auer, 1994
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Figure 1. Extracellular glucose regulates the LPS-induced iNOS gene expression and NO production in C6 rat glioma cells. Effect of glucose (0, 0.3, 1, 3, and 6 gm/l) on the induction of iNOS mRNA and on protein and NO production was examined after 6 hr (for iNOS mRNA level) or 24 hr (for iNOS protein and NO levels) of LPS (2 µg/ml) treatment. The cells were pretreated for 36 hr before LPS treatment. The nitrite level was normalized with total protein quantity. The 28S rRNA was used as an internal loading standard in Northern blot analysis. The procedures for measurement of RNA and of protein and NO are described in Materials and Methods. The error bars indicate the SEM (*p < 0.05, **p < 0.01, and ***p < 0.001 as compared with 0 gm/l of the glucose-treated group).
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Figure 2. The effect of 2-deoxy-D-glucose on LPS-induced NO production and iNOS gene expression in C6 rat glioma cells. At 6 hr (for iNOS mRNA level) or 24 hr (for iNOS protein and NO levels) after LPS (2 µg/ml) stimulation the effects of indexed concentrations of 2-deoxy-D-glucose (deoxy-glucose; 0, 0.1, 0.5, 1, and 5 mM) on the levels of iNOS mRNA and of protein and nitrite were examined. The cells were pretreated with deoxy-glucose for 36 hr before LPS (2 µg/ml) treatment in the presence of 6 gm/l glucose. The nitrite level was normalized with total protein quantity. Levels of 28S rRNA were used as an internal standard in Northern blot analysis. The error bar at each time indicates the SEM (*p < 0.05, **p < 0.01, and ***p < 0.001 as compared with 0 gm/l of the glucose-treated group).
The effect of extracellular glucose concentration on cell toxicity, viability, and intracellular ATP level
To investigate the possible involvement of cell toxicity or viability evoked by glucose availability in the regulation of iNOS gene expression, we performed the LDH assay and microculture tetrazolium colorimetric (MTT) assay after 36 hr of incubation with various concentrations of glucose (Fig. 3A,B). In glucose-starved conditions the C6 cells released the highest levels of LDH to media and showed the lowest cell viability (optical density of MTT). Although the addition of glucose reduced LDH release and increased cell viability up to 3 gm/l glucose, there was no significant difference between 3 and 6 gm/l of the glucose-treated groups. Because glucose is the major source for ATP generation in brain cells, the effect of extracellular glucose concentration on intracellular ATP level was examined after 36 hr of incubation with indexed glucose concentrations (Fig. 3C). In the glucose-starved group the intracellular ATP level was lowest. The addition of glucose increased the intracellular ATP level, but there was no significant difference among 1, 3, and 6 gm/l of the glucose-treated groups. These observations indicate that the intracellular level of ATP does not correlate with the enhancement of LPS-mediated induction of iNOS; therefore, it may not be responsible for glucose-mediated upregulation of iNOS.
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Figure 3. The effect of extracellular glucose concentration on cytotoxicity/viability of C6 rat glioma cells. C6 rat glioma cells were incubated with indexed concentrations of glucose (0, 1, 3, and 6 gm/l) for 36 hr. Lactate dehydrogenase (LDH) in medium (A), cell viability (MTT assay; B), and intracellular ATP level (C) were examined as described in Materials and Methods. The LDH activity and ATP level were normalized with total protein quantity. The error bars in each panel indicate the SEM (*p < 0.05, **p < 0.01, and ***p < 0.001 as compared with 0 gm/l of the glucose-treated group).
The effect of extracellular glucose concentration on the intracellular NADPH/NADP+ ratio and the possible involvement of G6PD in glucose-dependent enhancement of LPS-induced iNOS gene expression
Another metabolic pathway of glucose is the pentose phosphate pathway (PPP). The importance of PPP lies in the production of ribose and NADPH. To investigate the possible role of PPP on the induction of iNOS, we examined the effect of dehydroepiandrosterone (DHEA), an inhibitor of G6PD (rate-limiting enzyme in PPP), on glucose-mediated change in the ratio of NADPH/NADP+ and induction of iNOS. As shown in Figure 4A, the extracellular glucose increased the intracellular NADPH/NADP+ ratio in a dose-dependent manner. In addition, the high glucose-induced (6 gm/l) increase of NADPH/NADP+ ratio was reduced significantly by pretreatment of the cells with DHEA. The pretreatment with DHEA also decreased the LPS-induced NO production and iNOS gene expression in a dose-dependent manner in the presence of 6 gm/l glucose (Fig. 4). To confirm the role of G6PD in iNOS gene regulation, we incubated the cells with antisense DNA oligomer against rat G6PD mRNA and sequence-scrambled DNA oligomer as a control before treatment with LPS. As shown Figure 4C, antisense DNA oligomer reduced significantly the LPS-mediated increases in NO production and iNOS protein level as well as G6PD protein levels. This result further supported the involvement of G6PD in iNOS gene regulation.
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Figure 4. The effect of extracellular glucose concentration on the intracellular NADPH/NADP+ ratio and the possible role of G6PD in glucose-mediated upregulation of LPS-induced iNOS gene expression in C6 rat glioma cells. The C6 cells were treated with various glucose concentrations (0, 1, 3, and 6 gm/l) for 36 hr or DHEA (100 µM) plus 6 gm/l glucose for 0.5 hr before treatment with LPS (2 µg/ml) and then were harvested for measurement of NADPH and NADP+ levels as described in Materials and Methods (A). Each concentration of NADPH and NADP+ was normalized with total protein quantity. The effect of indexed concentrations of DHEA (0, 10, 50, and 100 µM) on nitrite production and on iNOS protein and its mRNA levels was examined in the presence or absence of LPS (B). The iNOS mRNA levels were measured after 6 hr of LPS treatment. Nitrite and iNOS protein were measured after 24 hr of LPS treatment. Cyclophilin (CPN) was used as an internal standard in Northern blot analysis. For the knockdown of G6PD the cells were transfected with glucose 6-phosphate dehydrogenase (G6PD) antisense DNA oligomer or its sequence-scrambled DNA oligomer as described in Materials and Methods (C). At 2 d after transfection the cells were stimulated with LPS, and NO production and the protein levels of iNOS and G6PD were measured. The error bars in each panel indicate the SEM (*p < 0.05, **p < 0.01, and ***p < 0.001 as compared with 0 gm/l of the glucose-treated group).
The major known function of PPP is the generation of ribose and reduced glutathione. As shown in Figure 5A, the pretreatment with ribose (5 mM) or glutathione monoethylester (GSHME; 500 µM), a cell-permeable analog of glutathione, had no effect on DHEA-evoked inhibition of iNOS gene expression and production of NO by LPS. To examine the effect of DHEA and GSHME on cellular glutathione level, we measured the intracellular glutathione level 4 hr after DHEA treatment. As shown in Figure 5B, the cellular glutathione level was reduced by the treatment with DHEA, whereas it increased by GSHME. These observations further support that ribose or glutathione was not involved in glucose-mediated induction of iNOS.
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Figure 5. The effect of glutathione monoethylester and ribose on DHEA-mediated inhibition of iNOS gene expression in C6 rat glioma cells. After incubation of cells with glutathione monoethylester (GSHME; 500 µM) or ribose (5 mM) for 0.5 hr, the cells were treated with vehicle (VHC; dimethylsulfoxide) or dehydroepiandrosterone (DHEA; 100 M) for 0.5 hr and then with LPS (2 µg/ml; A). The iNOS mRNA level and its protein and nitrite levels were measured after LPS treatment for 6 or 24 hr, respectively. Cyclophilin (CPN) was used as an internal loading standard in Northern blot analysis. To examine the cellular glutathione (GSH) level, we pretreated the cells with GSHME (500 µM) 0.5 hr before DHEA treatment (B). At 4 hr after DHEA treatment the cellular GSH levels were measured as described in Materials and Methods. The error bars in A and B indicate the SEM.
Activation of small GTPase is not involved in extracellular glucose-mediated regulation of iNOS gene expression
Because the reduction of acetyl-CoA and NADPH can evoke a subsequent reduction of protein isoprenylation by attenuation of intracellular levels of mevalonic acid, the effect of extracellular glucose concentration on membrane association of small GTPase was examined. As shown in Figure 6, A and B, various concentrations of glucose had no effect on the translocation of hRas and RhoA proteins to the membrane. Moreover, pretreatment with various concentrations of farnesyl pyrophosphate (FPP; 1, 5, and 10 µM) or geranylgeranyl pyrophosphate (GGPP; 1, 5, and 10 µM), ligands required for the translocation of small GTPase to plasma membrane, did not reverse the glucose starvation-evoked inhibition of LPS-induced NO production. To confirm the uninvolvement of farnesylation or geranyl-geranylation of hRas or RhoA protein in glucose-dependent NO production, we also examined the effect of lovastatin, an inhibitor of 3-hydroxy-3-methylglutaryl coenzyme A reductase that in turn blocks the de novo synthesis of farnesyl pyrophosphate and geranylgeranyl pyrophosphate, on LPS-induced NO production. Rather than inhibition, the pretreatment with lovastatin resulted in the enhancement of LPS-mediated NO production in the presence of 6 gm/l glucose (Fig. 6C). These observations indicate that the state of farnesylation or geranyl-geranylation of small GTPase is not responsible for glucose-mediated LPS-induced expression of iNOS and NO production.
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Figure 6. The uninvolvement of small GTPase in glucose-mediated regulation of NO production in C6 rat glioma cells. The effect of glucose on the distribution of protein levels of hRas (A) or RhoA (B) between plasma membrane or cytoplasmic fraction was examined (top panels). After treatment with indexed concentrations of glucose (0, 0.3, 1, 3, and 6 gm/l) for 36 hr the cells were fractionated into membrane or cytoplasmic proteins and analyzed by Western blot analysis. The bottom panels of A and B show the effect of farnesyl pyrophosphate (FPP; 0, 1, 5, and 10 µM) or geranylgeranyl pyrophosphate (GGPP; 0, 1, 5, and 10 µM) on the glucose-mediated production of nitrite in the presence or absence of LPS (2 µg/ml). C, The effect of various concentrations of lovastatin (0, 0.3, 1, and 3 µM) on LPS-induced nitrite production was examined in the presence of 6 gm/l glucose supplement. The nitrite levels were determined 24 hr after LPS treatment. The error bars in each panel indicate the SEM.
The effect of extracellular glucose concentration and DHEA on the NF-
To understand the mechanism of glucose-mediated induction of iNOS, we examined the effects of glucose and DHEA on LPS-induced DNA binding activity of AP-1, NF-,
forms) had no effect on LPS-induced C/EBP DNA binding activity. As shown in Figure 7E, C/EBP-
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Figure 7. The effect of extracellular glucose concentration and DHEA on the activation of NF-
The involvement of C/EBP response element in iNOS promoter and C/EBP-
To elucidate the involvement of C/EBP response element in iNOS gene expression, we examined the activity of wild-type -3.2 kb iNOS gene promoter/enhancer (pGL3/-3.2iNOS) and its mutant form (pGL3/-3.2iNOS
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Figure 8. The involvement of C/EBP response element in iNOS promoter and C/EBP-
Extracellular glucose regulates LPS-induced expression of iNOS and C/EBP-
To compare the role of glucose in iNOS gene expression in C6 rat glioma cells and primary cultured astrocytes, we pretreated the astrocytes with several concentrations of glucose (0, 1, 3, and 6 gm/l) for 36 hr before treatment with LPS. NO production, iNOS protein level, and C/EBP-
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Figure 9. Extracellular glucose regulates the LPS-induced iNOS gene expression and NO production in primary cultured rat astrocytes. The effects of glucose (0, 1, 3, and 6 gm/l) on the induction of NO production and iNOS protein level (A) and the protein levels of C/EBP-
Discussion
Recent studies have suggested that insulin has a protective role in global and focal ischemia (Voll and Auer, 1988Contrary to C6 rat glioma cells, hyperglycemic (6 gm/l) conditions did not enhance the LPS-mediated responses in primary astrocytes. Although the difference between astrocytes and C6 rat glioma cells in conditions of minimal requirement of glucose for the full activation of iNOS gene expression is not understood fully, the demand for higher level of exogenous glucose in highly dividing C6 rat glioma cells as compared with primary cultured astrocytes may contribute toward the observed difference in iNOS gene expression. Previously, Ste-Marie et al. (2001
Because glucose is one of the main energy sources for brain cells, its availability can affect cell viability and various signaling pathways, including the LPS-mediated signaling cascade. To know the cellular condition before LPS treatment, we examined the effect of glucose on cellular ATP level and LDH release or cell viability after 36 hr of glucose treatment. In contrast to the dose-dependent induction of iNOS gene expression by glucose, no differences were observed in ATP production or cell viability between 3 and 6 gm/l glucose, suggesting that the cellular level of ATP and related cell toxicity/viability influenced by extracellular glucose availability may not be the mediators in the observed glucose-dependent regulation of iNOS gene expression. However, we observed that the intracellular NADPH/NADP+ ratio paralleled the extracellular glucose concentration and induction of expression of iNOS. Furthermore, decreased intracellular NADPH/NADP+ after the treatment with DHEA, a known inhibitor of G6PD (a rate-limiting enzyme of the PPP) (Schwartz and Pashko, 1993
DHEA and its synthetic analogs are known to function as antiproliferative agents in animal tumor models and malignant cell lines via inhibition of G6PD in PPP. The production of ribose moiety and NADPH by PPP is important for the generation of ribonucleosides or deoxyribonucleosides (Schwartz et al., 1988
Several transcriptional factors, such as NF-
In summary, we report that extracellular glucose plays a role in the LPS-induced iNOS gene expression and NO production. This regulation may be attributable to the involvement of G6PD-dependent PPP and may indicate that the signal or signals for upregulation of expression of iNOS by extracellular glucose are mediated via the C/EBP-
Footnotes
Received Aug. 12, 2002; revised May. 27, 2003; accepted Jun. 5, 2003.These studies were supported by National Institutes of Health Grants NS-22576, NS-34741, NS-37766, and NS-40810.WearethankfultoDr.ShailendraGiriforcooperationinthisstudy,Dr.ErnestBarbosaandDr.AnneG.Gilg for proofreading this manuscript, and Joyce Bryan and Hope Terry for laboratory and secretarial assistance, respectively.
Correspondence should be addressed to Dr. Avtar K. Singh, Department of Pediatrics, Medical University of South Carolina, Clinical Science Building, Room 316, 171 Ashley Avenue, Charleston, SC 29425. E-mail: singhi{at}musc.edu.
Copyright © 2003 Society for Neuroscience 0270-6474/03/237470-09$15.00/0
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