Helicobacter pylori Induces I{kappa}B Kinase {alpha} Nuclear Translocation and Chemokine Production in Gastric Epithelial Cells

NF- ${kappa}$ B is an important transcriptional factor that is involvedin multiple cellular responses, such as inflammation and antiapoptosis.I ${kappa}$ B kinase ${alpha}$ (IKK ${alpha}$ ) and IKKß, which are critical regulatorsof NF- ${kappa}$ B activity, possess various mechanisms for NF- ${kappa}$ B activation.This variability in NF- ${kappa}$ B signaling may be associated with distinctinflammatory responses in specific cell types. The gastric pathogenHelicobacter pylori is known to activate NF- ${kappa}$ B. However, therole of IKK in H. pylori infection remains unclear. In thisreport, we show that H. pylori activates both IKK ${alpha}$ and IKKßin gastric cancer cells and enhances NF- ${kappa}$ B signaling in distinctmanners. We found that IKKß acted as an I ${kappa}$ B ${alpha}$ kinaseduring H. pylori infection, whereas IKK ${alpha}$ did not. H. pylori inducedIKK ${alpha}$ nuclear translocation in time-, multiplicity of infection-,and cag pathogenicity island-dependent manners. In contrast,p100 processing, which is a known IKK ${alpha}$ activity induced by severalcytokines, was not induced by H. pylori. Both IKKs were responsiblefor chemokine secretion by infected cells. However, the antiapoptoticeffect of H. pylori was merely transduced by IKKß.Microarray analysis and real-time PCR indicated that both IKKswere involved in the transcriptional activation of genes associatedwith inflammation, antiapoptosis, and signal transduction. Ourresults indicate that H. pylori activates NF- ${kappa}$ B via both IKK ${alpha}$ and IKKß using distinct mechanisms. IKK ${alpha}$ nuclear translocationinduced by H. pylori is indispensable for appropriate inflammatoryresponses but not for antiapoptosis, which suggests a criticalrole for IKK ${alpha}$ in gastritis development.

INTRODUCTION

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Introduction

Helicobacter pylori is a pathogen that causes human gastricdisease. About half of the world population is infected withthis bacterium, although only a relatively small proportionof infected patients develop symptomatic disease, such as gastroduodenalulcer, gastric cancer, and mucosa-associated lymphoid tissuelymphoma. Bacterial, environmental, and host genetic factorsmay affect the progress and outcome of gastric disease. Onesuch factor that is responsible for severe disease is the bacterialvirulence factor cag pathogenicity island (PAI) (reviewed inreferences 6, 32, and 36). H. pylori strains that carry cagPAI genes, called type I strains, are highly prevalent in patientswith gastroduodenal ulcer and gastric cancer (2, 4, 8). Previousstudies have revealed that type I H. pylori strains are capableof activating multiple intracellular signaling pathways in infectedepithelial cells (22, 26). The inflammatory, proliferative,and antiapoptotic responses observed in H. pylori-infected cellsin culture and in gastric tissues are possibly mediated by theactivation of intracellular signaling pathways, such as thosefor NF- ${kappa}$ B and mitogen-activated protein kinase.

NF- ${kappa}$ B is an important transcriptional factor that controls variousbiological processes, such as inflammation, cell survival ordeath, and cell cycle (reviewed in references 5, 14, 18, 20,and 23). The mechanism of NF- ${kappa}$ B activation by a variety of extracellularstimuli is unique in that it is induced rapidly and does notrequire de novo protein synthesis, thereby allowing the cellsto respond quickly to emergent situations, such as bacterialinfection (49). Most forms of NF- ${kappa}$ B, especially the most commonform of the p50-RelA dimer, are rendered inactive through bindingof the inhibitory protein I ${kappa}$ Bs. Phosphorylation-induced ubiquitinationof I ${kappa}$ Bs promotes its degradation, which in turn liberates NF- ${kappa}$ Bdimers as their active forms (reviewed in references 5, 14,18, and 23). The I ${kappa}$ B kinase (IKK) complex is a protein complexthat phosphorylates I ${kappa}$ Bs in response to upstream stimuli, andit is considered to be a critical regulator of NF- ${kappa}$ B activity(14, 20, 49).

The IKK complex contains three subunits: the catalytic subunitsIKK ${alpha}$ and IKKß and the regulatory subunit IKK ${gamma}$ (10, 30,37, 38, 45, 50). When overexpressed exogenously or synthesizedin an in vitro system, both IKK ${alpha}$ and IKKß phosphorylateI ${kappa}$ B proteins and activate NF- ${kappa}$ B (10, 30, 37, 45, 50). Earlierstudies on IKKß knockout cells have indicated thatIKKß is indispensable for I ${kappa}$ B phosphorylation, NF- ${kappa}$ Bactivation, and subsequent gene expression in response to proinflammatorystimuli (24, 25). In contrast, IKK ${alpha}$ knockout cells show normalI ${kappa}$ B ${alpha}$ phosphorylation and RelA nuclear translocation in responseto lipopolysaccharide or cytokines (16, 43). These results haveraised the question of whether IKK ${alpha}$ is involved physiologicallyin NF- ${kappa}$ B activation. Interestingly, IKK ${alpha}$ -deficient mice show morphologicalabnormalities, indicating the specific role of IKK ${alpha}$ that cannotbe compensated for by IKKß (16, 43). One of the specificactivities of IKK ${alpha}$ is the induction of p100 processing to p52.The phosphorylation of p100 by IKK ${alpha}$ results in p100 degradationand the generation of p52, which in turn dimerizes with RelBto form the NF- ${kappa}$ B subunit (9, 39). This pathway, which is calledthe alternative pathway, is considered to play an essentialrole in secondary lymphoid organ development and adaptive immunity(9, 39). Another specific function of IKK ${alpha}$ is to control geneexpression by direct translocation into the nucleus, which appearsto be important in epidermal differentiation and craniofacialmorphogenesis (1, 41, 46). These functional diversities of IKK ${alpha}$ and IKKß, as well as the variations in extra- andintracellular signaling that lead to the activation of eachIKK, may provide information on the numerous biological rolesof these molecules with respect to NF- ${kappa}$ B.

As NF- ${kappa}$ B is especially important for the immune system, the constitutiveactivation of NF- ${kappa}$ B is associated with inflammatory diseases(20, 23). Furthermore, aberrant NF- ${kappa}$ B activation leads to tumorigenesisvia antiapoptotic gene expression (19, 20). Thus, the detailedanalysis of this signaling in disease states will be usefulfor therapy development. Although H. pylori persistently infectsthe human stomach and activates NF- ${kappa}$ B in gastric tissues, theway in which it activates NF- ${kappa}$ B is not well understood. Furthermore,the subunit of IKK complex that is involved in H. pylori-inducedNF- ${kappa}$ B activation and the effects of these molecules on gastricdisease remain to be resolved. To achieve a better understandingof NF- ${kappa}$ B signaling in H. pylori-related gastric disease, we examinedthe role of IKK in H. pylori-infected gastric cancer cells.

MATERIALS AND METHODS

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Materials and Methods

Cell line and H. pylori strains. Cells of the AGS human gastric cancer cell line (ATCC CRL-1739)were maintained at 37°C in 5% CO₂ in Ham's F12 medium thatwas supplemented with 10% fetal bovine serum. TN2, a type IH. pylori isolate, and its isogenic mutants, TN2- ${Delta}$ cagA, TN2- ${Delta}$ cagE,TN2- ${Delta}$ PAI, and TN2- ${Delta}$ vacA, were maintained under microaerophilicconditions in Brucella broth that was supplemented with 5% horseserum (15, 26). The bacterial strains were centrifuged at 3,500x g for 5 min at 4°C and washed with phosphate-bufferedsaline (PBS), and the concentrations were estimated, using anoptical density at 560 nm (OD₅₆₀) of 0.1, as 4 x 10⁷ CFU/mlH. pylori.

The AGS cells were washed once with PBS, incubated in freshmedium, and then infected with H. pylori at a multiplicity ofinfection (MOI) of 100, except in indicated instances.

Plasmids and small interfering RNA (siRNA). Dominant-negative IKK ${alpha}$ , IKKß, and its empty vectorpRK5 were kindly donated by D. Goeddel (26). The reporter plasmids,pNF- ${kappa}$ B-Luc and pRL-TK, have also been described previously (26).RNA oligonucleotides for silencing IKK ${alpha}$ (5'-GCAGGCUCUUUCAGGGACA-3'),IKKß (5'-GGUGAAGAGGUGGUGGUGAGC-3'), TAK1 (5'-UGGCUUAUCUUACACUGGA-3')(42), and the nonsilencing control (5'-UUCUCCGAACGUGUCACGU-3')with two thymidine residues (dTdT) at the 3' end were synthesizedtogether with their corresponding antisense RNAs and were annealed(QIAGEN, Hilden, Germany).

Antibodies and reagents. Human lymphotoxin (LT) ${alpha}$ 1/ß2 and human tumor necrosisfactor alpha (TNF- ${alpha}$ ) were purchased from R&D Systems (Minneapolis,MN). As a positive control, 50 ng/ml LT ${alpha}$ 1/ß2 or 10ng/ml TNF- ${alpha}$ was added to the culture medium. Polyclonal anti-phospho-I ${kappa}$ B- ${alpha}$ (Ser32), anti-phospho-JNK (Thr183/Tyr185), and phospho-NF ${kappa}$ B2p100 (Ser864) antibodies were purchased from Cell SignalingTechnology (Beverly, MA). The polyclonal anti-IKK ${alpha}$ , anti-IKKß,anti-p50, and anti-TF-IID antibodies were from Santa Cruz Biotechnology(Santa Cruz, CA), and the monoclonal anti-IKK ${alpha}$ and polyclonalanti-p100/p52 antibodies were from Upstate Biotechnology (LakePlacid, NY). The monoclonal anti-TRAF2 antibody was purchasedfrom BD Biosciences (San Jose, CA), the polyclonal anti-TAK1antibody was from StressGen Biotechnologies Corp. (Victoria,Canada), and the monoclonal anti-actin antibody was from Sigma(St. Louis, MO).

Transfection and reporter assays. In the RNA interference experiments, AGS cells were seeded intissue culture plates 24 h before transfection and grown to30 to 50% confluence. The siRNA oligonucleotides were introducedat a concentration of 100 nM into the cells using Lipofectamine(Invitrogen Corp., Carlsbad, CA) according to the manufacturer'sinstructions. Forty-eight hours after siRNA transfection, thecells were washed and infected with H. pylori for the indicatedtime.

In the reporter analysis, AGS cells were seeded in 12-well tissueculture plates and transfected with 50 ng pNF- ${kappa}$ B-Luc, 10 ng pRL-TK,and 400 ng pRK or the dominant-negative IKK vector for 24 h.Where indicated, siRNA oligonucleotides were transfected asdescribed above 24 h before transfection of the reporter plasmids.The cells were supplemented with fresh culture medium and infectedwith H. pylori for 8 h. Luciferase activity was measured andcalculated from cell lysates as described previously, and theresults are represented as fold induction compared to the controlin three independent experiments.

Immunoblot analysis. For the preparation of total cell lysates, AGS cells that weretreated with the indicated siRNAs and infected with H. pylorifor different time periods were washed once with cold PBS andlysed in ice-cold Triton X-100 buffer (50 mM Tris/HCl [pH 7.6],1% Triton X-100, 5 mM EDTA, 1 mM Na₃VO₄, 10 mM NaF, 10 µg/mlleupeptin, 10 µg/ml aprotinin, 1 mM phenylmethylsulfonylfluoride). The cell lysates were centrifuged at 10,000 x g for10 min at 4°C, and the supernatants were stored as totalcell lysates. For the preparation of nuclear and cytosolic extracts,AGS cells were seeded in a 6-cm dish, transfected with the indicatedsiRNAs, and infected with H. pylori. The cells were washed withTris-buffered saline (TBS), suspended in 200 µl of BufferA (10 mM HEPES [pH 7.9], 10 mM KCl, 0.1 mM EDTA, 0.1 mM EGTA,0.75% Nonidet P-40, 1 mM dithiothreitol, protease inhibitorcocktail [Roche Molecular Biochemicals]), incubated on ice for3 min, and centrifuged at 1,500 x g for 4 min at 4°C. Thesupernatant was removed and used as the cytosolic extract. Thepellet was washed once with Buffer A without Nonidet P-40 andcentrifuged as described above, followed by resuspension in50 µl Buffer C (20 mM HEPES [pH 7.9], 400 mM NaCl, 1 mMEDTA, 1 mM EGTA, 10 mM dithiothreitol, protease inhibitor cocktail)and incubation on ice for 10 min with frequent mixing. Finally,the suspension was centrifuged at 14,000 x g for 10 min at 4°Cand the supernatant was used as the nuclear extract. Equal amountsof cell lysates and extracts were separated by sodium dodecylsulfate-polyacrylamide gel electrophoresis and transferred toa polyvinylidene difluoride membrane. The membrane was probedwith the indicated primary antibody followed by the horseradishperoxidase-conjugated secondary antibody and developed usingthe ECL plus kit (Amersham, Buckinghamshire, United Kingdom).The protein levels of phospho-I ${kappa}$ B- ${alpha}$ , phospho-JNK, IKK ${alpha}$ , and p100/52were determined by densitometry using KODAK 1D Image Analyzersoftware and normalized with the level of actin, TF-IID, orTRAF2.

Immunofluorescence. AGS cells were seeded in Lab-Tek chamber slides (Nalge NuncInternational, Naperville, IL) and infected with H. pylori forthe indicated time. The cells were washed twice with PBS, fixedin 2% paraformaldehyde for 30 min, washed with PBS, and permeabilizedwith 0.2% Triton X-100 for 1 h. After blocking with 10% normalgoat serum, the cells were incubated overnight at 4°C withthe polyclonal anti-IKK ${alpha}$ antibody diluted in PBS. The cells werethen washed three times with PBS and incubated with Alexa Fluor488 (Molecular Probes, Eugene, OR) for 1 h. The nuclei werevisualized by staining with propidium iodide. Images were obtainedusing the LSM510 confocal laser scanning microscope (Carl Zeiss,Oberkohen, Germany).

TUNEL assay. To investigate the effect of H. pylori infection on cell apoptosis,we used the TdT-mediated dUTP-biotin nick end-labeling (TUNEL)assay. AGS cells, which were treated with control or IKK siRNAsin Lab-Tek chamber slides, were maintained in serum-free mediumfor 24 h and infected with H. pylori at an MOI of 100 for afurther 8 h. The cells were washed three times with PBS, andapoptotic cells were stained with Apoptag (Serologicals Inc.,Norcross, GA) in accordance with the manufacturer's instructions.Apoptotic cells were visualized by fluorescein isothiocyanate,and the nuclei were stained with propidium iodide, followedby microscopic examination with the LSM510 confocal laser scanningmicroscope. The number of apoptotic cells, in a total of 1,500to 2,000 cells in each well, was counted in three independentexperiments, and the percentage of apoptotic cells was calculated.

Quantification of chemokines by ELISA. The interleukin-8 (IL-8) and GRO ${alpha}$ concentrations in the culturesupernatants were measured by enzyme-linked immunosorbent assay(ELISA) as specified by the manufacturer (Techne, Minneapolis,MN). AGS cells were plated in 24-well plates, transfected withsiRNAs for 48 h, and infected with H. pylori for a further 8h. The culture supernatants were then aspirated and stored at–70°C until they were subjected to the ELISA. Theconcentrations of IL-8 and GRO ${alpha}$ were determined using standardcurves obtained with the respective recombinant proteins. Thevalues are represented as the averages ± standard deviations(SD) of three independent experiments.

Microarray procedures. For RNA preparation, AGS cells were transfected with controlor IKK-specific siRNAs for 48 h. The cultures were supplementedwith fresh medium and subsequently infected with H. pylori for3 h. The RNA was extracted using Isogen (Wako, Osaka, Japan),the samples were treated with DNase for 1 h, and then the sampleswere purified using an RNA purification kit (QIAGEN). The cDNAmicroarray analysis was performed according to the manufacturer'sinstructions using the Human Chip Oligo DNA Microarray (DNAChip Consortium, Hokkaido, Japan), which contains approximately29,000 open reading frame oligo probes. Briefly, 5 µgof total RNA was amplified using the Amino Allyl MessageAmpaRNA kit (Ambion, Austin, TX). Antisense RNA (5 µg) fromcontrol or experimental samples, e.g., unstimulated versus infectedor control siRNA-transfected versus IKK siRNA-transfected, werelabeled with Cy5 or Cy3, respectively. The two fluorescentlylabeled probes were mixed and applied to a microarray, followedby incubation under humidified conditions at 60°C overnight.Fluorescent images of the hybridized microarrays were scannedwith a fluorescence laser confocal slide scanner (Affymetrix428 Array Scanner; Santa Clara, CA). The images were analyzedusing the ImaGene 4.2 software (Bio-Discovery, Marina Del Rey,CA) according to the manufacturer's instructions. To controlfor labeling differences and to reduce hybridization errors,all of the reactions were carried out in duplicate, wherebythe fluorescent dyes were switched.

Quantitative real-time PCR. RNA was prepared as described above from AGS cells that wereinfected with H. pylori for the indicated time. For quantitativePCR, cDNA was prepared using a combination of oligo(dT), randomprimers, and the Impron II Reverse Transcription System (Promega).Each PCR was carried out in triplicate in a 25-µl volumethat contained the SYBR Green Master mix (Applied Biosystems,Foster City, CA) and using the ABI Prism 7000 Sequence DetectionSystem (Applied Biosystems). The following PCR conditions wereused: 15 min at 95°C for the initial denaturation, followedby 45 cycles of 95°C for 30 s and 60°C for 30 s. Relativequantification of gene expression was performed using GAPDHmRNA as the internal standard. Two independent experiments wereperformed with similar results, and a representative was shown.The oligonucleotide primers for IL-8, A20, c-IAP2, MCL1, andsurvivin have been described previously (12, 35, 42, 48). Theprimer sequences for other genes, which were designed usingthe Primer Express software (Applied Biosystems), were as follows:XIAP sense, 5'-AGTGGTAGTCCTGTTTCAGCATCA-3', and antisense, 5'-CCGCACGGTATCTCCTTCA-3';GADD45ß sense, 5'-CACGCTCATCCAGTCCTTCTG-3', and antisense,5'-CCGACACCCGCACGAT-3'; BCL10 sense, 5'-TTTTTTGAGACAGTCTTGCTCTATCG-3',and antisense, 5'-AGCATGGGAGGCAGAAGTTG-3'.

Statistical methods. Statistical analysis was performed using the Student's t test,two sided, and Dunnett's post hoc tests for multiple comparisons.Differences were considered statistically significant with P< 0.05.

RESULTS

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Results

Role of IKKs on NF- ${kappa}$ B signaling in H. pylori-infected AGS cells. To investigate the roles of IKK ${alpha}$ and IKKß in H. pylori-infectedAGS cells, we initially performed a reporter assay for NF- ${kappa}$ B-dependenttranscription using kinase mutant forms of IKK ${alpha}$ and IKKß.As reported previously (11, 26), cotransfection of dominant-negativeIKKs decreased H. pylori-mediated NF- ${kappa}$ B reporter activity (Fig.1A), which indicates that the overexpression of dominant-negativeIKK ${alpha}$ or dominant-negative IKKß inhibits NF- ${kappa}$ B activation.We also assessed the effect of IKK gene silencing on this signalingpathway. The siRNAs for IKK ${alpha}$ , IKKß, or nonsilencingcontrol RNA were transfected in AGS cells, and NF- ${kappa}$ B reporteractivity was analyzed with or without H. pylori infection. Similarto the effect of the dominant-negative molecules, IKK ${alpha}$ and IKKßgene silencing decreased by 50% the H. pylori-induced NF- ${kappa}$ B reporteractivation (Fig. 1B).

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FIG. 1. IKK ${alpha}$ and IKKß are involved in H. pylori-induced NF- ${kappa}$ B activation. (A) The kinase mutant expression vector for IKK ${alpha}$ or IKKß, or the empty vector, was transfected into AGS cells together with the NF- ${kappa}$ B reporter and internal control plasmids. After 24 h, the cells were infected with H. pylori or left unstimulated for 8 h. NF- ${kappa}$ B reporter activation was measured. The values shown are the means ± SD; n = 3. (B) AGS cells were transfected with siRNA oligonucleotides for IKK ${alpha}$ , IKKß, or the nonsilencing control for 24 h, followed by transfection of the reporter and control plasmids. The cells were then infected with H. pylori or left unstimulated for 8 h. NF- ${kappa}$ B reporter activation is shown, as described for panel A. (C) AGS cells were treated with siRNA for the control or IKKs. The cells were serum starved for 24 h and then infected with H. pylori for the indicated time. Cell lysates were analyzed by immunoblotting with the indicated antibodies. The protein levels of phospho-I ${kappa}$ B ${alpha}$ or phospho-JNK were measured and normalized with that of actin. A representative of three independent experiments with similar results is shown.

We then performed immunoblots for phosphorylated I ${kappa}$ B ${alpha}$ to revealthe upstream event that leads to NF- ${kappa}$ B activation. As shown inFig. 1C, IKKß silencing dramatically reduced H. pylori-mediatedI ${kappa}$ B ${alpha}$ phosphorylation. In contrast, IKK ${alpha}$ silencing had a very limitedeffect on I ${kappa}$ B ${alpha}$ phosphorylation, although the siRNA for IKK ${alpha}$ apparentlydecreased the IKK ${alpha}$ protein level. These siRNAs for IKKs had onlyslight effects on H. pylori-induced JNK phosphorylation. Thus,we believe that IKK ${alpha}$ is involved in the NF- ${kappa}$ B signaling activationinduced by H. pylori through a mechanism that is distinct fromI ${kappa}$ B phosphorylation, which is transduced via IKKß activation.

Nuclear translocation of IKK ${alpha}$ , but not p100 processing, is induced by H. pylori infection of AGS cells. Recent studies on IKK ${alpha}$ or IKKß knockout cells haverevealed the specific functions of IKKs in cytokine signaling.To elucidate the role of IKK ${alpha}$ in H. pylori infection, we examinedthe IKK ${alpha}$ -specific signaling pathway, namely the processing ofp100, and the nuclear translocation of IKK ${alpha}$ . As reported forother cell lines (9), LT induced both I ${kappa}$ B ${alpha}$ and p100 phosphorylationin AGS cells (Fig. 2A). In LT-treated cells, the p100 levelgradually decreased and that of p52 increased, which indicatesthat LT activates the NF- ${kappa}$ B alternative pathway in this cellline. In contrast, H. pylori infection induced only I ${kappa}$ B ${alpha}$ phosphorylation.Neither p100 phosphorylation nor processing to p52 was observedin H. pylori-treated cells (Fig. 2A). This suggests that thealternative pathway of NF- ${kappa}$ B activation, which includes p100processing to p52, is not induced by H. pylori in AGS cells.To confirm these findings, we also investigated the effect ofH. pylori infection or LT treatment on IKK-silenced cells. Asshown in Fig. 2B, p52 protein induced by LT was severely reducedby IKK ${alpha}$ siRNA but not by IKKß siRNA, which demonstratesthe essential role of IKK ${alpha}$ in the alternative pathway. In contrast,H. pylori infection did not increase the p52 protein level inany cell type, although the basal p52 protein level was slightlyreduced in IKK-silenced cells. We also found that the p100 proteinlevel was increased significantly in H. pylori-infected IKK ${alpha}$ -silencedcells but not in IKKß-silenced cells. This resultalso indicates that p100 is a target gene of NF- ${kappa}$ B in H. pylori-infectedcells, especially via the IKKß-dependent classicalpathway. Collectively, these results clearly demonstrate thatH. pylori does not induce IKK ${alpha}$ -dependent p100 phosphorylationor its processing to p52 in AGS cells, despite p100 inductionvia the IKKß-dependent classical pathway.

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FIG. 2. H. pylori does not induce p100 processing to p52 in AGS cells. (A) AGS cells were treated with H. pylori or LT (50 ng/ml) for the indicated time. The cell lysates were analyzed by immunoblotting with the indicated antibodies. The protein levels of p100 and p52 relative to that of actin were determined. (B) AGS cells were transfected with siRNA oligonucleotides for the control, IKK ${alpha}$ , or IKKß and then treated with H. pylori or LT for 6 h. The cell lysates were analyzed by immunoblotting as described for panel A. H. p, H. pylori.

We also investigated whether H. pylori induces IKK ${alpha}$ nuclear translocation.Nuclear and cytosolic fractions of H. pylori-infected cellswere analyzed by immunoblotting for IKK ${alpha}$ . As shown in Fig. 3A,H. pylori induced IKK ${alpha}$ nuclear accumulation in a time-dependentmanner. Nuclear accumulation of IKK ${alpha}$ was observed 30 min afterinfection and increased for 1.5 h, after which the level remainedthe same. The time course of IKK ${alpha}$ nuclear translocation was similarto that of p50 nuclear translocation.

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FIG. 3. H. pylori infection induces IKK ${alpha}$ nuclear translocation in AGS cells. (A) AGS cells were infected with H. pylori for the indicated time or treated with TNF- ${alpha}$ for 2 h. The cells were fractioned into nuclear and cytosolic extracts. Aliquots of these extracts were analyzed by immunoblotting for IKK ${alpha}$ and p50. Antibodies directed against TRAF2 and TF-IID were used to verify the integrity of the fractionation procedure and to ensure equal loading. A representative of three independent experiments with similar results is shown. (B) AGS cells seeded in 4-well chamber slides were left untreated or were infected with H. pylori for 1 h. The cells were immunostained with the anti-IKK ${alpha}$ antibody and visualized by staining with Alexa Fluor 488. The nucleus was stained with propidium iodide. Phase-contrast images and merged images are shown. Arrows indicate the cells with IKK ${alpha}$ nuclear staining. (C) AGS cells were infected with H. pylori for the indicated time, and IKK ${alpha}$ nuclear translocation was assessed by immunofluorescence. The percentages of cells with IKK ${alpha}$ nuclear staining cells are calculated from the observation of 300 cells in three independent experiments and are indicated as the means ± SD. *, P < 0.05.

We also performed immunofluorescence staining to confirm IKK ${alpha}$ nuclear translocation. In uninfected AGS cells, IKK ${alpha}$ was localized,mainly in the cytosol. However, upon infection, nuclear stainingof IKK ${alpha}$ was observed in about 15 to 20% of the cells (Fig. 3B and C).These results indicate that H. pylori activates IKK ${alpha}$ and induces its nuclear translocation but does not induce p100processing in AGS cells.

Factors associated with H. pylori-induced IKK ${alpha}$ nuclear translocation. H. pylori activates the intracellular signaling pathways ofepithelial cell lines in MOI-dependent and cag PAI-dependentmanners (21, 22, 26). Thus, we investigated whether these bacterialfactors also affect IKK ${alpha}$ nuclear translocation. AGS cells wereinfected with H. pylori at the indicated MOI for 2 h, and nuclearextracts were subjected to immunoblotting for IKK ${alpha}$ . As shownin Fig. 4A, IKK ${alpha}$ nuclear accumulation was observed in cells thatwere infected with H. pylori at an MOI of 10. The levels ofIKK ${alpha}$ and p50 in the nucleus increased in relation to increasesin the infection ratio, up to an MOI of 100.

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FIG. 4. Factors associated with H. pylori-induced IKK ${alpha}$ nuclear translocation. (A) AGS cells were infected with H. pylori at the indicated MOI for 2 h. The nuclear extracts were immunoblotted for IKK ${alpha}$ , p50, and TF-IID. (B) AGS cells were infected with various isogenic mutants of H. pylori strain TN2 at an MOI of 100 for 2 h. Immunoblotting of nuclear extracts was performed as described for panel A. (C) AGS cells were transfected with siRNA for the nonsilencing control, TAK1, IKK ${alpha}$ , or IKKß for 48 h and subsequently infected with H. pylori for 2 h. The nuclear and cytosolic fractions were extracted and analyzed by immunoblotting. WT, wild type.

We also investigated the roles of bacterial virulence factorsin IKK ${alpha}$ nuclear translocation using cagA, cagE, cag PAI, andvacA mutant strains. Immunoblot analysis revealed that genedisruption of cagE or cag PAI reduced IKK ${alpha}$ nuclear accumulation(Fig. 4B). In contrast, in cagA and vacA mutant-infected cellswe observed almost the same level of nuclear IKK ${alpha}$ and p50 asin wild-type-infected cells. These results indicate that thecag PAI molecular transportation system is required for IKK ${alpha}$ activation. Although the CagA and VacA proteins are bacterialcytotoxins that enter epithelial cells (32, 36), these bacterialtoxins themselves do not induce either NF- ${kappa}$ B activation or IKK ${alpha}$ nuclear translocation.

We then assessed the upstream signaling event for IKK complexactivation. Several studies have revealed that TAK1 transducescytokine signaling to the IKK complex. Therefore, we used siRNAsfor TAK1 and IKKs to examine the importance of these moleculesfor H. pylori-induced IKK ${alpha}$ nuclear translocation. As shown inFig. 4C, TAK1 silencing reduced the nuclear translocation ofIKK ${alpha}$ as well as that of p50. In contrast, IKKß silencinghad no effect on IKK ${alpha}$ localization while p50 nuclear translocationwas severely inhibited. These results indicate that TAK1 isan important signaling intermediate for H. pylori-induced NF- ${kappa}$ Bactivation, which bifurcates upstream of the stimulus to bothIKK ${alpha}$ and IKKß.

The role of IKKs in H. pylori-induced epithelial cell responses. It has been reported that NF- ${kappa}$ B activation induced by H. pylorimediates cytokine production and antiapoptosis in gastric epithelialcells. Therefore, we assessed whether IKK ${alpha}$ activation in gastriccells affects these cellular responses. IL-8 production by H.pylori-infected AGS cells was measured by ELISA. In the controlcells, approximately 2,400 pg/ml IL-8 was produced after 8 hof H. pylori infection. However, cells treated with the IKK ${alpha}$ or IKKß siRNA showed severely decreased levels ofIL-8 production. In the IKK ${alpha}$ -silenced cells, H. pylori inducedabout 1,200 pg/ml IL-8, which was approximately half the levelinduced in the control cells (Fig. 5A). Another chemokine observedin H. pylori-infected gastric mucosa, GRO ${alpha}$ , has also been reportedto have chemotactic activities for neutrophils (47). The productionof GRO ${alpha}$ by H. pylori-infected cells was also reduced by IKK ${alpha}$ orIKKß silencing (Fig. 5B). These results indicate thatboth IKK ${alpha}$ and IKKß are necessary for chemokine production.

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FIG. 5. The roles of IKK ${alpha}$ and IKKß in H. pylori-induced inflammatory and antiapoptotic responses. (A and B) AGS cells were transfected with the indicated siRNAs for 48 h and were cultured with or without H. pylori for 8 h. The culture supernatants were assayed for IL-8 (A) or GRO ${alpha}$ (B) by ELISA. The values are the means ± SD from three independent experiments. *, P < 0.01; **, P < 0.05. (C) AGS cells were transfected with the indicated siRNAs, serum starved for 24 h, and subsequently infected with H. pylori for 8 h. The numbers of TUNEL-positive cells were calculated from more than 1,500 cells per slide in three independent experiments. The values are the means ± SD. *, P < 0.05; NS, not significant.

We also assessed the role of each IKK on cellular apoptosis.Using TUNEL staining, we evaluated the effect of H. pylori infectionon serum starvation-induced apoptosis. In control siRNA-transfectedcells, about 0.6% of the cells were apoptotic (Fig. 5C). Thepercentage of apoptotic cells was similar after IKK ${alpha}$ silencing.However, in the case of IKKß silencing, H. pyloriinfection enhanced the apoptosis of AGS cells (2.2% ±0.7%; P < 0.05 compared to control transfected cells). Theseresults indicate that the antiapoptotic effect of H. pyloriis transduced mainly through IKKß activation.

The role of IKKs in H. pylori-induced gene transcription. We next investigated the IKK ${alpha}$ target genes in H. pylori-infectedAGS cells. Cells that were treated with control or IKK-specificsiRNAs were infected with H. pylori for 3 h, and the transcriptionalprofiles were determined by microarray analysis. In the controloligonucleotide-transfected AGS cells, H. pylori infection up-regulated181 out of 21,000 genes. The 181 genes included those for immuneresponses, antiapoptosis, and signal transduction; representativegenes are shown in Table 1. Using siRNA, we found 15 of thegenes with enhanced expression were down-regulated more than20% by IKK ${alpha}$ silencing, and 25 of the genes were down-regulatedby IKKß silencing (Table 2). Interestingly, 12 outof 15 of the IKK ${alpha}$ -regulated genes were identical to IKKß-regulatedgenes. These results, based on microarray experiments, indicatethat most of the IKK ${alpha}$ target genes in H. pylori-infected AGScells are similar to IKKß target genes, which areactivated via the NF- ${kappa}$ B classical pathway. In addition, it appearsthat the induction of several genes, such as NF- ${kappa}$ B1 and CXCL2,requires signaling via IKKß, but not via IKK ${alpha}$ , forstimulus-dependent transcriptional activation.

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TABLE 1. Identification of genes that are enhanced by H. pylori infection^a

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TABLE 2. Genes regulated by IKKs in H. pylori-infected AGS cells^a

To confirm the microarray data and to evaluate sequential changesin gene induction, we performed real-time PCR for several genes.As shown in Fig. 6, the expression of IL-8 (A), cIAP2 (B), andMCL1 (C) was up-regulated by H. pylori infection but was effectivelyinhibited by the siRNAs for either IKK. These results are inaccordance with the microarray data. A20 (D), which negativelyregulates NF- ${kappa}$ B activity and is involved in antiapoptosis, wasalso up-regulated by H. pylori infection in a time-dependentmanner and down-regulated by IKK silencing. A20 induction wasnot observed in the current microarray experiments, althoughit was observed in a previous study (28). In contrast to theseH. pylori-inducible genes, other antiapoptotic genes were notaffected (E to H). Thus, IKK ${alpha}$ and IKKß appear to beequally involved in H. pylori-induced antiapoptotic gene expression,although the antiapoptotic phenotypes observed in cells silencedfor individual IKK subunits were different (Fig. 5C).

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FIG. 6. Sequential analysis of H. pylori-induced gene expression in IKK-silenced cells. (A to H) AGS cells were transfected with the indicated siRNAs for 48 h and were then infected with H. pylori for 0, 1.5, 3, and 6 h. The cDNA prepared from these cells was investigated for the indicated gene expression relative to GAPDH by real-time PCR. The reaction was performed in triplicate, and the data are shown as the means ± SD. Reverse transcription-PCR was performed from two independent infection experiments with similar results. The black diamond ( ${blacklozenge}$ ) represents the control siRNA-transfected cells, and the open square ( ${square}$ ) and open triangle ( ${triangleup}$ ) represent IKK ${alpha}$ and IKKß siRNA-transfected cells, respectively. *, P < 0.05 versus control siRNA-transfected cells.

DISCUSSION

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Discussion

In this report, we have examined the roles of IKK ${alpha}$ and IKKßin H. pylori-infected gastric cancer cells. Both of these kinasesare involved in NF- ${kappa}$ B activation and inflammatory cytokine production.IKKß is considered to act as a physiological I ${kappa}$ B kinaseduring H. pylori infection, while IKK ${alpha}$ does not have this activity.Our results reveal that H. pylori induces the nuclear translocationof IKK ${alpha}$ , which may be one of the important roles of IKK ${alpha}$ in gastriccancer cells. Chemokine expression induced by H. pylori infectionwas repressed by both IKK siRNAs, although the antiapoptoticeffects were abrogated only in IKKß-silenced cells.Thus, IKK ${alpha}$ and IKKß seem to regulate independent cellresponses through different mechanisms of NF- ${kappa}$ B activation inH. pylori-infected gastric cancer cells.

Although both IKK ${alpha}$ and IKKß were discovered as stimulus-dependentkinases of I ${kappa}$ B that are structurally related to each other, theirroles in cell biology may be different. IKKß is consideredto be an essential signal transducer in cytokine-mediated NF- ${kappa}$ Bactivation, thereby promoting cell survival and preventing apoptosis(24, 25, 49). However, in our analysis of H. pylori-infectedcells, not only the siRNA for IKKß but also the siRNAfor IKK ${alpha}$ reduced NF- ${kappa}$ B reporter activity. Therefore, we investigatedthe role of IKK ${alpha}$ in the NF- ${kappa}$ B pathway in AGS cells, especiallywith respect to IKK ${alpha}$ -specific signaling. We found that H. pyloriinduces the nuclear translocation of IKK ${alpha}$ , which was first reportedin TNF- ${alpha}$ -treated cells (1, 46). Similar to the classical NF- ${kappa}$ Bactivation mode (21, 26), IKK ${alpha}$ nuclear translocation is inducedby H. pylori in cag PAI- and MOI-dependent manners. Many bacterialcomponents, such as peptidoglycan, lipopolysaccharide, and flagellin,are known to target cellular receptors, called Toll-like receptors,and to induce I ${kappa}$ B ${alpha}$ phosphorylation and NF- ${kappa}$ B activation (reviewedin references 17 and 29). However, it has not been establishedwhether these bacterial components induce IKK ${alpha}$ nuclear translocationand inflammatory gene expression. Since the nontoxic H. pyloricag PAI mutant did not induce this type of signaling, the IKK ${alpha}$ activation observed for cag-positive strains in our experimentsis possibly associated with severe gastric disease.

Interestingly, H. pylori did not induce the activation of thealternative NF- ${kappa}$ B pathway in AGS cells. Recent studies have shownthat certain stimuli, such as LT, BAFF, and CD40, induce p100processing to p52, which then translocates into the nucleustogether with RelB (3, 9, 39). Furthermore, lipopolysaccharideactivates the alternative pathway in pre-B cells or primarydendritic cells (31). In our experiment, LT stimulation inducedp100 phosphorylation and increased p52 in the AGS cells. Thus,this cell line has a normal response with respect to alternativepathway signal transduction but is defective for activationof the H. pylori-mediated alternative pathway. H. pylori alsofailed to phosphorylate p100 in AGS cells. Collectively, theseresults indicate that H. pylori does not activate IKK ${alpha}$ kinaseactivity in this cell line, in spite of the ability of IKK ${alpha}$ toundergo nuclear translocation (Fig. 7). These results also suggestthat epithelial cell lines, such as AGS and MKN45, are not stimulatedby H. pylori lipopolysaccharide to activate either the classicalor alternative NF- ${kappa}$ B pathway (27). In contrast to the unresponsivenessof epithelial cells, we have found that H. pylori induces activationof the alternative pathway in lymphocytes and fibroblasts (34).Thus, it appears that the ability of H. pylori to activate thealternative NF- ${kappa}$ B pathway is cell type dependent.

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FIG. 7. Schematic representation of the role of IKK in human gastric cancer cells. The signalings activated by H. pylori are indicated with a boldface solid line, and those induced by LT are indicated with a broken line. cag-positive H. pylori activated TAK1 and IKK complex, followed by a classical pathway activation via IKKß and by IKK ${alpha}$ nuclear translocation in AGS cells. In contrast, LT induced classical pathway activation as well as alternative pathway activation through p100 processing.

Nuclear translocation of IKK ${alpha}$ is reported to regulate gene expressionby modifying histone function in TNF-stimulated cells. The kinaseactivity of IKK ${alpha}$ is considered to be essential for this process(1, 46). In contrast, for keratinocyte differentiation and normalmorphological development, which are also reported to be dependenton IKK ${alpha}$ , the kinase activity is not required, although its nucleartranslocation is indispensable (41). In this process, IKK ${alpha}$ isassociated with the suppression of the fibroblast growth factorfamily of genes, possibly via an indirect mechanism (41). Sinceit is difficult to determine the essential role of IKK ${alpha}$ in vivo,which may depend on the type and strength of the stimulus, thecell type, and cell environment, we have investigated IKK ${alpha}$ functionin H. pylori-infected gastric cells. In our experiments, IKK ${alpha}$ appeared to act as a positive regulator of gene expression,thereby resembling IKKß, since in microarray experimentsH. pylori-induced expression of chemokines and antiapoptoticgenes was repressed to a similar extent by IKK ${alpha}$ or IKKßsilencing.

In this study, IKK ${alpha}$ nuclear translocation was observed within30 min of H. pylori infection, which is similar to the timerequired for I ${kappa}$ B phosphorylation by IKKß and whichis clearly different from the kinetics of alternative pathwayactivation by other ligands, which usually takes several hours(9, 31). Furthermore, we have clarified that TAK1 is an importantupstream molecule for both IKK ${alpha}$ nuclear translocation and IKKß-dependentp50 nuclear translocation. As TAK1 is reported to be the criticalactivator of IKK in cytokine stimulation (33, 42), it is possiblethat TAK1 is the common upstream molecule for the IKKß-dependentclassical pathway and IKK ${alpha}$ nuclear translocation in H. pylori-infectedcells. Furthermore, we found that both IKKs were involved inNF- ${kappa}$ B activation and chemokine production in H. pylori-infectedcells. Thus, we speculate that both IKK ${alpha}$ nuclear translocationand IKKß-dependent I ${kappa}$ B phosphorylation are requiredfor sufficient gene expression by H. pylori (Fig. 7).

The antiapoptotic responses induced by H. pylori seemed to betransduced via IKKß. To elucidate these IKK phenotypicdifferences, we carried out a comprehensive and sequential analysisof the antiapoptotic genes in IKK silencing cells. Similar toprevious reports on cDNA array experiments of H. pylori-inducedgene expression, we found that genes associated with immuneresponses and signal transductions, such as IL-8, CXCL1, CXCL2,IkBa, p105, and ICAM-1, were up-regulated in AGS cells by H.pylori infection (7, 13, 28). Most of these genes were shownto be induced by cag-positive H. pylori infection. This is consistentwith our results demonstrating that these genes were suppressedby IKK silencing, as IKK activation by H. pylori was dependenton cag PAI. Furthermore, it has been reported that H. pyloriupregulates antiapoptotic genes like MCL1, cIAP2, A20, and GG2.1(13, 28, 40, 48). We also found a critical role of IKKs in antiapoptoticgene regulation (Table 2). However, in spite of the differencesin antiapoptotic effects (Fig. 5C), we could not find the differencesin antiapoptotic gene regulation between IKK ${alpha}$ -silencing cellsand IKKß-silencing cells. Thus, it is possible thatIKKß affects antiapoptosis not through gene regulationbut through other biological processes, such as posttranscriptionalmodification via its kinase activity. Previous reports on IKKßknockout cells have shown that the inactivation of NF- ${kappa}$ B signalingenhances JNK activity and affects proapoptosis (44). In ourexperiments using IKK-silenced cells, the enhancement of JNKactivity was not apparent. Furthermore, H. pylori infectiondid not enhance the expression of the XIAP gene (Fig. 6E), whichis reported to activate JNK. Since our experiments failed toclarify the IKKß-dependent antiapoptotic mechanism,further investigations of IKKß will facilitate theunderstanding of gastric diseases associated with dysregulatedapoptosis.

In conclusion, we have investigated the function of IKK ${alpha}$ in theH. pylori infection model using AGS cells. IKK ${alpha}$ is translocatedinto the nucleus upon infection, and chemokine expression isinduced via IKK ${alpha}$ . These results suggest that IKK ${alpha}$ activation inthe gastric mucosa is associated with severe inflammation andinflammation-induced carcinogenesis in vivo, as is IKKß.

ACKNOWLEDGMENTS

This study was supported in part by a grant from the SankyoFoundation of Life Science.

We thank Mitsuko Tsubouchi for her excellent technical assistance.

FOOTNOTES

* Corresponding author. Mailing address: Department of Gastroenterology, University of Tokyo, 7-3-1 Hongo, Bunkyo-ku, Tokyo 113-8655, Japan. Phone: 81-3-3815-5411. Fax: 81-3-3814-0021. E-mail: yohirata-tky{at}umin.ac.jp.

Editor: J. B. Bliska

REFERENCES

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