Role of p90 Ribosomal S6-Kinase-1 in Oltipraz-Induced Specific Phosphorylation of CCAAT/Enhancer Binding Protein-beta for GSTA2 Gene Transactivation

doi:10.1124/mol.105.018465

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First published on October 24, 2005; DOI: 10.1124/mol.105.018465

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Mol Pharmacol 69:385-396, 2006

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Role of p90 Ribosomal S6-Kinase-1 in Oltipraz-Induced Specific Phosphorylation of CCAAT/Enhancer Binding Protein- $beta$ for GSTA2 Gene Transactivation

Seung Jin Lee, and Sang Geon Kim

National Research Laboratory, College of Pharmacy and Research Institute of Pharmaceutical Sciences, Seoul National University, Seoul, Korea

Received August 29, 2005; accepted October 24, 2005

Abstract

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Abstract
Materials and Methods
Results
Discussion
References

Oltipraz, which has been extensively studied as a cancer chemopreventiveagent, promotes phosphatidylinositol 3-kinase-mediated activationof CCAAT/enhancer binding protein- $beta$ (C/EBP $beta$ ). Activated p90 ribosomalS6-kinase-1 (RSK1) phosphorylates major transcription factors,including C/EBP $beta$ . This study examined whether oltipraz inducesphosphorylation of C/EBP $beta$ at specific residues, and if so, whetherRSK1 regulates C/EBP $beta$ phosphorylation by oltipraz for the GSTA2gene transactivation. Subcellular fractionation and immunoblotanalyses revealed that oltipraz treatment increased the levelof C/EBP $beta$ phosphorylated at Ser¹⁰⁵ in the cytoplasm, which translocatedto the nucleus for DNA binding in rat H4IIE cells. Immunoprecipitation-immunoblot,chromatin-immunoprecipitation, and specific mutation analysesrevealed that Ser¹⁰⁵-phosphorylated C/EBP $beta$ recruited the cAMPresponse element-binding protein binding protein for histoneacetylation and transactivation of the GSTA2 gene. The roleof RSK1 in Ser¹⁰⁵-phosphorylation of C/EBP $beta$ by oltipraz and itsgene transactivation was evidenced by transfection experimentswith dominant-negative mutants of RSK1. In mouse Hepa1c1c, humanHepG2 cells, and rat primary hepatocytes, oltipraz induced phosphorylationof C/EBP $beta$ at Thr²¹⁷, Thr²⁶⁶, and Ser¹⁰⁵, respectively, via RSK1.The experiment using small-interference RNA of RSK1 confirmedthe essential role of RSK1 in the gene expression. Inhibitionof PI3-kinase activity prevented oltipraz-inducible Ser¹⁰⁵-phosphorylationof rat C/EBP $beta$ . Oltipraz treatment led to increases in the catalyticactivity and nuclear translocation of RSK1, which was abrogatedby PI3-kinase inhibition. In summary, oltipraz induces the phosphorylationof rat C/EBP $beta$ at Ser¹⁰⁵ (functionally analogous Thr^217/266 inmouse and human forms) in hepatocytes, which results in cAMPresponse element-binding protein-binding protein (CBP) recruitmentfor the GSTA2 gene transactivation, and the specific C/EBP $beta$ phosphorylationis mediated by RSK1 downstream of PI3-kinase.

Oltipraz (5-[2-pyrazinyl]-4-methyl-1,2-dithiol-3-thione) hasbeen studied extensively as a cancer chemopreventive agent formalignancies, including liver and colorectal cancer (Rao etal., 1993

; Kensler, 1997

). In experimental cancer preventionstudies, oltipraz reduced tumor incidence and multiplicity (Roebucket al., 1991

; Bolton et al., 1993

; Kensler, 1997

). A phase IIarandomized chemoprevention trial of oltipraz in residents ofQidong, China, supported that oltipraz might be clinically activeas a chemopreventive agent (Jacobson et al., 1997

; Wang et al.,1999

). Comprehensive mechanistic studies suggest that oltiprazexerts cancer chemopreventive effects through the inductionof glutathione S-transferase, a representative phase II detoxifyingenzyme (Jacobson et al., 1997

; Kensler, 1997

The family of C/EBPs plays important roles in regulating theexpression of hepatocyte-specific genes, particularly thoseassociated with cell survival or proliferation (Diehl, 1998;Buck and Chojkier, 2003). We reported that oltipraz promotesnuclear translocation of CCAAT/enhancer binding protein- $beta$ (C/EBP $beta$ )and its DNA binding activity for transactivation of the GSTA2gene, and that the pathway of phosphatidylinositol 3-kinase(PI3-kinase) regulates the activation of C/EBP $beta$ (Cho and Kim,2003b; Kang et al., 2003). In addition, we observed that mitogen-activatedprotein kinases (MAPKs), including ERK1/2, were neither activatedby oltipraz nor involved in C/EBP $beta$ -mediated gene expression (Kanget al., 2003). Yet, the kinase(s) responsible for the activationof C/EBP $beta$ by oltipraz remained to be elucidated. Therefore, weproposed the hypothesis that oltipraz activates C/EBP $beta$ by phosphorylationat specific site(s), which may be mediated by cellular kinase(s)downstream from PI3-kinase.

The members of p90 ribosomal S6-kinase (RSK) family play a criticalrole in mitogen-activated cell growth, differentiation, or survival(Bhatt and Ferrell, 1999; Frodin and Gammeltoft, 1999; Grosset al., 1999). Among the RSK isoforms, RSK1 is a major formexpressed in the tissues, including liver, muscle, and fat (Molleret al., 1994). The RSK1 contains two distinct kinase domainsthat are functionally active, and the N-terminal kinase of activatedRSK1 phosphorylates the cellular protein substrates, includingC/EBP $beta$ , cAMP response element-binding protein, c-Fos, and I ${kappa}$ B(Chen et al., 1993; Xing et al., 1996; Ghoda et al., 1997; Schoutenet al., 1997; Buck et al., 1999; Frodin and Gammeltoft, 1999).Activation of RSK1 by growth factor requires extracellular signal-regulatedkinase (ERK) docking near the C-terminal region (Roux et al.,2003), and the activated C-terminal kinase domain leads to autophosphorylation,located in the linker region (Vik and Ryder, 1997). Anotherphosphorylation by 3-phosphoinositide-dependent protein kinase-1(PDK1) in the activation loop of the N-terminal kinase domainallows RSK1 to phosphorylate the target proteins (Jensen etal., 1999; Richards et al., 1999; Williams et al., 2000).

Receptor-activated signaling pathways regulate phosphorylationof C/EBP $beta$ in its activation domain (Buck and Chojkier, 2003),which leads to the transcription of its target genes. It hasbeen shown that RSK activated downstream from the transforminggrowth factor- ${alpha}$ receptor tyrosine kinase induces phosphorylationof C/EBP $beta$ at specific residues such as Thr²¹⁷ in the mouse form(Buck et al., 1999). Phosphorylation of Thr²¹⁷ residue in mouseC/EBP $beta$ (Thr²⁶⁶ in the human form) turned out to be essentialfor transactivation of target genes (Buck and Chojkier, 2003).Because rat C/EBP $beta$ has evolved with a double mutation and thuslacks the phosphoacceptor, the C/EBP $beta$ form has a compensatorySer¹⁰⁵, whose phosphorylation is also catalyzed by RSK (Buckand Chojkier, 2003). Hence, Ser¹⁰⁵ residue in rat C/EBP $beta$ andfunctionally analogous residues Thr²¹⁷ and Thr²⁶⁶ in mouse andhuman forms, respectively, are the critical phosphoacceptorsthat are responsible for gene transactivation (Buck et al.,1999). In addition, C/EBP $beta$ phosphorylated at the specific residueby RSK1 nontranscriptionally prevents apoptosis of cells throughthe interaction with procaspases (Buck et al., 2001). Hence,RSK1-mediated specific phosphorylation of C/EBP $beta$ regulates cellsurvival.

In view of the activation of C/EBP $beta$ by oltipraz and the essentialrole of Ser¹⁰⁵ phosphorylation (analogous phosphorylations atThr^217/266 in mouse and human) in gene transactivation, we investigatedwhether oltipraz induces C/EBP $beta$ phosphorylation at the residuefor the GSTA2 gene transactivation and, if so, whether the phosphorylationof C/EBP $beta$ is mediated by RSK1. We additionally determined theeffects of oltipraz on Thr²¹⁷ or Thr²⁶⁶ phosphorylation in themouse and human forms of C/EBP $beta$ , respectively, and the role ofRSK1 in the phosphorylations. In addition, we verified the specificC/EBP $beta$ phosphorylation by RSK1 in primary cultured rat hepatocytes.Toward the end, we explored what the role of PI3-kinase is inRSK1-mediated C/EBP $beta$ phosphorylation by oltipraz. Now, we reportthat oltipraz induces specific C/EBP $beta$ phosphorylation for theGSTA2 gene transactivation via RSK1 and that PI3-kinase contributesto the RSK1-mediated phosphorylation of C/EBP $beta$ .

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
References

Materials. [ ${gamma}$ -³²P]ATP (3000 mCi/mmol) was purchased from PerkinElmerLife and Analytical Sciences (Boston, MA). Anti-C/EBP ${alpha}$ , anti-C/EBP $beta$ ,anti-C/EBP ${delta}$ , anti-Ser¹⁰⁵-phosphorylated C/EBP $beta$ (sc-16994-R), anti-Thr²¹⁷-phosphorylatedC/EBP $beta$ (sc-16993-R), anti-CBP, anti-RSK1, anti-HA, anti-Myc,and anti-actin antibodies were obtained from Santa Cruz Biotechnology(Santa Cruz, CA). Anti-acetylated histone antibody was purchasedfrom Upstate Biotechnology (Waltham, MA). Anti-Thr¹⁸⁹-phosphorylatedC/EBP $beta$ , anti-ERK, and anti-Thr^42/44-phosphorylated ERK antibodieswere supplied from Cell Signaling Technology (Beverly, MA).Horseradish peroxidase-conjugated goat anti-rabbit and rabbitanti-goat IgGs were purchased from Zymed Laboratories (San Francisco,CA). U0126 was obtained from Alexis Corporation (Läufelfingen,Switzerland). LY294002 and other reagents in the molecular studieswere supplied from Calbiochem (Darmstadt, Germany). S6 rsk substratepeptide was purchased from Santa Cruz Biotechnology. The plasmidof C/EBP-containing GSTA2 promoter region (-1651 bp to +66 bp)was kindly provided by Dr. C. B. Pickett (Schering Plough, Kenilworth,NJ). The plasmids encoding HA-C-terminal truncated (CTT)-RSK1and HA-K112/464R-RSK1 were kind gifts from Dr. J. Blenis (HarvardMedical School, Boston, MA). The overexpression vector of p85subunit of PI3-kinase was obtained from Dr. A. Toker (The BostonBiomedical Research Institute, Boston, MA). MKK1 dominant-negativemutant was a gift from Dr. N G. Ahn (University of Colorado,Boulder, CO).

Cell Culture. Rat H4IIE, mouse Hepa1c1c, and human HepG2 cellswere obtained from American Type Culture Collection (Manassas,VA). Primary hepatocytes were isolated from male Sprague-Dawleyrats according to the method published previously, with slightmodifications (Buck et al., 2001; Kang et al., 2003). Cellswere maintained in Dulbecco's modified Eagle's medium containing10% fetal calf serum (FCS), 50 U/ml penicillin, and 50 µg/mlstreptomycin at 37°C in a humidified atmosphere with 5%CO₂. After deprivation of serum for 24 h, the cells were incubatedwith oltipraz (CJ Corp., Seoul, Korea) and dissolved in dimethylsulfoxide for the indicated time period at 37°C.

Subcellular Fractionation. Total cell lysates, cytosolic fractions,and nuclear extracts were prepared according to methods publishedpreviously (Park et al., 2004). In brief, cells were centrifugedat 2300g for 3 min and allowed to swell after the addition ofthe lysis buffer. The lysate samples were centrifuged at 10,000gfor 10 min to obtain cell lysates. To prepare cytosolic fractionsand nuclear extracts, cells were centrifuged at 2300g for 3min and allowed to swell after the addition of 100 µlof hypotonic buffer. The lysates were incubated for 10 min onice and then centrifuged at 7200g for 5 min at 4°C. Thesupernatants were used as cytosolic fractions. Pellets containingcrude nuclei were resuspended in 50 µl of extraction buffer.Nuclear extracts were prepared from the samples by centrifugationat 15,000g for 10 min and stored -70°C until use. Proteincontent was determined by the Bradford assay (Bio-Rad proteinassay kit; Bio-Rad, Hercules, CA).

Immunoblot Analysis. SDS-polyacrylamide gel electrophoresisand immunoblot analysis were performed according to procedurespublished previously (Kang et al., 2003).

Gel Shift Assay. A double-stranded probe containing the C/EBPconsensus oligonucleotide was used for gel shift analysis afterend-labeling of the probe with [ ${gamma}$ -³²P]ATP and T₄ polynucleotidekinase, as described previously (Kang et al., 2003; Park etal., 2004). Specificity of binding was determined by competitionexperiments, known as immunoinhibition assays. For immunoinhibitionassays, anti-Ser¹⁰⁵-phosphorylated C/EBP $beta$ , anti-Thr¹⁸⁹-phosphorylatedC/EBP $beta$ , or anti-Sp1 antibody (1 µg each) was added to thereaction mixture after initial 10-min incubation and additionallyincubated with the probe for 30 min at 25°C. Samples wereloaded onto 4% polyacrylamide gels at 100 V. The gels were removed,fixed, and dried, followed by autoradiography.

Immunoprecipitation. To determine the physical interaction ofCBP with Ser¹⁰⁵-phosphorylated C/EBP $beta$ , a fraction of cell lysates(100-µg proteins in 300 µl) was incubated with apolyclonal rabbit anti-CBP antibody overnight at 4°C. Theantigen-antibody complex was immunoprecipitated after incubationfor 2 h at 4°C with protein G-agarose. Immune complex wassolubilized in 2x Laemmli buffer and boiled for 5 min. Sampleswere separated and analyzed using 7.5% SDS-polyacrylamide gelelectrophoresis and then transferred to nitrocellulose membranes.The samples were then immunoblotted with antibodies directedagainst Ser¹⁰⁵- or Thr¹⁸⁹-phosphorylated C/EBP $beta$ . Blots were developedusing an ECL chemiluminescence detection kit.

Chromatin Immunoprecipitation Assays. H4IIE cells were treatedwith oltipraz for 12 h, and then formaldehyde was added to thecells to a final concentration of 1%. Ser¹⁰⁵-phosphorylatedC/EBP $beta$ , CBP, or acetylated histone was cross-linked to chromatinby incubating the cells for 10 min at 37°C. The cells werewashed with ice-cold phosphate-buffered saline and lysed inthe Tris-HCl buffer (50 mM), pH 8.1, containing 1% SDS and 10mM EDTA. The lysates were sonicated and centrifuged at 10,000gfor 10 min to remove debris. The supernatants containing chromatinwere diluted with 10 volumes of the chromatin immunoprecipitation(ChIP) dilution buffer (16.7 mM Tris-HCl, pH 8.1, 167 mM NaCl,1.2 mM EDTA, 0.01% SDS, and 1.1% Triton X-100). One tenth ofthe chromatin solution was reserved for total input. The remainingsolution was precleared with protein G-agarose, subsequentlyincubated with each antibody (1 µg) for 12 h at 4°Cwith shaking, and then further incubated with protein G-agarosefor 2 h. The immunoprecipitates were washed, reverse cross-linkedby adding 5 M NaCl to a final concentration of 200 mM, and incubatedfor 4 h at 65°C, as described previously (Duong et al.,2002). ChIP assay was also carried out with anti-Thr¹⁸⁹-phosphorylatedC/EBP $beta$ antibody, which was used as a negative control. DNA wasphenol-chloroform-extracted. PCR was performed with specificprimers flanking the C/EBP binding site in the GSTA2 gene promoter(sense: 5'-GGACAACACACTCAGCTTTG-3'; antisense: 5'-TCAGTGCAGCCTGTGAGTC-3')or flanking the $beta$ -actin gene promoter (sense: 5'-CGTTCCGAAATTGCCTTTTA-3';antisense: 5'-GGAGCTGCAAGGAGGTTGTA-3'). Amplified fragments(347 bp, 121 bp) were analyzed on a 2% agarose gel.

Mutagenesis Assay. C/EBP $beta$ amplified from pCDNA3.1(+)-rat C/EBP $beta$ (Cho and Kim, 2003a) using specific primers was inserted intopGEM-T vector (Promega, Madison, WI) and subcloned into theBamHI/HindIII sites of the pCMV-Tag3A plasmid (Stratagene, LaJolla, CA). Specific base substitution was made by oligonucleotide-mediatedmutagenesis according to the manufacturer's instruction (Stratagene).Ser¹⁰⁵ residue in rat C/EBP $beta$ was mutated to alanine using a mutagenicprimer (5'-GTAACCGTAGTCGGCCGGCTTCTTGCTCGG-3'). The DNA sequencewas verified by using an automatic DNA sequence analyzer.

Transient Transfection and pGL-1651 Promoter-Luciferase Assay.To determine the activity of C/EBP $beta$ -mediated target gene transactivation,we used the pGL1651-luciferase reporter assay system accordingto the procedures published previously (Cho and Kim, 2003b;Park et al., 2004). Cells were transiently transfected withpGL1651-promoter luciferase construct in combination with theplasmid of pCMV-Tag3A-C/EBP $beta$ or pCMV-Tag3A-C/EBP $beta$ -S105A (Ala¹⁰⁵mutant of rat C/EBP $beta$ ). In some experiments, HA-CTT-RSK1 or HA-K112/464R-RSK1plasmid was cotransfected with the pGL-1651 construct. In brief,cells (5 x 10⁵ cells/well) were replated in six-well platesovernight, serum-starved for 6 h, and transiently transfectedwith 1 µg of pGL-1651-luciferase construct and 0.3 µgof pCMV- $beta$ -galactosidase plasmid in the presence of Lipofectaminereagent (both from Invitrogen, Carlsbad, CA) for 3 h. The pCMV- $beta$ -galactosidaseplasmid was used to evaluate the transfection efficiency. Transfectedcells were incubated in Dulbecco's modified Eagle's medium containing1% FCS for 3 h and exposed to oltipraz for 18 h at 37°C.For $beta$ -galactosidase activity, 10 µg of cell lysates wasadded to the solution containing 0.88 mg/ml o-nitrophenyl- $beta$ -D-galactopyranoside,100 µM MgCl₂, and 47 mM $beta$ -mercaptoethanol in 100 mM sodiumphosphate buffer. The reaction mixture was incubated for 12h at 37°C, and the absorbance was determined at 420 nm.The relative luciferase activity was calculated by normalizingfirefly luciferase activity to that of $beta$ -galactosidase.

H4IIE, Hepa1c1c, HepG2 cells, or primary cultured rat hepatocyteswere also transiently transfected with the plasmid encodingHA-CTT-RSK1 or HA-K112/464R-RSK1 and incubated for the indicatedtime period to assess the extent of C/EBP $beta$ phosphorylation.

Knockdown Experiment Using siRNA. To knockdown RSK1, HepG2 cellswere transfected with the siRNA against human RSK1 (Silencer-validatedsiRNA against RSK1, Ambion, Austin, TX). pGL-1651-promoter luciferaseconstruct was cotransfected with the RSK siRNA or a nonspecificscRNA (100 pmol/ml) using Lipofectamine 2000 according to themanufacturer's instructions. On day 3 after transfection, thecells were incubated with oltipraz for 18 h. The whole lysateswere used for the luciferase activity assay. Immunoblot analysisconfirmed RSK1 knockdown 3 days after transfection.

Stable Transfection. For the preparation of PI3-kinase p85 [p85(+)]or MKK1 dominant-negative mutant [MKK1(-)] cells, H4IIE cellswere transfected with the respective plasmid and incubated for48 h, as described previously (Cho and Kim, 2003b; Kang et al.,2003). Geneticin was added to select the resistant colonies.

RSK1 Kinase Assay. Cells that had been incubated in the mediumwithout serum for 24 h were treated with vehicle or oltipraz(30 µM) for the indicated time period, harvested, andlysed in the buffer containing 25 mM Tris-HCl, pH 7.4, 2 mMdithiothreitol, 10 mM MgCl₂, 5 mM $beta$ -glycerophosphate, 1 mM Na₃VO₄,and 1 mM phenylmethylsulfonyl fluoride. RSK1 in cell lysates(300 µg) was immunoprecipitated with anti-RSK1 antibody.Immunoprecipitates were washed three times in lysis buffer,and once in kinase buffer containing Tris-HCl (25 mM, pH 7.4),10 mM MgCl₂, 25 mM $beta$ -glycerophosphate, 1 mM Na₃VO₄, 2 mM dithiothreitol,1 mM phenylmethylsulfonyl fluoride, 1 µg/ml leupeptin,and 200 µM ATP. Kinase reaction was initiated by addingS6 rsk substrate peptide (5 µg per assay) and 2 µCiof [ ${gamma}$ -³²P]ATP to a 20-µl reaction mixture, and continuedfor 30 min at 30°C. After brief centrifugation, the supernatantof reaction mixture was spotted onto p81 phosphocellulose paper(Upstate Biotechnology). The paper was washed with 0.8% phosphoricacid for 5 min three times and subsequently with 90% ethanolfor 5 min. The membrane was dried and transferred to 5 ml ofscintillation cocktail, and the radioactivity of phosphorylatedsubstrate was measured using a $beta$ -counter (PerkinElmer Wallac,Gaithersburg, MD).

Statistical Analysis. Scanning densitometry of the immunoblotswas performed with Image Scan and Analysis System (Alpha Innotech,San Leandro, CA). The area of each lane was integrated usingthe software AlphaEase, version 5.5, followed by backgroundsubtraction. One-way analysis of variance was used to assessstatistical significance of differences among treatment groups.For each statistically significant effect of treatment, theNewman-Keuls test was used for comparisons between multiplegroup means. The data were expressed as means ± S.E.The criterion for statistical significance was set at p <0.05 or < 0.01.

Results

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Abstract
Materials and Methods
Results
Discussion
References

Induction of C/EBP $beta$ by Oltipraz. Our previous study showed thatoltipraz induces nuclear translocation of C/EBP $beta$ and promotesC/EBP $beta$ binding to the C/EBP binding site (Kang et al., 2003).In view of the importance of C/EBPs as transcriptional factors,we sought to determine the expression of major forms of C/EBPin H4IIE cells treated with oltipraz. Immunoblot analysis revealedthat the levels of C/EBP $beta$ were increased 12 to 48 h after oltipraztreatment compared with untreated control (Fig. 1), whereasthose of C/EBP ${alpha}$ and ${delta}$ forms were unaffected. Thus, activationof C/EBP $beta$ by oltipraz involves the induction of C/EBP $beta$ .

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Fig. 1. Expression of C/EBP isoforms in cells treated with oltipraz. The levels of C/EBP $beta$ , C/EBP ${alpha}$ , and C/EBP ${delta}$ isoforms were determined in the lysates of cells treated with oltipraz for 3 to 48 h. Each lane was loaded with 20 µg of cell lysates. Actin was used as a control. Results were confirmed by repeated experiments.

Alignment of RSK1- or ERK-Phosphorylated Residues in Rat, Mouse,and Human C/EBP $beta$ . Activation of C/EBP $beta$ for gene transcriptioninvolves phosphorylation of specific residues in its activationdomain. In Fig. 2A, parts of the sequences of rat, mouse, andhuman homologous forms of C/EBP $beta$ were aligned, and specific phosphorylationresidues with numbers were indicated. RSK1 induces phosphorylationof Ser¹⁰⁵ in rat C/EBP $beta$ (Buck et al., 1999

). Because Ser¹⁰⁵ inrat C/EBP $beta$ is replaced with alanine in the mouse and human homologousforms, phosphorylation residues activated by RSK1 should differin these species. Thr²¹⁷ is the RSK1-induced phosphorylationresidue in mouse C/EBP $beta$ (Buck et al., 1999

), which is functionallyanalogous to Ser¹⁰⁵ in rat C/EBP $beta$ (Fig. 2B). Thr²⁶⁶ in humanform of C/EBP $beta$ is equivalent to Thr²¹⁷ in the mouse form. ActivatedERK directly phosphorylates other residues, namely Thr¹⁸⁹, Thr¹⁸⁸,and Thr²³⁵ in rat, mouse, and human forms of C/EBP $beta$ , respectively(Fig. 2B) (Nakajima et al., 1993

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Fig. 2. Alignment of RSK1- or ERK-phosphorylated residues in rat, mouse, and human homologous forms of C/EBP $beta$ . A, alignment of the partial sequences of rat, mouse, and human C/EBP $beta$ . The residues that are equivalent to Ser¹⁰⁵, Thr¹⁸⁹, and Ala²¹⁸ in rat C/EBP $beta$ are highlighted for comparison. B, the specific residues that are phosphorylated by RSK1 or ERK. The residues in rat, mouse, and human homologous forms of C/EBP $beta$ phosphorylated by RSK1 or ERK were indicated.

Ser¹⁰⁵ Phosphorylation of C/EBP $beta$ by Oltipraz. Immunoblot experimentswere conducted with cell lysates to determine whether the levelsof rat C/EBP $beta$ (38 and 35 kDa) phosphorylated at the residue ofSer¹⁰⁵ or Thr¹⁸⁹ were increased. Oltipraz only minimally increasedSer¹⁰⁵ phosphorylation of 38-kDa C/EBP $beta$ in lysates. Hence, insubsequent studies, we focused on the phosphorylation of the35-kDa form. The levels of Ser¹⁰⁵-phosphorylated 35-kDa C/EBP $beta$ were enhanced 6 to 24 h after treatment of cells with oltipraz,whereas those of Thr¹⁸⁹-phosphorylated C/EBP $beta$ were unchanged(Fig. 3A). The results provided evidence that 35-kDa C/EBP $beta$ wasphosphorylated at Ser¹⁰⁵, but not Thr¹⁸⁹, by oltipraz treatmentin H4IIE cells. Next, the localization of C/EBP $beta$ was determinedby subcellular fractionations and immunoblot analyses. PhosphorylatedC/EBP $beta$ at Ser¹⁰⁵ was located predominantly in the cytoplasm ofH4IIE cells treated with oltipraz for 6 h (Fig. 3A, middle).However, when cells were treated with oltipraz for 12 h, Ser¹⁰⁵-phosphorylatedC/EBP $beta$ showed nuclear localization to a greater extent. At 24h of oltipraz treatment, Ser¹⁰⁵-phosphorylated C/EBP $beta$ was foundin both the cytoplasm and the nucleus (Fig. 3A, middle and right).The levels of Thr¹⁸⁹-phosphorylated C/EBP $beta$ in nuclear or cytoplasmicfractions were unchanged after oltipraz treatment.

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Fig. 3. Oltipraz activation of C/EBP $beta$ by Ser¹⁰⁵ phosphorylation. A, immunoblot analysis of phosphorylated C/EBP $beta$ . The levels of C/EBP $beta$ phosphorylated at Ser¹⁰⁵ or Thr¹⁸⁹ were determined by immunoblot analyses in lysates prepared from H4IIE cells treated with oltipraz for 3 to 48 h (left). The levels of phosphorylated C/EBP $beta$ were also determined in the cytosolic and nuclear fractions of oltipraz-treated cells (3-24 h) (middle and right). Equal loading of proteins was verified by probing the replicate blots for actin. Each lane contained 20 µg of lysate (or cytosolic) proteins or 10 µg of nuclear proteins. B, gel shift analysis of Ser¹⁰⁵-phosphorylated C/EBP $beta$ binding to the C/EBP binding site. Nuclear extracts were prepared from H4IIE cells cultured with 30 µM oltipraz for 12 h. All lanes contained 10 µg of nuclear extracts and 5 ng of labeled C/EBP consensus oligonucleotide. Immunoinhibition assays were carried out by incubating the nuclear extracts (oltipraz, 12 h) with the polyclonal antibody directed against Ser¹⁰⁵- or Thr¹⁸⁹-phosphorylated C/EBP $beta$ or Sp1. Arrowheads indicate shifted DNA bound with Ser¹⁰⁵-phosphorylated C/EBP $beta$ . Results were confirmed by repeated experiments.

Next, we confirmed the formation of C/EBP $beta$ -DNA binding complexesafter oltipraz treatment (Fig. 3B). To determine whether theincrease in the band intensity by oltipraz obtained in gel shiftassays occurred as a result of phosphorylation of C/EBP $beta$ at Ser¹⁰⁵,an immunoinhibition experiment was performed with the antibodydirected against Ser¹⁰⁵- or Thr¹⁸⁹-phosphorylated C/EBP $beta$ . Thepresence of anti-Ser¹⁰⁵-phosphorylated C/EBP $beta$ antibody completelyabolished the band intensity of the C/EBP $beta$ -DNA binding complex,whereas either anti-Thr¹⁸⁹-phosphorylated C/EBP $beta$ or anti-Sp1antibody failed to do so (Fig. 3B). The antibody competitionassays verified that oltipraz-induced C/EBP $beta$ -DNA binding activityis specifically dependent on Ser¹⁰⁵-phosphorylated C/EBP $beta$ . Thesedata provided evidence that oltipraz treatment led to an increasein C/EBP $beta$ phosphorylation at Ser¹⁰⁵, but not Thr¹⁸⁹, in H4IIEcells and that Ser¹⁰⁵-phosphorylated C/EBP $beta$ served as an activeform in the formation of C/EBP $beta$ -DNA binding complex.

Association of Ser¹⁰⁵-Phosphorylated C/EBP $beta$ with CBP. To investigatewhether an increase in Ser¹⁰⁵ phosphorylation of C/EBP $beta$ enhancedrecruitment of CBP coactivator for gene transactivation, H4IIEcells were serum-starved for 24 h and then treated with oltiprazfor the indicated time periods. Nuclear extracts prepared fromuntreated cells or cells treated with oltipraz were immunoprecipitatedwith anti-CBP antibody and then immunoblotted with anti-Ser¹⁰⁵-phosphorylatedC/EBP $beta$ antibody. Formation of CBP-Ser¹⁰⁵-phosphorylated C/EBP $beta$ complex was increased after stimulation of cells with oltiprazfor 12 to 24 h (Fig. 4A), during which time period the levelof Ser¹⁰⁵-phosphorylated C/EBP $beta$ in the nuclear fraction maximallyincreased (Fig. 4A, right). In contrast, Thr¹⁸⁹-phosphorylatedC/EBP $beta$ , immunoprecipitated with CBP, was unchanged. These dataprovide evidence that oltipraz treatment enhances the levelof Ser¹⁰⁵-phosphorylated C/EBP $beta$ that is capable of interactingwith CBP coactivator.

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Fig. 4. Recruitment of CBP to Ser¹⁰⁵-phosphorylated C/EBP $beta$ . A, association of CBP with Ser¹⁰⁵-phosphorylated C/EBP $beta$ . Interaction of CBP with Ser¹⁰⁵- or Thr¹⁸⁹-phosphorylated C/EBP $beta$ was determined in H4IIE cells treated with 30 µM oltipraz for 3 to 24 h. Whole-cell lysates were precipitated with anti-CBP antibody and immunocomplexes were immunoblotted with anti-Ser¹⁰⁵-phosphorylated or anti-Thr¹⁸⁹-phosphorylated C/EBP $beta$ antibody. Aliquots from the input were loaded for immunoblot of actin. Results were confirmed by repeated experiments. B, ChIP assays. The DNA-protein complexes prepared from cells treated with vehicle or oltipraz (30 µM, 12 h) were immunoprecipitated with anti-Ser¹⁰⁵-phosphorylated C/EBP $beta$ , anti-CBP, anti-acetylated histone, or anti-Thr¹⁸⁹-phosphorylated C/EBP $beta$ antibody. The samples were PCR-amplified using primers flanking the proximal and distal regions of the DNA comprising the C/EBP binding site in the GSTA2 promoter. A set of control experiment was carried out for the $beta$ -actin gene. One tenth of the total input was used as a loading control. Results were confirmed by repeated experiments. C, specific mutagenesis assay. The effect of specific mutation of Ser¹⁰⁵ residue in C/EBP $beta$ on oltipraz-inducible luciferase expression from pGL-1651 GSTA2 promoter was assessed in H4IIE cells. Luciferase activities were measured in cells treated with vehicle or oltipraz (30 µM, 18 h) or in cells transfected with the plasmid encoding Myc-C/EBP $beta$ . Data represented the mean ± S.E. with four separate experiments (significant compared with vehicle; ^*, p < 0.05). In another set of experiment, oltipraz-inducible change in luciferase expression was determined in cells transfected with the plasmid encoding Myc-C/EBP $beta$ or Myc-C/EBP $beta$ -S105A. Values were expressed as the changes relative to the respective vehicle-treated control and represented the mean ± S.E. with four to five separate experiments (significant compared with Myc-C/EBP $beta$ ; #, p < 0.05). Immunoblot analysis confirmed the expression of Myc-C/EBP $beta$ or Myc-C/EBP $beta$ -S105A.

Next, to determine the association of Ser¹⁰⁵-phosphorylatedC/EBP $beta$ with CBP on the target gene promoter, we performed ChIPanalysis. The DNA-protein complexes were immunoprecipitatedwith anti-Ser¹⁰⁵-phosphorylated C/EBP $beta$ , anti-CBP, or anti-acetylatedhistone antibody, followed by reversal of cross-linking andPCR amplification using primers flanking the proximal and distalregions of the DNA comprising the C/EBP binding site in theGSTA2 gene promoter (Fig. 4B). In the cells treated with oltipraz(12 h), the intensities of the three PCR products were all distinctlyhigher compared with vehicle-treated control. The intensitiesof the PCR products using primers flanking the proximal anddistal regions of the $beta$ -actin gene promoter (a housekeeping gene)were unaffected by oltipraz. In the sample immunoprecipitatedwith anti-acetylated histone antibody, the intensity of thePCR product from the $beta$ -actin gene was intense in control cellsbut was not further increased after oltipraz treatment (Fig. 4B).In contrast to the result obtained with Ser¹⁰⁵-phosphorylatedC/EBP $beta$ immunoprecipitate, the band intensity in Thr¹⁸⁹-phosphorylatedC/EBP $beta$ immunoprecipitate was not enhanced by oltipraz.

Next, we assessed the functional role of Ser¹⁰⁵ phosphorylationof C/EBP $beta$ by oltipraz in target gene transactivation by the specificmutagenesis assay. Oltipraz treatment was capable of increasingluciferase expression from the pGL-1651 GSTA2 promoter thatcontains the C/EBP binding site (Fig. 4C, left). Likewise, theexpression of Myc-C/EBP $beta$ promoted the gene transcription. Exposureof cells transfected with the myc-C/EBP $beta$ plasmid to oltiprazfor 18 h resulted in a greater increase in luciferase expression(i.e., $~$ 1.6-fold increase relative to C/EBP $beta$ alone) (Fig. 4C,right). The expression of Myc-Ala¹⁰⁵ mutant of C/EBP $beta$ , comparedwith that of Myc-C/EBP $beta$ , completely abolished the ability ofoltipraz to promote luciferase expression from pGL-1651 (Fig. 4C,right). These results indicate that Ser¹⁰⁵ phosphorylationof C/EBP $beta$ , which is promoted by oltipraz treatment, leads torecruitment of CBP to the GSTA2 gene promoter and enhances histoneacetylation for the gene transcription.

Ser¹⁰⁵ Phosphorylation of C/EBP $beta$ by RSK1. In view of the roleof RSK1 in the phosphorylation of C/EBP $beta$ , we sought to determinewhether RSK1 is responsible for Ser¹⁰⁵ phosphorylation of C/EBP $beta$ .Transfection with the KH3 plasmid, a control vector, allowedcells to phosphorylate C/EBP $beta$ at Ser¹⁰⁵ in response to oltipraz(30 µM, 12 h). In contrast, expression of HA-CTT-RSK1or constitutively inactive kinase-dead mutant of RSK1 (HA-K112/464R-RSK1)completely inhibited oltipraz enhancement in Ser¹⁰⁵ phosphorylationof C/EBP $beta$ , as determined by immunoblot analyses in lysates (Fig. 5A).In contrast, Thr¹⁸⁹ phosphorylation was unchanged by theplasmids. In parallel with this, the increase in the level ofnuclear Ser¹⁰⁵-phosphorylated C/EBP $beta$ was prevented by overexpressionof HA-CTT-RSK1 or HA-K112/464R-RSK1 (Fig. 5A).

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Fig. 5. The role of RSK1 in Ser¹⁰⁵ phosphorylation of C/EBP $beta$ and gene transactivation by oltipraz. A, the levels of Ser¹⁰⁵-phosphorylated C/EBP $beta$ . The levels of C/EBP $beta$ phosphorylated at Ser¹⁰⁵ or Thr¹⁸⁹ were determined by immunoblot analyses in lysates or nuclear fractions prepared from H4IIE cells that had been treated with oltipraz (12 h) after transfection with the HA-tagged plasmid encoding a truncated RSK1 (CTT-RSK1) or a kinase-dead mutant form of RSK1 (K112/464R-RSK1). Each lane was loaded with 20 µg of lysates or 10 µg of nuclear proteins. Expression of HA-CTT-RSK1 or HA-K112/464R-RSK1 was verified by immunoblotting for HA. Equal loading of proteins in each lane was verified by probing the replicate blot for actin. B, repression of C/EBP $beta$ -mediated promoter luciferase activity by dominant-negative mutants of RSK1. Cells were cotransfected with the pGL-1651 and CMV- $beta$ -galactosidase plasmids (33:1) in combination with KH3 (empty vector), HA-CTT-RSK1 or HA-K112/464R-RSK1 plasmid at a ratio of 1:1 and the cells were exposed to oltipraz for 18 h. Activation of the reporter gene was calculated as a relative change to $beta$ -galactosidase activity. The value for luciferase activity was expressed as relative luciferase unit of cell lysates and represented the mean ± S.E. with four separate experiments (significant compared with KH3 in untreated cells; ^*, p < 0.05, KH3 in untreated cells = 100%).

Thereafter, we determined the effects of dominant-negative mutantsof RSK1 on oltipraz-inducible expression of the pGL-1651 luciferasereporter gene (Kang et al., 2003). As expected, transfectionof cells with HA-CTT-RSK1 or HA-K112/464R-RSK1 entirely inhibitedthe ability of oltipraz to stimulate reporter gene expressionfrom pGL-1651 (Fig. 5B). KH3, which was used as a control, didnot inhibit the reporter gene expression. This finding indicatesthat RSK1 mediates Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by oltiprazfor GSTA2 gene transactivation.

RSK1-Dependent Phosphorylation of C/EBP $beta$ in Other Species. Wethen determined whether oltipraz induced phosphorylation ofthe residue in mouse or human C/EBP $beta$ functionally analogous toSer¹⁰⁵ of rat C/EBP $beta$ . Immunoblot analysis revealed that phosphorylationof C/EBP $beta$ at Thr²¹⁷ or Thr²⁶⁶ was promoted by oltipraz (30 µM,12 h) in mouse Hepa1c1c cells and human HepG2 cells, respectively(Fig. 6A). Increases in C/EBP $beta$ phosphorylation at the Thr^217/266residues by oltipraz were abolished by transfection with theplasmid encoding HA-K112/464R-RSK1. Hence, RSK1 contributesto Thr^217/266 phosphorylation by oltipraz in mouse and humanC/EBP $beta$ . In addition, we verified the role of RSK1 in Ser¹⁰⁵ phosphorylationof C/EBP $beta$ by oltipraz in primary cultured rat hepatocytes. Oltipraz(30 µM, 12 h) was capable of inducing C/EBP $beta$ phosphorylationat Ser¹⁰⁵ in the primary hepatocytes (Fig. 6B). As expected,a dominant-negative mutant of RSK1 prevented oltipraz-induciblephosphorylation of C/EBP $beta$ .

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Fig. 6. The functional role of RSK1 in C/EBP $beta$ phosphorylation in mouse, human cell lines, or primary hepatocytes. A, RSK1-mediated Thr^217/266 phosphorylation by oltipraz in mouse and human C/EBP $beta$ . The levels of Thr²¹⁷- or Thr²⁶⁶-phosphorylated C/EBP $beta$ were assessed by immunoblot analyses in lysates prepared from mouse Hepa1c1c or human HepG2 cells that had been treated with oltipraz (30 µM, 12 h) after transfection with the plasmid encoding HA-K112/464R-RSK1. B, the role of RSK1 in Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by oltipraz in primary cultured rat hepatocytes. Rat hepatocytes were incubated in the medium containing 10% FCS for 24 h, transiently transfected with the plasmid encoding HA-K112/464R-RSK1 using Lipofectamine 2000, and then treated with oltipraz for 12 h, as described under Materials and Methods. Control cells were transfected with KH3 and empty plasmid. Equal loading of proteins in each lane was verified by probing the replicate blot for actin. Expression of HA-K112/464R-RSK1 was verified by immunoblotting for HA. Results were confirmed by separate experiments. C, the effect of RSK1 knockdown on the C/EBP $beta$ -mediated gene transactivation by oltipraz. HepG2 cells were transfected with RSK1 siRNA or scRNA in combination with pGL-1651, incubated for 3 days, and then treated with vehicle or 10 µM oltipraz for 18 h. The luciferase expression from pGL-1651 was analyzed in cell lysates. Aliquots of the samples were subjected to immunoblot analyses. Values were expressed as the changes relative to the respective vehicle-treated control and represented the mean ± S.E. with three separate experiments (significant compared with scRNA transfection: ^**, p < 0.01).

In addition, we used the knockdown technique to verify the functionalrole of RSK1 in the GSTA2 gene transactivation by oltipraz.Knockdown of RSK1 by transfection of HepG2 cells with the siRNAthat specifically catalyzes degradation of human RSK1 mRNA resultedin a substantial decrease in the luciferase expression frompGL-1651 (Fig. 6C, left). In this experiment, scrambled RNA(scRNA) was used as a nonspecific RNA. Immunoblot analysis confirmeda decrease in RSK1 expression by the siRNA (Fig. 6C, right).The human RSK1 siRNA failed to degrade rat RSK1 (SupplementalData S1), which confirmed its specificity.

Effects of MKK1 Inhibition on Oltipraz Activation of C/EBP $beta$ andGene Expression. Activation of ERK initiates an activating processof RSK1 by epidermal growth factor (Roux et al., 2003). To studywhether the MKK1/ERK pathway was involved in the increase inSer¹⁰⁵ phosphorylation of C/EBP $beta$ by oltipraz, we assessed theeffect of U0126, an MKK1 inhibitor, on the phosphorylation inlysates. U0126 weakly but insignificantly prevented an increasein Ser¹⁰⁵ phosphorylation of C/EBP $beta$ in the lysates prepared fromH4IIE cells treated with oltipraz for 12 h (Fig. 7A, left).We also monitored the levels of Ser¹⁰⁵-phosphorylated C/EBP $beta$ in H4IIE cells or cells stably transfected with dominant-negativemutant of MKK1 [MKK1(-)] (Fig. 7A, right). Increase in nuclearSer¹⁰⁵-phosphorylated C/EBP $beta$ by oltipraz was marginally repressedby MKK1(-) transfection. U0126 treatment or MKK1(-) transfectioncompletely inhibited the activation of ERK1/2 by insulin-likegrowth factor (100 ng/ml, 10 min). Therefore, it is unlikelythat an increase in Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by oltiprazis under the control of ERK1/2.

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Fig. 7. The role of ERK in C/EBP $beta$ activation by oltipraz. A, the effects of MKK1 inhibition on Ser¹⁰⁵ phosphorylation of C/EBP $beta$ in cell lysates. The effect of ERK in Ser¹⁰⁵ phosphorylation of C/EBP $beta$ was assessed by using U0126 or MKK1(-) stable transfection. H4IIE cells that had been treated with U0126 (10 µM, 1 h) were further incubated with oltipraz (30 µM, 12 h) in the continuing presence of U0126. Cells were stably transfected with the plasmid encoding MKK1(-). Inhibition of ERK activation by U0126 treatment or MKK1(-) transfection was confirmed by immunoblotting phosphorylated ERK1/2 and total ERK1/2 (p-ERK and ERK, respectively) in cells exposed to insulin-like growth factor (IGF, 100 ng/ml, 10 min). B, the role of ERK in nuclear translocation of Ser¹⁰⁵-phosphorylated C/EBP $beta$ . Immunoblot analyses were performed with the nuclear fractions prepared from cells treated as described in A. Data represent the mean ± S.E. with four separate experiments (significant compared with control: ^*, p < 0.05; ^**, p < 0.01) (N.S., not significant). C, the effect of MKK1(-) transfection on oltipraz-inducible luciferase-reporter activity. Luciferase activity was measured in lysates of H4IIE cells treated with vehicle or oltipraz (18 h) after transfection with PCMV (empty vector) or MKK1(-). Cells were transfected with pGL-1651-luciferase reporter plasmid, as described in Fig. 3C. Data represented the mean ± S.E. with four separate experiments (significant compared with control: ^*, p < 0.05).

We also monitored the levels of Ser¹⁰⁵-phosphorylated C/EBP $beta$ in nuclear fractions prepared from cells treated with U0126or MKK1(-) cells to determine whether the activity of ERK wasrequired for nuclear translocation of Ser¹⁰⁵-phosphorylatedC/EBP $beta$ . Immunoblot analyses demonstrated that either U0126 treatmentor MKK1(-) transfection only weakly blocked an increase in nuclearSer¹⁰⁵-phosphorylated C/EBP $beta$ by oltipraz (Fig. 7B). The extentof increase in nuclear Ser¹⁰⁵-phosphorylated C/EBP $beta$ by oltiprazwas comparable with that in lysates, indicating that the activityof ERK1/2 was unnecessary for nuclear translocation of the phosphorylatedC/EBP $beta$ by oltipraz. In addition, MKK1(-) transfection failedto prevent enhancement in pGL-1651 luciferase expression byoltipraz (Fig. 7C). These results show that Ser¹⁰⁵ phosphorylationof C/EBP $beta$ and target gene transactivation by oltipraz do notrequire MKK1-ERK-mediated activation process.

PI3-Kinase-Dependent Ser¹⁰⁵ Phosphorylation. The pathway ofPI3-kinase is involved in a number of cellular responses bygrowth stimuli (Katso et al., 2001). We reported previouslythat C/EBP $beta$ activation is dependent on the activity of PI3-kinase(Kang et al., 2003). To determine whether Ser¹⁰⁵ phosphorylationof C/EBP $beta$ by oltipraz was controlled by PI3-kinase, we measuredthe levels of Ser¹⁰⁵-phosphorylated C/EBP $beta$ in lysates or nuclearfractions. H4IIE cells were incubated with LY294002 (10 µM),a chemical inhibitor of PI3-kinase, for 1 h and then exposedto oltipraz (30 µM). Immunoblot analysis revealed thatLY294002 blocked oltipraz-inducible phosphorylation of C/EBP $beta$ at Ser¹⁰⁵ in lysates (Fig. 8A). In addition, increase in thelevel of nuclear Ser¹⁰⁵-phosphorylated C/EBP $beta$ was almost completelyabolished by treatment with LY294002 or stable transfectionwith the p85(+) subunit of PI3-kinase (Fig. 8B). Additionalimmunoblot assays showed that the levels of total C/EBP $beta$ wereunchanged by LY294002 treatment (data not shown), indicatingthat prevention of oltipraz-inducible Ser¹⁰⁵ phosphorylationof C/EBP $beta$ by PI3-kinase inhibition was not caused by a decreasein C/EBP $beta$ expression. Our results showed that PI3-kinase regulatedSer¹⁰⁵ phosphorylation of C/EBP $beta$ .

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Fig. 8. PI3-kinase-dependent Ser¹⁰⁵-phosphorylation of C/EBP $beta$ by oltipraz. A, the levels of Ser¹⁰⁵-phosphorylated C/EBP $beta$ in cell lysates. H4IIE cells that had been serum-starved for 24 h were pretreated with LY294002 (10 µM) for 1 h and further incubated with 30 µM oltipraz for 12 h in the continuing presence of LY294002. Ser¹⁰⁵-phosphorylated C/EBP $beta$ was assessed by immunoblot analysis in cell lysates. Equal loading of proteins was verified by probing the replicate blots for actin. B, the levels of nuclear Ser¹⁰⁵-phosphorylated C/EBP $beta$ . Nuclear proteins obtained from cells treated with oltipraz (30 µM, 12 h) in the presence or absence of 10 µM LY294002 were subjected to immunoblot analysis. Cells stably expressing the p85 subunit of PI3-kinase were used to assess the role of PI3-kinase in Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by oltipraz. The relative levels of Ser¹⁰⁵-phosphorylated C/EBP $beta$ were assessed by scanning densitometry of the immunoblots. Data represent the mean ± S.E. with three separate experiments (significant compared with control: ^**, p < 0.01; significant compared with oltipraz alone: ##, p < 0.01; control level = 1); p85(+), overexpression of p85 subunit.

Role of PI3-Kinase in the Activation of RSK1 by Oltipraz. Wefinally determined the kinase activity of RSK1 in cells exposedto oltipraz for a variety of time periods. Treatment of H4IIEcells with oltipraz resulted in rapid increases in the catalyticactivity of RSK1 toward S6 rsk substrate peptide (Fig. 9A).RSK1 activity in lyates maximally increased 1 h after treatment,which gradually decreased from the maximum at later times. Increasein RSK activity was observed at least up to 24 h. In view ofthe fact that Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by oltipraz dependedon the pathway involving PI3-kinase, we were interested in whetherRSK1 activation by oltipraz was under the control of PI3-kinase.We observed that LY294002 treatment for 1 h before the additionof oltipraz abrogated an increase in the kinase activity ofRSK1 by oltipraz (Fig. 9B). Nuclear translocation of RSK1 stimulatedby oltipraz treatment (12 h) was consistently prevented by concomitanttreatment of cells with LY294002 (Fig. 9C). The role of PI3-kinasefor RSK1 activation was confirmed in cells stably transfectedwith the plasmid encoding p110 or p85 subunit of PI3-kinase(Supplemental Data S2). These results provide evidence thatincrease in RSK1 kinase activity by oltipraz requires the basalPI3-kinase activity. Wortmannin was not used as an inhibitorin this experiment because the agent at the concentration effectivefor PI3-kinase inhibition elicited nuclear translocation ofRSK1 (Supplemental Data S3).

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Fig. 9. PI3-kinase-dependent RSK1 activation by oltipraz. A, increase in the kinase activity of RSK1 by oltipraz. H4IIE cells were incubated with 30 µM oltipraz for the indicated time periods. RSK1 activity toward S6 rsk substrate peptide was determined in cell lyates by monitoring ³²P radioactivity. Data represent the mean ± S.E. with three separate experiments (significant compared with control: ^*, p < 0.05; ^**, p < 0.01; zero time control = 1). B, the effect of PI3-kinase inhibition on the kinase activity of RSK1. H4IIE cells were treated with vehicle or oltipraz in the presence or absence of LY294002 (10 µM) for 1 h. The kinase activity was measured as described above. Values are expressed as the change in RSK1 activity relative to vehicle-treated control and represented the mean ± S.E. with four separate experiments (significant compared with control: ^*, p < 0.05; significant compared with oltipraz treatment: #, p < 0.05). C, the effect of PI3-kinase inhibition on the nuclear translocation of RSK1 induced by oltipraz. Immunoblot analysis was performed in the nuclear fractions prepared from cells treated with oltipraz in the presence or absence of LY294002 (10 µM) for 12 h. Equal loading of proteins was verified by probing the replicate blot for actin. Each lane contained 10 µg of proteins. Results were confirmed by three separate experiments and a representative blot is shown.

	Discussion

Top Abstract Materials and Methods Results Discussion References

Activation of C/EBP $beta$ , which involves the process of nuclear translocationand C/EBP $beta$ binding to the C/EBP binding site, requires phosphorylationsat specific residues by cellular kinases (Frodin and Gammeltoft,1999

). In the present study, we found that activation of C/EBP $beta$ by oltipraz involved specific Ser¹⁰⁵ phosphorylation in therat form and Thr^217/266 phosphorylations in the mouse and humanforms. Oltipraz did not enhance Thr¹⁸⁹ phosphorylation of C/EBP $beta$ ,which is known to be catalyzed by Ras-MAPK or Cdk (Nakajimaet al., 1993

; Shuman et al., 2004

). Lack of an increase in theThr¹⁸⁹ phosphorylation may explain no mitogenic effect of oltipraz(Ruggeri et al., 2002

) because Thr¹⁸⁹-phosphorylated C/EBP $beta$ hasbeen implicated in the cell-cycle progression (Shuman et al.,2004

). The level of Ser¹⁰⁵-phosphorylated C/EBP $beta$ in nuclear fractionincreased with a reciprocal decrease in its cytoplasmic content.At 6 h after oltipraz treatment, we observed a notable increasein Ser¹⁰⁵ phosphorylation of C/EBP $beta$ in the cytoplasm. In fact,the level of cytoplasmic Ser¹⁰⁵-phosphorylated C/EBP $beta$ at theearly time increased to a greater extent than that in the nucleus,whereas the nuclear form gradually increased at later timesafter oltipraz treatment. The early increase in cytoplasmicSer¹⁰⁵ phosphorylation suggested that the phosphorylation maybe mediated by the cytoplasmic enzyme activated by oltipraz.Therefore, oltipraz-inducible Ser¹⁰⁵ phosphorylation of C/EBP $beta$ is likely to occur initially in the cytoplasm, and then thephosphorylated form translocates into the nucleus. On the otherhand, the enzyme that activates C/EBP $beta$ may translocate into thenucleus with C/EBP $beta$ for phosphorylation.

The immunoprecipitation and ChIP assays demonstrated that Ser¹⁰⁵-phosphorylatedC/EBP $beta$ was functionally active in gene transcription. N-terminaltransactivation domain of C/EBP $beta$ may interact with CBP/p300 coactivator,which is critical for C/EBP $beta$ -mediated gene transactivation (Minket al., 1997). In the present study, we revealed that oltipraztreatment increased the level of Ser¹⁰⁵-phosphorylated C/EBP $beta$ that is capable of binding to CBP, inducing histone acetylationfor the GSTA2 gene transactivation. The C/EBP $beta$ gene containsthe C/EBP $beta$ binding site(s) in the promoter region (GenBank accessionnumber 178567) (Mink et al., 1999). The role of Ser¹⁰⁵-phosphorylatedC/EBP $beta$ in gene transactivation was additionally supported bythe finding that oltipraz specifically increased the expressionof C/EBP $beta$ but not C/EBP ${alpha}$ or C/EBP ${delta}$ . Thus, it is highly likely thatoltipraz induction of C/EBP $beta$ after initial activation of pre-existingC/EBP $beta$ by Ser¹⁰⁵ phosphorylation contributes to persistent genetransactivation. Although Thr¹⁸⁹ phosphorylation of rat C/EBP $beta$ was unchanged after oltipraz treatment, we observed that Thr¹⁸⁹-phosphorylatedC/EBP $beta$ constitutively interacted with CBP and bound to the promoterregion of the GSTA2 gene (Fig. 3). Hence, the Thr¹⁸⁹ phosphorylationmight be responsible for the constitutive gene expression. Activationof C/EBP $beta$ may be mediated by multiple phosphorylations at theserine or threonine residues within the molecule (Buck and Chojkier,2003). In the present study, the specific mutagenesis analysisof C/EBP $beta$ lends support to the essential role of Ser¹⁰⁵ phosphorylationfor oltipraz's inducible gene transcription, as evidenced bythe complete abrogation of oltipraz's increase in C/EBP $beta$ -mediatedgene expression in cells transfected with Myc-C/EBP $beta$ -S105A. Ourresults provide compelling evidence that Ser¹⁰⁵ plays a criticalrole in C/EBP $beta$ activation by oltipraz.

Rat C/EBP $beta$ is known to be phosphorylated at the residue of Ser¹⁰⁵by RSK1 (Buck et al., 1999). In cells transfected with the plasmidencoding truncated or kinase-dead mutant form of RSK1, oltiprazfailed to induce Ser¹⁰⁵ phosphorylation of C/EBP $beta$ or GSTA2 genetransactivation. Thus, Ser¹⁰⁵ phosphorylation of 35-kDa C/EBP $beta$ seemed to be mediated by RSK1. C/EBP $beta$ is phosphorylated by othercellular kinases including PKC, protein kinase A, and Ras-MAPK(Nakajima et al., 1993; Trautwein et al., 1993, 1994; Buck etal., 1999; Hanlon et al., 2001). PKC may phosphorylate rat C/EBP $beta$ at the residue of Ser¹⁰⁵, whereas MAPK downstream from Ras phosphorylatesThr²³⁵ of human C/EBP $beta$ (analogous to Thr¹⁸⁹ in the rat form).GF109203 (PKC inhibitor) did not inhibit the Ser¹⁰⁵ phosphorylationof C/EBP $beta$ by oltipraz (Supplemental Data S3). Oltipraz's increasein Ser¹⁰⁵-phosphorylated C/EBP $beta$ was also unaffected by pretreatmentwith rapamycin (inhibitor of p70 ribosomal S6-kinase, 100 µM)or H89 (protein kinase A inhibitor, 20 µM) (data not shown)but weakly inhibited by Akt inhibitor IV (Supplemental DataS3). Thus, the possibility that Akt affects C/EBP $beta$ phosphorylationwas not completely excluded, although oltipraz failed to stimulateAkt (Kang et al., 2003).

We showed that RSK1 regulated Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by oltipraz in primary rat hepatocytes as well as H4IIE cells.In addition, oltipraz enhanced phosphorylation of the mouseor human C/EBP $beta$ at the residue of Thr²¹⁷ or Thr²⁶⁶, which wasalso catalyzed by RSK1. The role of human RSK1 in C/EBP $beta$ -mediatedgene activation was additionally supported by the RSK1 knockdownexperiment. Our results provide evidence that activation ofthe C/EBP $beta$ forms by oltipraz involves functionally analogousphosphorylation at the specific residues by RSK1 in the species.Oltipraz activation of C/EBP $beta$ by specific phosphorylation wouldresult in a conformational change of the protein for DNA bindingand gene transactivation. The finding that oltipraz activatesC/EBP $beta$ via RSK1 brings insights into the role of organic compoundsin activating the critical signaling pathway and cellular functions.

We showed previously that the pathways of MAPKs, ERK1/2, p38kinase, and c-Jun N-terminal kinase, were not responsible forC/EBP $beta$ -mediated glutathione S-transferase induction by oltipraz(Kang et al., 2003). In the current study, the extent of increasein Ser¹⁰⁵ phosphorylation of C/EBP $beta$ or C/EBP $beta$ -mediated gene transactivationby oltipraz in MKK1(-) cells was almost comparable with thatin control, suggesting that oltipraz was capable of stimulatingthe Ser¹⁰⁵ phosphorylation independent of MKK1-ERK activity.In general, activation of ERK1/2 is necessary for RSK1 activationby epidermal growth factor (Roux et al., 2003). The observationsthat Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by oltipraz was minimallydecreased by chemical inhibition of MKK1-ERK1/2 and that RSK1regulated Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by oltipraz indicatethat RSK1 activation elicited by oltipraz may not need the constitutiveactivity of ERK1/2. This is consistent with our previous observationthat oltipraz did not enhance the activity of MAPK and thatactivation of C/EBP $beta$ by oltipraz was independent of the ERK activity.

RSK1 activation by growth factors requires ERK docking nearthe C-terminal region (Roux et al., 2003). Ser³⁸⁰ phosphorylationof RSK1 (i.e., autophosphorylation) is catalyzed by the C-terminalkinase domain of activated RSK1. Activation of ERK initiatesa series of activating processes of RSK1 (Roux et al., 2003),which includes autophosphorylation of RSK1. We found that theRSK1 levels in cell lysates were unchanged after oltipraz treatment.In additional experiments, we observed that Ser³⁸⁰ phosphorylationin RSK1 was increased by oltipraz treatment, which was persistentfor up to 24 h. Increase in RSK1 kinase activity by oltiprazparalleled that in the Ser³⁸⁰ phosphorylation. It has been reportedthat RSK1 activated by epidermal growth factor or gonadotropin-releasinghormone translocates into the nucleus (Roux et al., 2003; Shahet al., 2003). After oltipraz treatment, RSK1, which was presentin the cytoplasm under the resting condition, localized in thenucleus. Taken together, our data support that oltipraz treatmentresults in activation of RSK1. In contrast to the activationof MAPKs and PI3-kinase by mitogens, oltipraz did not increasethe activities of the kinases (Kang et al., 2003). No changein oltipraz-inducible Ser¹⁰⁵ phosphorylation of C/EBP $beta$ by MKK1-ERK1/2inhibition supports that the mechanistic basis of RSK1 activationby oltipraz may differ from that by growth factors. The molecularbasis as to how oltipraz activates RSK1 remains to be elucidated.

The PI3-kinase pathway affects cell growth, survival, and motility.We showed previously that PI3-kinase regulates C/EBP $beta$ translocation,thus controlling C/EBP $beta$ activation in response to oltipraz orhepatocyte growth factor (Cho and Kim, 2003b; Kang et al., 2003).In this study, we found for the first time that oltipraz increasedthe activity of RSK1 for C/EBP $beta$ activation and that increasesin the metabolic activity and nuclear translocation of RSK1were dependent on the PI3-kinase activity. In general, fullactivation of RSK1 requires phosphorylation by PDK1, a constitutivelyactive kinase downstream of PI3-kinase (Casamayor et al., 1999;Richards et al., 2001). After activation by PDK1, RSK1 translocatesto the nucleus (Shah et al., 2003). In the current study, PI3-kinaseinhibition prevented nuclear translocation of RSK1 by oltipraz.We observed that either chemical inhibition of PI3-kinase orstable transfection with the plasmid encoding p85 regulatorysubunit almost completely inhibited an increase in Ser¹⁰⁵-phosphorylatedC/EBP $beta$ in the nuclear fraction, which was in line with the PI3-kinasedependence of RSK1 activation. It is likely that interruptionof C/EBP $beta$ activation by PI3-kinase inhibition, presumably throughPDK1 (and/or Akt) inhibition, results from no phosphorylationin C/EBP $beta$ at Ser¹⁰⁵. This is consistent with our previous observation(Kang et al., 2003) and also with the report that full RSK1activation requires PDK1 activity downstream from PI3-kinase.The data indicate that RSK1-mediated Ser¹⁰⁵ phosphorylationof C/EBP $beta$ by oltipraz requires the constitutive activity of PI3-kinase.

In conclusion, oltipraz induces phosphorylation of rat C/EBP $beta$ form at Ser¹⁰⁵ and the mouse and human forms at Thr^217/266.RSK1 activation by oltipraz, which is dependent on PI3-kinasebut not ERK1/2, contributes to the specific phosphorylationof C/EBP $beta$ that leads to recruitment of CBP coactivator for GSTA2gene transactivation. RSK1-mediated phosphorylation of C/EBP $beta$ at specific residues by a pharmacological agent and its genetransactivation holds a significant implication for the moleculartarget of oltipraz.

Footnotes

This work was supported by the National Research LaboratoryProgram (2001-2006), Korea Science and Engineering Foundation,The Ministry of Education, and Human Resources Development,the Republic of Korea.

Article, publication date, and citation information can be foundat http://molpharm.aspetjournals.org.

doi:10.1124/mol.105.018465.

ABBREVIATIONS: RSK, p90-ribosomal S6-kinase; C/EBP $beta$ , CCAAT/enhancerbinding protein- $beta$ ; ChIP, chromatin immunoprecipitation; CTT-RSK,C-terminal truncated-p90-ribosomal S6-kinase; ERK, extracellularsignal-regulated kinase; MAPK, mitogen-activated protein kinase;PDK1, 3-phosphoinositide-dependent protein kinase-1; PI3, phosphatidylinositol3; CBP, cAMP response element-binding protein binding protein;bp, base pair(s); HA, hemagglutinin; FCS, fetal calf serum;PCR, polymerase chain reaction; siRNA, small-interference RNA;scRNA, scrambled RNA; PKC, protein kinase C; GF109203, bisindoly-maleimide;U0126, 1,4-diamino-2,3-dicyano-1,4-bis(methylthio)butadiene;LY294002, 2-(4-morpholinyl)-8-phenyl-1(4H)-benzopyran-4-onehydrochloride; H89, N-[2-(4-bromocinnamylamino)ethyl]-5-isoquinoline.

The online version of this article (available at http://molpharm.aspetjournals.org)contains supplemental material.

Address correspondence to: Dr. Sang Geon Kim, College of Pharmacy, Seoul National University, Sillim-dong, Kwanak-gu, Seoul 151-742, South Korea. E-mail: sgk{at}snu.ac.kr

References

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Abstract
Materials and Methods
Results
Discussion
References

Bhatt RR and Ferrell JE Jr (1999) The protein kinase p90 RSK as an essential mediator of cytostatic factor activity. Science (Wash DC) 286: 1362-1365.[Abstract/Free Full Text]

Bolton MG, Munoz A, Jacobson LP, Groopman JD, Maxuitenko YY, Roebuck BD, and Kensler TW (1993) Transient intervention with oltipraz against aflatoxin-induced hepatic tumorigenesis. Cancer Res 53: 3499-3504.[Abstract/Free Full Text]

Buck M and Chojkier M (2003) Signal transduction in the liver: C/EBP $beta$ modulates cell proliferation and survival. Hepatology 37: 731-738.[CrossRef][Medline]

Buck M, Poli V, Hunter T, and Chojkier M (2001) C/EBP $beta$ phosphorylation by RSK creates a functional XEXD caspase inhibitory box critical for cell survival. Mol Cell 8: 807-816.

Role of p90 Ribosomal S6-Kinase-1 in Oltipraz-Induced Specific Phosphorylation of CCAAT/Enhancer Binding Protein- for GSTA2 Gene Transactivation

Role of p90 Ribosomal S6-Kinase-1 in Oltipraz-Induced Specific Phosphorylation of CCAAT/Enhancer Binding Protein- $beta$ for GSTA2 Gene Transactivation