IL-10-inducible Bcl-3 negatively regulates LPS-induced TNF-{alpha} production in macrophages

doi:10.1182/blood-2003-04-1228

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Blood, 1 December 2003, Vol. 102, No. 12, pp. 4123-4129.
Prepublished online as a Blood First Edition Paper on August 7, 2003; DOI 10.1182/blood-2003-04-1228.

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IMMUNOBIOLOGY
IL-10-inducible Bcl-3 negatively regulates LPS-induced TNF- ${alpha}$ production in macrophages
Hirotaka Kuwata, Yasuyuki Watanabe, Hiroyuki Miyoshi, Masahiro Yamamoto, Tsuneyasu Kaisho, Kiyoshi Takeda, and Shizuo Akira
From the Department of Host Defense, Research Institute for Microbial Diseases, Osaka University, Japan; Exploratory Research for Advanced Technology (ERATO), Japan Science and Technology Corporation, Suita, Osaka, Japan; the Subteam for Manipulation of Cell Fate, BioResource Center, RIKEN Tsukuba Institute, Tsukuba, Ibaraki, Japan; and RIKEN Research Center for Allergy and Immunology, Yokohama, Kanagawa, Japan.

   Abstract

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Interleukin-10 (IL-10) plays an important role in preventionof chronic inflammation in vivo. However, the molecular mechanismby which IL-10 exerts its anti-inflammatory response is poorlyunderstood. Here, we performed a microarray analysis and identifiedBcl-3 as an IL-10-inducible gene in macrophages. Lentiviralvector-mediated expression of Bcl-3 inhibited lipopolysaccharide(LPS)-induced production of tumor necrosis factor ${alpha}$ (TNF- ${alpha}$ ), butnot IL-6, in macrophages. In Bcl-3-transduced and IL-10-pretreatedmacrophages, LPS-induced nuclear translocation of nuclear factor ${kappa}$ B (NF- ${kappa}$ B) p65 was not impaired. However, DNA binding by NF- ${kappa}$ Bp50/p65 was profoundly inhibited. Nuclear localization of Bcl-3was associated with inhibition of LPS-induced TNF- ${alpha}$ production.Overexpression of Bcl-3 suppressed activation of the TNF- ${alpha}$ promoter,but not the IL-6 promoter. Bcl-3 interacted with NF- ${kappa}$ B p50 andwas recruited to the TNF- ${alpha}$ promoter, but not the IL-6 promoter,indicating that Bcl-3 facilitates p50-mediated inhibition ofTNF- ${alpha}$ expression. Furthermore, Bcl-3-deficient macrophages showeddefective IL-10-mediated suppression of LPS induction of TNF- ${alpha}$ ,but not IL-6. These findings suggest that IL-10-induced Bcl-3is required for suppression of TNF- ${alpha}$ production in macrophages.(Blood. 2003; 102:4123-4129)

   Introduction

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Interleukin-10 (IL-10) is produced by activated macrophagesand T cells, and plays an important role in anti-inflammatoryresponses.¹ Indeed, mice lacking IL-10 or the IL-10 receptordeveloped chronic enterocolitis and showed enhanced inflammatoryresponses.^2-4 Furthermore, transfer of the IL-10 gene reducedthe incidence of colitis in mice, and treatment with IL-10 isnow anticipated to be used clinically for patients with inflammatorybowel diseases.^5,6 The anti-inflammatory activity of IL-10 ismainly elicited by inhibition of the activity of macrophages/monocytes.IL-10 inhibits lipopolysaccharide (LPS)-induced production ofinflammatory cytokines, including tumor necrosis factor ${alpha}$ (TNF- ${alpha}$ ),IL-6, and IL-12, by macrophages. Many attempts have been madeto elucidate the mechanism by which IL-10 inhibits cytokineproduction by macrophages, and several models have been proposed.These include inhibition of nuclear factor ${kappa}$ B (NF- ${kappa}$ B) and mitogen-activatedprotein (MAP) kinase activity, and reduction of transcriptionand stability of mRNA for cytokine genes.^7-10 However, the precisemechanism by which IL-10 suppresses macrophage activity remainsunclear.
The IL-10 receptor consists of the ligand binding subunit, IL-10R1,and an accessory subunit, IL-10R2. Binding of IL-10 to the IL-10receptor induces activation of the Janus kinase (JAK) familyof tyrosine kinases, Jak1 and Tyk2, which are constitutivelyassociated with IL-10R1 and IL-10R2, respectively.¹ Jak1 andTyk2 activation is followed by phosphorylation of the latenttranscription factor signal transducer and activator of transcription3 (Stat3). Studies with gene-targeted mice have revealed thatJak1 and Stat3 play a pivotal role in the IL-10 signaling pathway.Macrophages from Jak1-deficient mice did not show an anti-inflammatoryresponse to IL-10.^11,12 Mice in which Stat3 was specificallydeleted in the myeloid lineage cells, including macrophages,developed chronic enterocolitis. Macrophages from these mutantmice were unresponsive to IL-10.¹³ Furthermore, a recent studywith additional gene deletions demonstrated that overproductionof IL-12p40 from Stat3-deficient macrophages caused enhancedTh1 responses leading to the development of Th1-dependent chronicenterocolitis.¹⁴ These studies indicate that macrophages arethe main target cells of IL-10, which exhibits anti-inflammatoryresponses in vivo. Several studies have indicated that de novoprotein synthesis is required for IL-10 inhibition of LPS-inducedcytokine production.^9,15,16 Therefore, genes induced by IL-10-mediatedStat3 activation in macrophages are expected to be responsiblefor anti-inflammatory responses. In this context, several IL-10-induciblegenes, such as SOCS3 and heme oxygenase-1, have been identified.^17-19However, it is still controversial how these gene products contributeto anti-inflammatory responses.
In this study, we addressed the mechanism by which IL-10 inhibitsLPS-induced TNF- ${alpha}$ production in macrophages. A gene array analysisled to the identification of several IL-10 target genes, includingBcl-3, in macrophages. Introduction of these genes into macrophagesby lentiviral vectors revealed that Bcl-3 inhibited LPS-inducedTNF- ${alpha}$ production. Bcl-3 was associated with NF- ${kappa}$ B p50 and preferentiallyrecruited to the TNF- ${alpha}$ promoter. Macrophages from Bcl-3-deficientmice were defective in IL-10-mediated suppression of TNF- ${alpha}$ production.Thus, Bcl-3 induced by IL-10 is responsible for inhibition ofLPS-induced TNF- ${alpha}$ production in macrophages.

   Materials and methods

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Reagents and cell culture
LPS from Escherichia coli (O55:B5) was purchased from Sigma(St Louis, MO). The mouse macrophage cell line (RAW264.7) andhuman embryonic kidney cells (293T) were cultured in Dulbeccomodified Eagle medium (DMEM) supplemented with 10% fetal bovineserum (FBS), 100 µg/mL streptomycin, and 10 U/mL penicillinG. Mouse peritoneal macrophages were collected by peritoneallavage with Hanks balanced salt solution at 3 days after intraperitonealinjection of 2 mL of 4% sterile thioglycollate into 8- to 12-week-oldmice. Peritoneal macrophages were cultured in RPMI 1640 mediumwith 10% FBS, 100 µg/mL streptomycin, and 10 U/mL penicillinG.
Mice
The generation of myeloid cell-specific Stat3-deficient micewas described previously.¹³ IL-10- and Bcl-3-deficient micewere purchased from The Jackson Laboratory (Bar Harbor, ME).
Affymetrix gene expression profiling
RAW264.7 and peritoneal macrophages were treated with IL-10(10 ng/mL) for 2, 4, or 6 hours. Total RNA was extracted withan RNeasy kit (Qiagen, Hilden, Germany), followed by mRNA purificationwith an Oligotex mRNA Kit (Pharmacia, Piscataway, NJ). Double-strandedcDNA was synthesized from 1 µg mRNA with the SuperScriptChoice System (Invitrogen, Carlsbad, CA) primed with T7-(dT)24 primer. These cDNAs were used to prepare biotin-labeled cRNAby an in vitro transcription reaction performed using T7 RNApolymerase in the presence of biotinylated-ribonucleotides,according to the manufacturer's protocol (Enzo Diagnostics,Farmingdale, NY). The cRNA product was purified using an RNeasykit (Qiagen), fragmented, and hybridized to Affymetrix MurineGenome U74Av2, Bv2, and Cv2 microarray chips, according to themanufacturer's protocol (Affymetrix, Santa Clara, CA). The hybridizedchips were stained, washed, and scanned with a GeneArray Scanner(Affymetrix).
Electrophoretic mobility shift assay (EMSA)
Macrophages were treated with 10 ng/mL IL-10 for 18 hours, andstimulated with 100 ng/mL LPS for 60 minutes. Then, nuclearproteins were extracted, and then incubated with an end-labeled,double-stranded oligonucleotide containing a NF- ${kappa}$ B binding siteof the TNF- ${alpha}$ promoter in 25 µL binding buffer (10 mM HEPES-KOH[N-2-hydroxyethylpiperazine-N'-2-ethanesulfonic acid-potassiumhydroxide, pH 7.8], 50 mM KCl, 1 mM EDTA [ethylenediaminetetraaceticacid, pH 8.0], 5 mM MgCl₂, and 10% glycerol) for 20 minutesat room temperature and loaded on a native 5% polyacrylamidegel. The DNA-protein complexes were visualized by autoradiography.The specificities of the shifted bands were determined by addingantibodies specific for p65 and p50 (Santa Cruz Biotechnology,Santa Cruz, CA).
Production of lentiviral vector and infection
The lentiviral vector, CSII-EF-MCS-IRES-hrGFP (cPPT-containingSIN vector plasmid containing multicloning sites for cDNA insertionfollowed by the internal ribosomal entry site-green fluorescentprotein [IRES-GFP] sequence under the control of the EF-1 ${alpha}$ promoter),was used to generate CSII-EF-Bcl-3 and CSII-EF-SOCS3. Woodchuckhepatitis virus posttranslational regulatory element (PRE) wasligated at the 3' end of GFP. The lentiviral vectors were cotransfectedinto 293T cells with pMDLg/p RRE (packaging plasmid), pRSV-Rev(Rev expression plasmid), and pMD.G (VSV-G expression plasmid).Infectious lentiviruses in the culture supernatants were harvestedat 48 hours after transfection. RAW cells (5 x 10⁵) were culturedwith the lentiviruses for 24 hours and then the culture mediumwas replaced. The transduction efficiency was monitored by GFPexpression.
Flow cytometric analysis
Cells were stimulated with 100 ng/mL LPS, harvested, and incubatedwith 4% paraformaldehyde. The cells were then incubated witha phycoerythrin (PE)-conjugated anti-TNF- ${alpha}$ antibody (Ab; PharMingen,San Diego, CA). Stained cells were analyzed in a fluorescence-activatedcell sorter (FACS) Calibur using the Cell Quest software (BectonDickinson, San Jose, CA).
Measurement of cytokines and NO in culture supernatants
RAW cells and peritoneal macrophages (5 x 10⁴) were culturedin 96-well plates with 30 ng/mL interferon ${gamma}$ (IFN ${gamma}$ ) and 10 ng/mLLPS for 24 hours. The concentrations of TNF- ${alpha}$ and IL-6 in theculture supernatants were determined by enzyme-linked immunosorbentassay (ELISA) according to the manufacturer's instructions (GenzymeTechne, Minneapolis, MN). The concentration of nitric oxide(NO) was measured using Griess reagents according to the manufacturer'sinstructions (Dojindo, Kumamoto, Japan).
Luciferase assay
Mouse Bcl-3 expression constructs were cloned into the pEF-BOSmammalian expression vector. The TNF ${alpha}$ and IL-6 promoters containinggenomic fragments from -1260 to +140 and -1232 to +39, respectively,were cloned into the pGL3-basic vector (Promega, Madison, WI).RAW cells were transfected with expression constructs usingthe Superfect transfection reagent (Qiagen). The luciferaseactivities of total cell lysates were measured using the Dual-luciferasereporter assay system (Promega). The Renilla-luciferase reportergene (50 ng) was used as an internal control. In all cases,the data were normalized for transfection efficiency by dividingthe firefly luciferase by that of the Renilla luciferase.
Immunoprecipitation assays
For immunoprecipitation assay, Myc-tagged Bcl-3 and Flag-taggedp50, p52 were cloned into pEF-BOS and pcDNA3.1, respectively.These expression vectors were transfected into 293 cells usingLipofectoamine 2000 (Invitrogen). Transfected cells were solubilizedwith 1 mL radioimmunoprecipitation assay (RIPA) lysis buffer(50 mM Tris [tris(hydroxymethyl)aminomethane]-HCl, pH 7.4, 150mM NaCl, 1% Triton X-100, 1 mM EDTA, 0.5% Na-deoxycholate, 1mM phenylmethylsulfonyl fluoride [PMSF], and 1 mg/mL each leupeptinand pepstatin). Whole cell lysates were incubated with antibodiesto Myc-Tag 9B11 (Cell Signaling Technology, Beverly, MA), anti-FlagM2 antibody (Sigma). Immunoprecipitates were separated on sodiumdodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE),transferred to polyvinylidene fluoride (PVDF) membrane, andincubated with anti-Myc tag antibody (A-14; Santa Cruz Biotechnology)or anti-Flag M2 antibody. Bound antibodies were visualized withan enhanced chemiluminescence system (Perkin Elmer, Boston,MA).
Immunofluorescence staining and confocal microscopy
Cells on 3.5-cm dishes were washed with Tris-buffered saline(TBS) and fixed with 3.7% formaldehyde in TBS for 15 minutesat room temperature. After permeabilization with 0.2% TritonX-100, cells were washed with TBS and incubated with a rabbitanti-Bcl-3 Ab (Santa Cruz Biotechnology) in TBS containing 1%bovine serum albumin at 10 ng/mL, followed by incubation withAlexa Fluor 594-conjugated goat anti-rabbit immunoglobulin G(IgG; Molecular Probes, Eugene, OR). To stain the nucleus, cellswere cultured with 0.5 µg 4',6-diamidino-2-phenylindole(DAPI; Wako, Osaka, Japan). Confocal microscopy was performedusing an LSM510 model confocal microscope (Carl Zeiss, Oberkochem,Germany).
Chromatin immunoprecipitation
Chromatin immunoprecipitation (ChIP) was performed essentiallywith a described protocol (Upstate Biotechnology, Lake Placid,NY). In brief, RAW cells were transfected with Myc-tagged Bcl-3and Flag-tagged p50 expression vectors using Nucleofector (Amaxa,Germany). At 48 hours after transfection, cells were stimulatedwith 100 ng/mL LPS for 2 hours and then fixed with formaldehydefor 10 minutes. The cells were lysed, sheared by sonication,and incubated overnight with specific antibody followed by incubationwith protein A-agarose saturated with salmon sperm DNA (UpstateBiotechnology). Precipitated DNAs were analyzed by quantitativepolymerase chain reaction (PCR, 35 cycles) using primers 5'-ACTAGCCAGGAGGGAGAACAGAAACTC-3'and 5'-CACAAGCAGGAATGAGAAGAGGCTGAG-3' for the TNF- ${alpha}$ promoterand 5'-TAGCAGCAGGTCCAACTGTGCTATCTG-3' and 5'-AAGCCTCCGACTTGTGAAGTGGTATAG-3'for the IL-6 promoter.

   Results

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Identification of IL-10-inducible genes in macrophages
In order to identify IL-10-inducible genes that are responsiblefor the inhibition of LPS-induced cytokine production, a microarrayanalysis was performed. Thioglycollate-elicited mouse peritonealmacrophages and RAW264.7 cells were treated with 10 ng/mL IL-10for 2, 4, and 6 hours, and gene induction was analyzed. Thisanalysis resulted in the identification of several IL-10-induciblegenes, including SOCS3, p19^INK4D, and the IL-4 receptor ${alpha}$ , whichwere all shown previously to be induced by IL-10 in macrophages.^18-20Among these IL-10-inducible genes, we found that expressionof Bcl-3 was induced 3-fold in both RAW264.7 cells and peritonealmacrophages (Figure 1A, data not shown). We confirmed the IL-10-inducedmRNA expression of Bcl-3 and SOCS3 in RAW264.7 cells and peritonealmacrophages by Northern blotting (Figure 1B). Both Bcl-3 andSOCS3 mRNA expression were rapidly induced within one hour ofIL-10 treatment. In peritoneal macrophages from IL-10-deficientmice, IL-10-induced mRNA expression of Bcl-3 and SOCS3 was enhancedcompared with wild-type macrophages. However, IL-10-inducedBcl-3 and SOCS3 expression was completely abolished in Stat3-deficientmacrophages, indicating that the IL-10-induced expression ofboth genes is dependent on the Stat3-mediated pathway (Figure 1C).Addition of cycloheximide did not block the induction ofeither Bcl-3 or SOCS3 mRNA, indicating that protein synthesisis not required for the IL-10 induction of these genes (Figure 1D).

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Figure 1.. Microarray analysis of IL-10-inducible genes in macrophages. (A) Genes induced by IL-10 in peritoneal macrophages. Representative results in peritoneal macrophages treated with 10 ng/mL IL-10 for 4 hours are shown in the scatter plot. Similar results were observed in peritoneal macrophages treated with IL-10 for 2 hours, and RAW cells treated for 2 hours and 4 hours. (B) RAW cells and peritoneal macrophages were cultured in the absence or presence of 10 ng/mL IL-10 for the indicated periods. Total RNA was extracted and analyzed by a Northern blot using ³²P-labeled Bcl-3 and SOCS3. Hybridization with a ${beta}$ -actin probe confirmed even loading of RNA in each lane. Data are representative of 3 independent experiments. (C) Peritoneal macrophages isolated from wild-type, IL-10-deficient, and Stat3-mutant mice were treated with 10 ng/mL IL-10 for 2 hours. Total RNA was extracted and analyzed for Bcl-3 and SOCS3 expression by Northern blotting. KO indicates knock-out. (D) Peritoneal macrophages isolated from wild-type mice were treated with 10 ng/mL IL-10 for 2 hours in the presence or absence of 1 µg/mL cycloheximide (CHX) for 0.5 hours. Samples were analyzed by Northern blotting as in panel B.

Lentiviral transduction of Bcl-3 into macrophages results in reduced LPS-induced TNF- ${alpha}$ production
We next tried to transfer these IL-10-inducible genes into macrophages.Since macrophages are not susceptible to most gene-transfermethods, we tested lentiviral vectors that are capable of transducingnondividing cells.^21-23 To assess the transduction efficiency,the CSII-EF lentiviral vector containing the green fluorescentprotein (GFP) gene was used to transduce several types of macrophagesand efficient transduction was achieved (GFP-positive cellsrepresented more than 80% of RAW cells, 50% of bone marrow-derivedmacrophages, and 30% of peritoneal macrophages). We then constructedlentiviral vectors containing Bcl-3 or SOCS3 (Figure 2A) andtransduced them into RAW264.7 cells and bone marrow-derivedmacrophages. The lentiviral vector containing only the GFP (CSII-EF)was used as a control in all experiments. RAW264.7 cells andbone marrow-derived macrophages were infected with lentivirus,and after 2 days of culture, cells were stimulated with LPSand analyzed for TNF- ${alpha}$ production by intracellular staining.As shown in Figure 2B, neither lentiviral infection alone norwith SOCS3 caused any change in the LPS-induced TNF- ${alpha}$ productionin RAW264.7 cells. In contrast, expression of Bcl-3 resultedin a dramatic decrease in the number of cells producing TNF- ${alpha}$ (Figure 2B). Similar findings were also observed in bone marrowmacrophages (data not shown). Next, GFP-positive cells wereisolated by FACS and stimulated with LPS, and the productionof TNF- ${alpha}$ in the culture supernatants was analyzed (Figure 2C).Cells expressing GFP alone secreted significant amounts of TNF- ${alpha}$ in response to LPS. However, LPS-induced secretion of TNF- ${alpha}$ wasseverely reduced in cells transduced with Bcl-3/GFP. We alsoanalyzed the LPS-induced mRNA expression of TNF- ${alpha}$ (Figure 2D).Introduction of Bcl-3/GFP severely impaired LPS induction ofTNF- ${alpha}$ mRNA. Thus, lentiviral expression of Bcl-3 in macrophagesinhibited the LPS-induced production of TNF- ${alpha}$ . However, in RAW264.7cells transduced with Bcl-3/GFP, LPS-induced IL-6 productionwas not reduced, indicating that the expression of Bcl-3 didnot result in the impairment of all LPS responses in macrophages(Figure 2E). We next lentivirally expressed I ${kappa}$ B ${epsilon}$ , an inhibitorof ${kappa}$ B ${epsilon}$ , that is structurally related to Bcl-3.²⁴ Lentiviral expressionof I ${kappa}$ B ${epsilon}$ in RAW 264.7 cells did not inhibit LPS-induced TNF- ${alpha}$ production,indicating that Bcl-3 is specifically involved in the inhibitionof LPS-induced TNF- ${alpha}$ production in macrophages (Figure 2F).

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Figure 2.. Lentiviral introduction of Bcl-3 results in reduced LPS-induced TNF- ${alpha}$ production in macrophages. (A) Schematic drawings of the lentivirus vector containing a murine Bcl-3 or SOCS3 gene cassette. (B) RAW cells were infected with lentivirus expressing Bcl-3/GFP or SOCS3/GFP. After infection for 24 hours, RAW cells were washed and additionally incubated for 2 days. The cells were then stimulated with LPS (10 ng/mL) for 6 hours, intracellularly stained for TNF- ${alpha}$ , and analyzed by flow cytometry. (C) GFP-positive cells were collected with FACS, and stimulated with IFN- ${gamma}$ (30 ng/mL) and LPS (10 ng/mL) for 24 hours. The concentration of TNF- ${alpha}$ in the culture supernatants was determined by ELISA. Error bars indicate SD. (D) GFP-positive cells (GFP alone and Bcl-3/GFP) were purified and stimulated with LPS (100 ng/mL) for 4 hours, and then total RNA extracts were analyzed for the mRNA expression of TNF- ${alpha}$ . Hybridization with the ${beta}$ -actin probe confirmed even loading of RNA in each lane. (E) GFP-positive cells were stimulated with IFN- ${gamma}$ (30 ng/mL) and LPS (10 ng/mL) for 24 hours. The IL-6 concentration in the culture supernatants was measured by ELISA. Error bars indicate SD. (F) RAW cells were infected with a lentivirus expressing I ${kappa}$ B ${epsilon}$ /GFP. After infection for 24 hours, RAW cells were washed and additionally incubated for 2 days. The cells were then stimulated with LPS (10 ng/mL) for 6 hours and analyzed for intracellular production of TNF- ${alpha}$ by flow cytometry.

Nuclear expression of Bcl-3 is required for inhibition of LPS-induced TNF- ${alpha}$ production
In accordance with previous reports, expression of Bcl-3 waspredominantly observed in the nucleus in Bcl-3/GFP-transducedRAW cells^25-27 (Figure 3B, upper). We addressed whether thisnuclear localization of Bcl-3 was associated with the inhibitionof LPS responses. Bcl-3 is composed of 7 central ankyrin repeats,which are essential for interaction with NF- ${kappa}$ B p50 and p52 homodimers,and an N-terminal basic nuclear localization sequence (NLS).^28,29We generated deletion mutants that lacked the N-terminal NLS( ${Delta}$ N) or the N-terminal 154 residues including the first ankyrinrepeat ( ${Delta}$ ANK) and lentivirally introduced these mutants intoRAW cells (Figure 3A). Immunofluorescent staining with an anti-Bcl-3Ab detecting the C-terminal portion of the Bcl-3 protein showedthat ${Delta}$ N and ${Delta}$ ANK were not localized in the nucleus but expressedin the cytoplasm (Figure 3B). When LPS-induced TNF- ${alpha}$ productionwas analyzed, cells transduced with ${Delta}$ N/GFP and ${Delta}$ ANK/GFP did notshow any reduction in TNF- ${alpha}$ production (Figure 3C). Thus, thenuclear localization of Bcl-3 was associated with its inhibitoryeffect on TNF- ${alpha}$ production.

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Figure 3.. Nuclear-localized Bcl-3 inhibits the LPS response in macrophages. (A) Schematic structures of the deletion mutants of Bcl-3. ${Delta}$ N lacks the N-terminal nuclear localization signal. ${Delta}$ ANK lacks the N-terminal 154 residues including the first ankyrin repeat. (B) Lentivirus-infected RAW cells (green) were stained with anti-Bcl-3 (red) and DAPI (blue), and analyzed by confocal microscopy. Scale bar: 2 µm. (C) Lentivirus-infected RAW cells were stimulated with LPS (10 ng/mL) for 6 hours, stained with anti-TNF- ${alpha}$ , and analyzed by flow cytometry.

We next analyzed LPS-induced NF- ${kappa}$ B activation in cells transducedwith Bcl-3/GFP. GFP-positive cells were isolated by FACS andstimulated with LPS for 60 minutes, and p65 expression in thenucleus was analyzed by Western blotting (Figure 4A). LPS-inducednuclear translocation of p65 was observed in Bcl-3-transducedcells as well as in cells transduced with GFP alone. We nextanalyzed the DNA binding activity of NF- ${kappa}$ B (Figure 4B). LPS stimulationled to enhanced DNA binding activity of p50/p50 homodimers andp50/p65 heterodimers in cells transduced with GFP alone. InBcl-3-transduced cells, the DNA binding activity by p50/p50homodimers was observed before LPS stimulation, and furtherLPS stimulation did not induce any activation of p50/p65 heterodimers.In IL-10-pretreated peritoneal macrophages and RAW cells, LPS-inducednuclear translocation of p65 was normally observed, but theDNA binding activity of p50/p65 heterodimers was severely reduced(Figure 4C-D). The specificity of the bands was confirmed bysupershifts by treatment with anti-p50 and anti-p65 antibodies(Figure 4D). These findings are similar to those observed inBcl-3-transduced macrophages, indicating that IL-10-inducibleBcl-3 is required for suppression of NF- ${kappa}$ B activity in the nucleus.

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Figure 4.. Impaired NF- ${kappa}$ B activity in Bcl-3-transduced and IL-10-pretreated macrophages. (A) Western blot showing the nuclear expression of p65 subunit of NF- ${kappa}$ B after LPS stimulation (1 hour) in RAW cells transduced with GFP alone or Bcl-3/GFP. (B) RAW cells transduced with GFP alone or Bcl-3/GFP were stimulated with LPS and nuclear extracts were subjected to EMSA. There are 2 types of NF- ${kappa}$ B binding to the probe, p50/p65 heterodimers and p50/p50 homodimers, indicated by the arrow and arrowhead, respectively. (C) Western blot showing the nuclear expression of p65 before and 60 minutes after LPS stimulation in nonpretreated (med) and IL-10-pretreated (IL-10) RAW macrophages. (D) RAW cells were pretreated with 10 ng/mL IL-10 for 18 hours and stimulated with 10 ng/mL LPS for 60 minutes. Nuclear extracts were subjected to EMSA using the NF- ${kappa}$ B binding site of the TNF- ${alpha}$ promoter as a probe. The specificities of the shifted bands were determined by adding specific Abs to p50 (arrow) and p65 (arrowhead). Similar results were observed in mouse peritoneal macrophages.

Ectopic expression of Bcl-3 inhibits LPS-induced activation of the TNF- ${alpha}$ promoter, but not the IL-6 promoter
We next examined the effect of transient overexpression of Bcl-3on LPS-induced activation of the TNF- ${alpha}$ and IL-6 promoters usinga reporter gene assay. Bcl-3 overexpression suppressed LPS-inducedtranscriptional activity of the TNF- ${alpha}$ promoter in RAW cells (Figure 5A).In contrast, Bcl-3 expression had no effect on LPS-inducedtransactivation of the IL-6 promoter in RAW cells (Figure 5B).Overexpression of Bcl-3 ${Delta}$ N, the mutant Bcl-3 lacking the N-terminalNLS, did not suppress the activity of the TNF- ${alpha}$ promoter, indicatingthat the N-terminal NLS is required for suppression of the TNF- ${alpha}$ promoter (Figure 5A). Thus, Bcl-3 has an inhibitory effect onthe LPS-induced activation of the TNF- ${alpha}$ promoter, but not theIL-6 promoter.

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Figure 5.. Overexpression of Bcl-3 inhibits LPS-induced transactivation of the TNF- ${alpha}$ promoter. (A) RAW cells were transiently cotransfected with the TNF- ${alpha}$ promoter-luciferase construct (10 ng) and the expression vectors for full-length Bcl-3 or ${Delta}$ N (10 ng, 100 ng, or 500 ng), as indicated. After 24 hours of transfection, cells were treated with or without 1 µg/mL LPS for 8 hours and then the luciferase activities were measured. Data are representative of 3 independent experiments yielding similar results. Data are expressed as relative fold activation compared with the nonstimulated (-) set. (B) RAW cells were transiently cotransfected with the IL-6 promoter-luciferase construct (100 ng) and the expression vector for Bcl-3 (10 ng, 100 ng, or 500 ng), as indicated. The cells were treated with 1 µg/mL LPS for 8 hours and luciferase activity was detected. Representative results of 3 independent experiments are shown. (C) The 293 cells were transfected with various combinations of pEF-BOS-Myc-Bcl-3, pcDNA3.1-Flag-p50, and pcDNA3.1-Flag-p52 in a 6-well dish (each 1 µg/well). Total amount of transfected DNA was kept at 2 µg by adding pEF-BOS or pcDNA 3.1. p50 and p52 were immunoblotted by anti-Flag antibody (M2 monoclonal antibody). Bcl-3 was immunoblotted by rabbit polyclonal anti-c-Myc antibody. Plasmids transfected are indicated on top of the panel. (D) RAW cells expressing Myc-Bcl-3 and Flag-p50 were stimulated with 100 ng/mL LPS for 2 hours, and chromatin immunoprecipitation assays were performed with ${alpha}$ -Myc or ${alpha}$ -Flag antibodies. The detection of the immunoprecipitated TNF- ${alpha}$ promoter (left panel) or IL-6 promoter (right panel) was analyzed by PCR with promoter-specific primers. Representative of 3 independent experiments. (E) RAW cells were transiently cotransfected with pELAM-1, Flag-p50 (0, 1, 10, 100 ng/well), and pEF-BOS Bcl-3 (100 ng/well) expression plasmids. After 24 hours of transfection, cells were treated with 1 µg/mL LPS for 8 hours and then luciferase activity was detected. Data are expressed as relative fold activation compared with the nontransfected set. Error bars indicate SD.

We further addressed the mechanism by which Bcl-3 inhibits theTNF- ${alpha}$ promoter activity. Consistent with the previous reports,^28,29coimmunoprecipitation analysis showed that Bcl-3 interactedwith NF- ${kappa}$ B p50 and p52 (Figure 5C). We next performed chromatinimmunoprecipitation (ChIP) assays to further investigate whetherBcl-3 regulates activity of the TNF- ${alpha}$ promoter. Since the availableanti-Bcl-3 antibody could not be used for immunoprecipitation,we expressed Myc-tagged Bcl-3 and Flag-tagged p50 in RAW cellsand used them for the experiments. RAW cells were stimulatedwith LPS for 2 hours, and ChIP assays were performed using anti-Mycand anti-Flag Abs (Figure 5D). In RAW cells expressing Bcl-3and p50, both Bcl-3 and p50 were recruited to the TNF- ${alpha}$ promoterbefore LPS stimulation. LPS stimulation did not induce any changein the recruitment of Bcl-3 and p50. In contrast, Bcl-3 wasnot recruited to the IL-6 promoter. Furthermore, LPS-inducedp50 recruitment was normally observed in the IL-6 promoter,indicating that Bcl-3 expression did not have any effect onthe IL-6 promoter. We next analyzed the effect of p50 overexpressionon activity of the TNF- ${alpha}$ promoter (Figure 5E). Although expressionof a small amount of p50 enhanced activity of the TNF- ${alpha}$ promoter,increasing amounts of p50 suppressed the promoter activity.Coexpression of Bcl-3 further enhanced p50-mediated suppressionof the TNF- ${alpha}$ promoter activity. Taken together, these resultssuggest that Bcl-3 is specifically involved in suppression ofthe TNF- ${alpha}$ promoter together with NF- ${kappa}$ B p50.
Macrophages from Bcl-3-deficient mice are defective in IL-10-induced suppression of TNF- ${alpha}$ production
Finally, we analyzed whether Bcl-3 deficiency resulted in defectiveIL-10 responses. Peritoneal macrophages were isolated from wild-typeand Bcl-3-deficient mice, pretreated with increasing amountsof IL-10, and stimulated with LPS. In wild-type mice, IL-10pretreatment resulted in a dose-dependent suppression of LPS-inducedproduction of TNF- ${alpha}$ and IL-6 (Figure 6A-B). The IL-10-inducedsuppression of IL-6 production was similarly observed in Bcl-3-deficientmacrophages (Figure 6A). However, when Bcl-3-deficient macrophageswere pretreated with less than 1 ng/mL IL-10, suppression ofLPS-induced TNF- ${alpha}$ production was scarcely detected, althoughhigher concentrations of IL-10 partially decreased TNF- ${alpha}$ production(Figure 6B). When macrophages from wild-type mice were pretreatedwith 10 ng/mL IL-10, LPS-induced TNF- ${alpha}$ mRNA expression was severelyinhibited, but only partial impairment was observed in Bcl-3-deficientmacrophages (Figure 6C). Thus, Bcl-3-deficient macrophages showeddefective IL-10-mediated suppression of LPS-induced TNF- ${alpha}$ production,demonstrating that IL-10-induced Bcl-3 is critical for the inhibitionof LPS-induced TNF- ${alpha}$ production.

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Figure 6.. Bcl-3-deficient macrophages are defective in IL-10-mediated suppression of LPS-induced TNF- ${alpha}$ production. (A-B) Peritoneal macrophages from wild-type and Bcl-3-deficient mice were pretreated with IL-10 at the indicated concentrations for 18 hours and stimulated with 100 ng/mL LPS for an additional 24 hours. Concentrations of IL-6 (A) and TNF- ${alpha}$ (B) in the culture supernatants were measured by ELISA. The experiments were repeated with 3 different animals and produced similar results. Open circles indicate wild-type mice; closed squares, Bcl-3-deficient mice. (C) Peritoneal macrophages from wild-type and Bcl-3-deficient mice were pretreated with 10 ng/mL IL-10 for 18 hours and stimulated with 100 ng/mL LPS for 2 hours. TNF- ${alpha}$ mRNA expression was analyzed by Northern blotting.

   Discussion

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

In this study, we analyzed the mechanism by which IL-10 exhibitsnegative regulatory effects on macrophages. A microarray analysisled to the identification of IL-10-inducible genes in macrophages.In the course of analyzing the mechanism underlying the anti-inflammatoryeffect of IL-10, several IL-10-inducible genes have so far beenidentified.^17-20,30 Among these gene products, heme oxygenase-1(HO-1) and SOCS3 have been proposed to be involved in IL-10-mediatedsuppression of macrophage activity.^17,18 SOCS3 is a member ofthe family of suppressors of cytokine signaling (SOCS) proteins,which play important roles in the negative regulation of cytokinesignaling pathways.³¹ A member of this family, SOCS1, has recentlybeen shown to negatively regulate LPS signaling, as well ascytokine signaling, since SOCS1-deficient mice were highly sensitiveto LPS.^32,33 Similarly, in vitro studies indicated that IL-10-inducedSOCS3 negatively regulates the LPS induction of TNF- ${alpha}$ and IL-6in macrophages.¹⁸ In this study, however, lentiviral expressionof SOCS3 did not cause any reduction in LPS-induced TNF- ${alpha}$ productionin macrophages (Figure 2).
In addition to SOCS3, we identified Bcl-3 as an IL-10-induciblegene in macrophages. Bcl-3 is a member of the I ${kappa}$ B protein family,harboring ankyrin repeat domains. However, unlike other I ${kappa}$ B proteins,which are associated with NF- ${kappa}$ B transcription factors and sequesterthem in the cytoplasm, Bcl-3 is localized in the nucleus.^25,34The role of Bcl-3 in the regulation of NF- ${kappa}$ B activity is stillcontroversial. Although several studies have indicated thatBcl-3 is a negative regulator of NF- ${kappa}$ B,^28,35-37 Bcl-3 has beenshown to act as a transcriptional activator in some cases.^25,34Studies with Bcl-3-deficient mice have demonstrated an importantrole of Bcl-3 in B-cell and T-cell functions, but how Bcl-3functions in macrophages remains unclear.^38,39 Lentiviral expressionof Bcl-3 inhibited LPS-induced production of TNF- ${alpha}$ , but not IL-6,in macrophages (Figure 2). Overexpression of Bcl-3 also inhibitedLPS-induced activation of the TNF- ${alpha}$ promoter, but not the IL-6promoter, in macrophages (Figure 5). Furthermore, Bcl-3-deficientmacrophages showed defective IL-10-mediated suppression in theproduction of TNF- ${alpha}$ , but not IL-6 (Figure 6). Thus, the presentstudy clearly demonstrates that Bcl-3 functions as a negativeregulator of LPS-induced TNF- ${alpha}$ production in macrophages. Bcl-3interacted preferentially with homodimers of p50 and p52, neitherof which harbors the transactivation domains^25,34,40 (Figure 5C).Furthermore, Bcl-3 was preferentially recruited to theTNF- ${alpha}$ promoter and enhanced p50-mediated inhibition of the TNF- ${alpha}$ promoter activity (Figure 5D-E). Therefore, although the molecularmechanism by which Bcl-3 inhibits TNF- ${alpha}$ production remains unclear,Bcl-3 may interfere with the transcriptional activity of NF- ${kappa}$ Bin the TNF- ${alpha}$ promoter through association with p50 or p52.
In Bcl-3-transduced macrophages, the LPS-induced DNA bindingactivity of NF- ${kappa}$ B p50/p65 heterodimers was impaired, and thiswas also observed in IL-10-pretreated macrophages. However,LPS-induced IL-6 production was not impaired in Bcl-3-transducedcells. From these observations, we hypothesize 2 possibilities.First, although the inductions of both TNF- ${alpha}$ and IL-6 are dependenton NF- ${kappa}$ B, individual NF- ${kappa}$ B subunits differentially regulate theinduction of inflammatory cytokine genes. For instance, theIL-12p40 gene is selectively regulated by the c-Rel subunit,⁴¹and the IL-6 gene is mainly regulated by the p50 subunit, sincemacrophages from mice lacking the p50 subunit were defectivein LPS-induced production of IL-6, but not TNF- ${alpha}$ .⁴² Introductionof increasing amounts of p50 into RAW cells resulted in a dose-dependentinhibition of transactivation of the TNF- ${alpha}$ promoter, but notthe IL-6 promoter (Figure 5E; H.K., unpublished data, February2003). These results indicate that p50 subunits, especiallyp50 homodimers, may have an inhibitory effect on the TNF- ${alpha}$ promoter,but not the IL-6 promoter, and may enable LPS induction of theIL-6 gene in IL-10-pretreated macrophages. Alternatively, sincethe IL-6 gene has been shown to be regulated by several transcriptionfactors, such as NF-IL6 and AP-1 family members in additionto NF- ${kappa}$ B, IL-6 may be induced by activation of these transcriptionfactors. Thus, IL-10-inducible Bcl-3 is responsible for partof the IL-10-mediated suppression of macrophage activity, andadditional molecules must be involved in the IL-10-mediatedmacrophage suppression. Indeed, although Stat3 mutant mice producedtremendously high levels of inflammatory cytokines in responseto LPS, Bcl-3-deficient mice did not show increased production(Takeda et al¹³; and H.K., unpublished data, March 2003). Anovel molecule harboring ankyrin repeats and showing high similaritywith Bcl-3 has been identified as I ${kappa}$ B ${zeta}$ /IL-1-inducible nuclearankyrin-repeat protein (INAP)/molecule possessing ankyrin repeatsinduced by lipopolysaccharide (MAIL).^43-45 I ${kappa}$ B ${zeta}$ /INAP/MAIL hasbeen shown to be induced in macrophages by inflammatory stimulisuch as IL-1 and Toll-like receptor (TLR) ligands, and is preferentiallyexpressed in the nucleus. Thus, although lentiviral expressionof I ${kappa}$ B ${epsilon}$ had no effect on the LPS response, other Bcl-3-relatedmolecules may have regulatory roles in NF- ${kappa}$ B activation.
In this study, we identified Bcl-3 as an IL-10-inducible moleculeresponsible for the suppression of LPS-induced TNF- ${alpha}$ production.However, as-yet-unknown mechanisms underlying IL-10-mediatedsuppression of macrophages must exist. Further studies willbe required to fully understand the inhibitory function of IL-10in macrophages, which will certainly be very beneficial forthe clinical treatment of inflammatory bowel diseases.

   Acknowledgements

We thank N. Okita for technical assistance, P. Lee for criticalreading of the manuscript, and E. Horita and M. Hashimoto forsecretarial assistance.

   Footnotes

Submitted April 18, 2003; accepted July 28, 2003.
Prepublished online as Blood First Edition Paper, August 7,2003; DOI 10.1182/blood-2003-04-1228.

Supported by grants from Special Coordination Funds, the Ministryof Education, Culture, Sports, Science, and Technology, andthe Japan Research Foundation for Clinical Pharmacology.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: Shizuo Akira, Department of Host Defense, Research Institute for Microbial Diseases, Osaka University, 3-1 Yamada-oka, Suita Osaka 565-0871, Japan; e-mail: sakira{at}biken.osaka-u.ac.jp.

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  Copyright © 2003 by American Society of Hematology         Online ISSN: 1528-0020





	Copyright © 2003 by American Society of Hematology Online ISSN: 1528-0020

IL-10-inducible Bcl-3 negatively regulates LPS-induced TNF- production in macrophages

IL-10-inducible Bcl-3 negatively regulates LPS-induced TNF- ${alpha}$ production in macrophages