Mitogen-Activated Protein Kinase p38 Controls the Expression and Posttranslational Modification of Tristetraprolin, a Regulator of Tumor Necrosis Factor Alpha mRNA Stability

doi:10.1128/MCB.21.9.6461-6469.2001

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Molecular and Cellular Biology, October 2001, p. 6461-6469, Vol. 21, No. 19
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.9.6461-6469.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Mitogen-Activated Protein Kinase p38 Controls the Expression and Posttranslational Modification of Tristetraprolin, a Regulator of Tumor Necrosis Factor Alpha mRNA Stability

Kamal R. Mahtani, Matthew Brook, Jonathan L. E. Dean, Gareth Sully, Jeremy Saklatvala, and Andrew R. Clark^*

Kennedy Institute of Rheumatology Division, Imperial College School of Medicine, Hammersmith, London W6 8LH, United Kingdom

Received 4 May 2001/Returned for modification 25 June 2001/Accepted 6 July 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Signal transduction pathways regulate gene expression in part by modulating the stability of specific mRNAs. For example,the mitogen-activated protein kinase (MAPK) p38 pathway mediatesstabilization of tumor necrosis factor alpha (TNF- $alpha$ ) mRNA in myeloidcells stimulated with bacterial lipopolysaccharide (LPS). Thezinc finger protein tristetraprolin (TTP) is expressed in responseto LPS and regulates the stability of TNF- $alpha$ mRNA. We show thatstimulation of RAW264.7 mouse macrophages with LPS induces thebinding of TTP to the TNF- $alpha$ 3' untranslated region. The p38 pathwayis required for the induction of TNF- $alpha$ RNA-binding activity andfor the expression of TTP protein and mRNA. Following stimulationwith LPS, TTP is expressed in multiple, differentially phosphorylatedforms. We present evidence that phosphorylation of TTP is mediatedby the p38-regulated kinase MAPKAPK2 (MAPK-activated protein kinase2). Our findings demonstrate a direct link between a specificsignal transduction pathway and a specific RNA-binding protein,both of which are known to regulate TNF- $alpha$ gene expression at aposttranscriptionallevel.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

The cytoplasmic concentration of a given mRNA is a function of its rates of synthesis and degradation. The regulation of mRNAstability is therefore an important means of modulating gene expresssion(9, 16, 20, 36). For example, the rapid and transientinduction of several genes is mediated by transient transcriptionalactivation and transient stabilization of intrinsically unstablemRNAs. Control of mRNA stability is mediated by cis-acting sequenceswithin 5' or 3' untranslated regions (UTRs) or, in some cases,within the coding region. The best-characterized regulatory elementsare the adenosine/uridine-rich elements (AREs) within 3' UTRsof cytokine, growth factor, and proto-oncogene mRNAs, often containingseveral copies of the motif AUUUA (4, 8, 46). OverlappingAUUUA motifs or single copies within a uridine-rich context areable to confer instability upon otherwise stable reporter mRNAs(8, 28, 46, 57). It is assumed that the regulation ofmRNA stability is mediated by trans-acting RNA-binding factorswhich interact with these cis-acting elements. ARE-binding regulatorsof mRNA stability include AUF1 (3, 12, 32, 45, 47,56), HuR (1, 11, 15, 38) and tristetraprolin (TTP)(6, 7, 29, 48).

There is growing evidence that AU-rich elements do not simply confer mRNA instability; rather, they also participate in thedynamic regulation of gene expression in response to externalstimuli. For example, AREs from the 3' UTRs of interleukin-8 (IL-8)or cyclooxygenase-2 mRNA mediate regulation of mRNA stabilityby the mitogen-activated protein kinase (MAPK) p38 pathway (33,34, 55). This pathway is activated by proinflammatory stimulisuch as bacterial lipopolysaccharide (LPS), IL-1, tumor necrosisfactor alpha (TNF- $alpha$ ), and UV light (21, 27, 35, 43). MAPKp38 is phosphorylated and activated by MAPK kinase MKK6 or MKK3(14, 22, 37, 39) and in turn phosphorylates its own substrates,including the kinase MAPK-activated protein kinase 2 (MAPKAPK2)(17, 41). The effects of p38 upon mRNA stability are mediatedby MAPKAPK2 (34, 55), although the relevant substrate(s) ofMAPKAPK2 remain(s) to be identified conclusively. The stabilityof TNF- $alpha$ mRNA is regulated by the p38 pathway in myeloid celllines (2, 42, 53). Its 3' UTR contains an ARE with five(mouse) or six (human) repeats of the AUUUA motif, which is ableto mediate the stabilization of a reporter mRNA by the p38 pathwayin HeLa cells (2). The deletion of this region from the mousegenomic TNF- $alpha$ locus results in elevated basal and LPS-inducedTNF- $alpha$ expression, chronic inflammatory arthritis, and inflammatorybowel disease (25). The stability of the modified TNF- $alpha$ transcriptappears to be increased, and the negative regulation of TNF- $alpha$ expression by a p38 inhibitor isablated.

A similar syndrome of inflammatory arthritis and bowel disease is observed in mice deficient in TTP (otherwise known as Nup475,TIS11, or Zfp36) (49). This is a member of a novel class ofRNA-binding proteins containing two CCCH zinc fingers and threetetraproline (PPPP) motifs and was initially described as beingencoded by an immediate-early mitogen-induced gene (13, 19,31, 52). In macrophages, its expression is also induced byLPS or by TNF- $alpha$ itself (7). The inflammatory syndrome of TTP-nullmice is caused by increased stability of TNF- $alpha$ mRNA and consequentoverexpression of the cytokine (5, 7, 49). In transfectedHEK293 cells, TTP destabilizes a coexpressed TNF- $alpha$ reporter mRNA(29). In extracts from transfected HEK293 cells, binding ofoverexpressed TTP to the TNF- $alpha$ ARE can be detected by electrophoreticmobility shift assays (EMSAs) or by UV cross-linking (7, 29,30). The binding of endogenous TTP protein to this regulatoryelement has not previously beendescribed.

In summary, TTP is believed to destabilize TNF- $alpha$ mRNA in an ARE-dependent manner, forming a negative-feedback loop which functionsto restrain TNF- $alpha$ biosynthesis. TTP is known to exist as a phosphoproteinin vivo and to be phosphorylated by MAPK p42 in vitro (51).However the mechanisms of regulation of TTP expression and functionhave not been characterized. Here, we demonstrate that an LPS-inducibleTNF- $alpha$ ARE-binding factor in mouse RAW264.7 macrophage cells containsTTP. Following stimulation of RAW264.7 cells with LPS, TTP proteinis expressed in several, differentially phosphorylated forms.We present evidence that the p38 signal transduction pathway regulatesboth the expression and the posttranslational modification ofTTP.

	MATERIALS AND METHODS

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Materials. Salmonella enterica serovar Typhimurium LPS was from Sigma-Aldrich Company, Ltd., and was used at a concentration of 10 ngml¹. Sheep anti-rabbit MAPKAPK2 antibody was from Upstate Biotechnology,Inc. The rabbit antiserum to the C-terminal peptide of MAPK p38has been described previously (44). Rabbit antisera were raisedagainst the peptides SAIYESLQSMSHDLSC and CPRRLPIFNRISVSE (BabrahamInstitute, Cambridge, United Kingdom), corresponding to, respectively,the amino-terminal and the carboxy-terminal 16 amino acids ofmurine TTP. Recombinant MAPKAPK2 has been described previously(40). Recombinant human hsp27 was from Bioquote, Ltd. Recombinantprotein phosphatase 2A (PP2A) was prepared by S. Sarsfield atthe Kennedy Institute of Rheumatology. SB203580 was from Calbiochem-Novabiochem,Ltd.

A baculovirus glutathione S-transferase (GST)-MKK6b expression vector was the gift of A. Finch (UCSF Cancer Center), and abacterial GST-p38 $alpha$ expression vector was the gift of S. Lumb (Celltech,Slough, United Kingdom). The mouse TNF- $alpha$ 3' UTR was amplifiedby PCR from a plasmid containing the entire TNF- $alpha$ locus (giftfrom A. Shakov). Human glyceraldehyde-3-phosphate dehydrogenase(GAPDH) and TNF- $alpha$ 3' UTR fragments were amplified by PCR fromgenomic DNA. PCR products were subcloned into pBluescript KS(+)(Stratagene, La Jolla, Calif.), and sequenced. A full-length murineTTP cDNA (I.M.A.G.E. clone 3823873) was obtained from the AmericanType Culture Collection (Manassas, Va.). The coding region wasamplified by PCR, cloned in frame into pGEX2T (Amersham Pharmacia,Little Chalfont, United Kingdom), and sequenced. Sequences ofoligonucleotides used in PCR are available on request from thecorrespondingauthor.

Preparation of cell extracts. Human monocytes were prepared by elutriation from peripheral blood (10) and treated with macrophage colony-stimulating factor(M-CSF) (100 ng/ml) overnight before stimulation with LPS. RAW264.7cells (ATCC TIB-71) were maintained as described previously (2).Cell extracts were prepared as described previously (24). Alloperations were performed at 0 to 4°C. The cells were cooled onice for 5 min, rinsed once with ice-cold phosphate-buffered saline,and harvested by scraping. Then, the cells were pelleted by centrifugationat 600 × g for 10 min and washed once more in phosphate-bufferedsaline. The cells were lysed by the addition of buffer A (20 ×10⁶ cells/100 µl), containing 10 mM HEPES (pH 7.6), 3 mM MgCl₂, 40mM KCl, 2 mM dithiothreitol (DTT), 5% glycerol, 0.5% NP-40, 0.5mM phenylmethylsulfonyl fluoride, 10 µM E64, 4 µg of aprotininper ml, 4 µg of pepstatin per ml, 100 µM sodium vanadate, and1 µM microcystin. After gentle pipetting, the cells were lefton ice for 15 min to swell and burst. Nuclei were removed by centrifugationat 600 × g for 10 min. The supernatant, designated the cytoplasmicextract, was aliquoted and snap-frozen at $-$ 70°C. Protein concentrationswere determined by Bradford proteinassay.

In vitro transcription. RNA probes were prepared as follows. Template DNA was linearized to completion by appropriate restriction digestion and thenpurified by phenol-chloroform extraction and ethanol precipitation.Labeled transcripts were synthesized by in vitro transcriptionof the linearized templates (1 µg of DNA) with 20 U of T7 polymerasein the presence of transcription buffer (Promega), 10 mM DTT,20 U of recombinant RNasin RNase inhibitor (Sigma), 125 µM (each)ATP, GTP, and CTP, 12 µM UTP, and 20 µCi of [ $alpha$ -³²P]UTP (800 Ci/mmol; Amersham Pharmacia) in a final volume of 20µl. Transcription was carried out for 1 h at 37°C and was stoppedby the addition of 10 U of RNase-free DNase (Life Technologies).Reaction mixtures were brought to a volume of 100 µl with distilledwater and extracted once with phenol-chloroform. The riboprobewas then purified on a S200 spin column (Amersham Pharmacia) andstored at $-$ 20°C.

EMSA. RNA band shift assays were performed essentially as described previously (24). The protein extracts were incubated withthe indicated RNA probes in RNA-binding buffer containing 20 mMHEPES (pH 7.6), 3 mM MgCl₂, 40 mM KCl, 2 mM DTT, and 5% glycerolin a total volume of 20 µl. Typically, 10 µg of protein was incubatedwith 400,000 to 500,000 cpm of $alpha$ -³²P-labeled RNA probe, corresponding to approximately 20 fmol ofRNA. The reaction mixture was incubated on ice for 20 min. RNaseT1 and heparin sulfate were added to final concentrations of 50U/ml and 5 mg/ml, respectively, and the reaction was allowed tocontinue for a further 20 min on ice. Quantities (3 µl) of loadingbuffer (90% glycerol, 0.025% bromophenol blue) were added to thesamples, which were then resolved by electrophoresis on a 0.5×Tris-borate-EDTA nondenaturing 4% polyacrylamide gel at 150 Vfor 6 h at 4°C. Gels were dried, autoradiographed, and analyzedusing a phosphorimager (FLA2000;Fuji).

Western blotting. RAW264.7 mouse macrophage extracts were prepared as described above, separated by sodium dodecyl sulfate (SDS)-polyacrylamidegel electrophoresis (PAGE) and electrophoretically transferredto polyvinylidene fluoride microporous membrane (NEN Life Sciences).The membrane was probed with a rabbit polyclonal antiserum raisedagainst the C terminus of mouse TTP and then with a peroxidase-coupledsecondary antibody (Dako). Proteins were detected using an enhancedchemiluminescence system (AmershamPharmacia).

Northern blotting. RNA was purified from RAW264.7 cells using QIAamp RNA blood kits (Qiagen, Crawley, United Kingdom). At each experimental timepoint, 20 µg of RNA was subjected to Northern blotting as describedpreviously (2). The probe was a 1-kb full-length murine TTPcDNA fragment, labeled using ReadyToGo reagents (Amersham Pharmacia).Prior to transfer and blotting of the gel, 18S and 28S ribosomalRNAs were visualized by staining with Sybr green (Molecular Probes)and quantified using a phosphorimager (FLA2000;Fuji).

p38 MAPK and MAPKAPK2 kinase assays. GST-MKK6b was expressed in baculovirus-infected Sf9 cells. GST-TTP, GST-p38 $alpha$ , and His₆-tagged MAPKAPK2 were expressed in Escherichiacoli DH5 $alpha$ . Purification of GST fusion proteins was by glutathioneSepharose affinity chromatography with Amersham Pharmacia reagentsby the corresponding protocols. Purification of His₆-tagged MAPKAPK2was by Ni-nitrilotriacetic acid (NTA) chromatography with Qiagenreagents, using the correspondingprotocols.

Assays using recombinant proteins were performed by mixing the purified kinases with 4 µCi of [ $gamma$ -³²P]ATP in 30 µl of kinase buffer (20 mM HEPES [pH 7.6], 20 mM sodium $beta$ -glycerophosphate, 200 mM NaCl, 10 mM MgCl₂, 10 mM NaF, 2 mMDTT, 0.5 mM EDTA, 0.5 mM EGTA, and 0.1 mM sodium orthovanadate).The quantities of proteins were as follows: for GST-MKK6b, 1 µg;for GST-p38 $alpha$ , 1 µg; for His₆-tagged MAPKAPK2, 2 µg; for GST-TTP,2 µg; and for hsp27, 2 µg.

For the immune-complex kinase assays, RAW264.7 cells were stimulated with LPS for the time periods indicated in the legendsto the figures and the lysates were prepared as described above.Lysate (300 µg) was used in kinase assays that were carried outas described previously (2, 10).

	RESULTS

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One LPS-inducible and five constitutive factors bind to the TNF $alpha$ 3'-UTR. To detect RNA-protein interactions, cytoplasmic protein extracts were prepared from M-CSF-treated, unstimulated, or LPS-stimulatedhuman peripheral blood monocytes. These extracts were used inEMSAs with a radiolabeled RNA probe corresponding to the full-length3' UTR of human TNF- $alpha$ . An LPS-inducible complex of intermediatemobility was readily detected (Fig. 1, lanes 1 and 2). The experimentwas repeated using extracts of untreated or LPS-stimulated RAW264.7mouse macrophage cells, which produce large quantities of TNF- $alpha$ in response to LPS. Five complexes, designated, respectively,C1, C2, C3, C5, and C6, were detected in control extracts (Fig.1, lanes 5 and 6). Complexes C5 and C6 migrated very similarlybut could be distinguished on the basis of competition or mappingexperiments (data not shown). Stimulation of RAW264.7 cells for2 h with LPS (10 ng/ml) led to the formation of an additionalcomplex, C4, of similar mobility to the monocyte LPS-induciblecomplex. The mouse TNF- $alpha$ 3' UTR is 68% identical to the humansequence but 91% identical within the central AU-rich region.Similar patterns of protein-RNA complexes were observed usinga mouse TNF- $alpha$ 3' UTR probe (Fig. 1, lanes 3 and 4), with the exceptionthat C6 was not detected. The apparent induction of C4 variedbetween experiments (with levels in the range of 4- to 10-fold).C4 was not detected if the phosphatase inhibitors sodium orthovanadateand microcystin were omitted from the lysis buffer (data not shown).The cytoplasmic extract of RAW264.7 cells was further fractionatedby high-speed centrifugation at 100,000 × g. C4 was detected inboth the soluble supernatant (S100) and the solubilized pellet(P100) generated by this step (data not shown). The P100 fractioncontains high-molecular-weight complexes, including ribosomes,and is the location of most of the TNF- $alpha$ mRNA in LPS-stimulatedRAW264.7 cells (11). Unfractionated cytoplasmic extracts wereused in all subsequent experiments. Murine and human full-lengthTNF- $alpha$ 3' UTR probes were used interchangeably, since C4 was detectedwith both probes.

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FIG. 1. LPS-inducible binding of a factor to human and mouse TNF- $alpha$ 3' UTRs. M-CSF-treated human peripheral blood monocytes or RAW264.7 cells were stimulated with 10 ng of LPS per ml for 2 h, and then cytoplasmic extracts were prepared. EMSAs were performed using 10 µg of cytoplasmic extract and 20 fmol of ³²P-labeled human or mouse full-length TNF- $alpha$ 3' UTR probes. Lanes 1 and 2, cytoplasmic extract of unstimulated or LPS-stimulated, M-CSF-treated human peripheral blood monocytes probed with ³²P-labeled human full-length TNF- $alpha$ 3' UTR probes; lanes 3 and 4, cytoplasmic extract of unstimulated or LPS-stimulated RAW264.7 cells probed with mouse full-length TNF- $alpha$ 3' UTR probes; lanes 5 and 6, cytoplasmic extract of unstimulated or LPS-stimulated RAW264.7 cells probed with ³²P-labeled human full-length TNF- $alpha$ 3' UTR probes. The well-resolved complexes evident in lanes 5 and 6 are labeled C1 to C6.

Formation of C4 is dependent upon the TNF- $alpha$ ARE. In order to map TNF- $alpha$ mRNA sequences involved in the formation of C4, EMSAs were performed using cytoplasmic extracts of unstimulatedor LPS-stimulated RAW264.7 cells, as well as a series of truncated3' UTR probes, shown schematically in Fig. 2A. A control GAPDH3' UTR probe formed no LPS-inducible complexes (Fig. 2B); therefore,stimulation of RAW264.7 cells with LPS does not simply inducenonspecific RNA-binding activity. A TNF- $alpha$ 3' UTR probe lackingthe ARE (probe 707) failed to generate C4 under these conditions.A probe containing only the ARE (probe 75) generated C4, althoughrelatively weakly. The presence of additional 3' sequences (inprobes 562 and 342) enhanced the formation of C4, yet a 3' UTRprobe lacking the ARE (probe 268) failed to generate C4. A probecontaining all but the last 137 nucleotides of the TNF- $alpha$ 3' UTR(probe 645) generated a relatively weak C4. Therefore the centralAU-rich region of the TNF- $alpha$ 3' UTR is necessary but not sufficientfor optimal formation of an LPS-inducible protein-RNA complex,and additional sequences lying 3' to the ARE contribute to complexformation.

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FIG. 2. Mapping of protein interactions with the TNF- $alpha$ 3' UTR. (A) Schematic of truncated TNF- $alpha$ 3'UTR probes. (B) Results for EMSAs in which 20 fmol of each probe was used with 10 µg of cytoplasmic extract prepared from untreated RAW264.7 cells ( $-$ ) or from cells stimulated for 2 h with 10 ng of LPS per ml (+).

The specificity of protein interactions with the TNF- $alpha$ 3' UTR was further analyzed by competition assays (Fig. 3). C4 wasnot competed by a control GAPDH RNA that was devoid of AUUUA motifs,but it was competed efficiently by an excess of unlabeled full-length(782-nucleotide [nt]) TNF- $alpha$ 3' UTR. The 75-nt TNF- $alpha$ ARE was aless efficient competitor for the formation of C4, and a 707-ntcompetitor lacking the ARE was less efficient still, with residualcomplex remaining detectable in the presence of a 100-fold molarexcess of competitor. This experiment suggests that competitorprobes 75 and 707 bind C4 protein(s) with affinities roughly 1and 2 orders of magnitude lower, respectively, than that of thefull-length TNF- $alpha$ 3' UTR. Again, this indicates that the ARE playsa critical role in the formation of C4 and that sequences lyingoutside the ARE may provide additional sites of protein-RNA interaction.The higher-mobility complexes C5 and/or C6 (not resolved in theseexperiments) were competed similarly by 782- and 707-nt RNAs butnot by the 75-nt ARE, and they therefore presumably involve sequenceslying outside the ARE. Finally, as indicated in Fig. 3B, C4 wasefficiently competed by poly(U) but not by poly(A), -(C), or -(G)RNA [data from poly(C) and poly(G) competitions not shown]. Therefore,in common with several RNA-binding factors thought to be involvedin the regulation of mRNA stability, the proteins present in C4bind specifically to AUUUA repeats or to U-rich RNA.

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FIG. 3. Specificity of protein interactions with the TNF- $alpha$ 3' UTR. EMSAs were performed as described for Fig. 1 and 2, using a full-length human TNF- $alpha$ 3' UTR probe and 10 µg of cytoplasmic extract from LPS-stimulated RAW264.7 cells. Competitor RNA was added to the binding reaction mixtures 20 min prior to the addition of labeled probe. (A) Protein interactions with specific RNA competitors present, as indicated, in 1- to 100-fold molar excess over the probe. (B) Protein interactions with poly(U) or poly(A) RNA present, as indicated, in 1- to 1,000-fold excess (by mass) over the probe.

Induction of C4 is relatively slow and requires de novo gene expression. The kinetics of the induction of C4 by LPS were examined following LPS stimulation of RAW264.7 cells (Fig. 4A). C4 was notdetectable until at least 1 h after the administration of thestimulus but thereafter was sustained for at least 16 h. The relativeslowness of this induction suggested a requirement for de novogene expression, which was assessed using inhibitors of transcriptionand translation (Fig. 4B). In order to minimize exposure of cellsto the toxins actinomycin D and cycloheximide, LPS stimulationwas performed for only 1 h in these experiments; hence, the inductionof C4 was submaximal. The inhibition of either transcription ortranslation blocked the induction of C4, confirming a requirementfor de novo gene expression. In contrast, C3, which contains theRNA-stabilizing protein HuR (11), was upregulated in the cytoplasmfollowing treatment with actinomycin D. Actinomycin D has beenreported to stimulate the translocation of HuR from the nucleusto the cytoplasm (38).

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FIG. 4. LPS-induction of TNF- $alpha$ 3' UTR binding activity requires de novo gene expression. (A) Cytoplasmic extracts prepared from RAW264.7 cells at the indicated times after stimulation with 10 ng of LPS per ml. Ten micrograms of each extract was used in an EMSA with 20 fmol of full-length human TNF- $alpha$ 3' UTR probe. The first lane (marked with a minus sign) contains RNA probe but no protein. (B) RAW264.7 cells preincubated with vehicle, with cycloheximide (CHX [10 µg/ml]) or with actinomycin D (AmD [1 µg/ml]) for 15 min and then stimulated with LPS for 1 h prior to the preparation of cytoplasmic extracts. Ten micrograms of each extract was used in an EMSA with 20 fmol of full-length human TNF- $alpha$ 3' UTR probe.

LPS-induced complex contains TTP. Expression of TTP mRNA is induced following stimulation of mouse macrophages with LPS, peaking roughly 1 h after the administrationof the stimulus and remaining elevated for at least 4 h (7).Overexpressed TTP binds to the TNF- $alpha$ 3' UTR (29, 30), althoughthe regulated binding of endogenous protein to this RNA has notbeen described. To test the hypothesis that C4 contains TTP, antibodieswere raised against the amino and carboxy termini of the mouseprotein. In EMSAs, C4 was induced over a 2-h time course as previouslydescribed (Fig. 5). No supershift of C4 was observed in the presenceof a preimmune serum. In the presence of an immune serum raisedagainst the amino terminus of TTP, a low-mobility, supershiftedcomplex was generated, with a corresponding total depletion ofthe LPS-inducible complex. Identical results were obtained usingan antiserum raised against the carboxy terminus of TTP (datanot shown). The LPS-inducible complex therefore contains TTP.

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FIG. 5. LPS-induced complex contains TTP. Cytoplasmic extracts of LPS-stimulated RAW264.7 cells were prepared, and EMSAs were performed as described for Fig. 4, except that the probe was murine, and 1 µl of preimmune serum or anti-TTP serum was present in each 20-µl binding reaction mixture. The supershifted C4 is indicated with an asterisk.

Induction of TTP gene expression by LPS is dependent upon MAPK p38. The induction of TTP protein following LPS stimulation of RAW264.7 cells was assessed by Western blotting using the amino-terminalTTP antibody described above (Fig. 6A). Unlike other investigators(50), we were unable to detect TTP protein in unstimulated cells.Antigen was first detected 45 min after stimulation, was maximallyinduced by 2 h after stimulation, and remained elevated for atleast 4 h. The expression of TTP was accompanied by an apparentchange in molecular size from a high-mobility form of approximately36 kDa (Fig. 6A, band a) to an intermediate form (Fig. 6A, bandb), and finally to a low-mobility form of approximately 45 kDa(Fig. 6A, band c [also, see Fig. 7]). This alteration of mobilitysuggests a posttranslational modification such as phosphorylation.As the MAPK p38 pathway is known to regulate TNF- $alpha$ mRNA stability,a p38 inhibitor was used to investigate the involvement of thispathway in the expression and modification of TTP. At a concentrationof 1 µM, SB203580 inhibits p38 activity by approximately 90% inLPS-stimulated RAW264.7 cells and has minimal effects upon otherMAPK pathways (2). The preincubation of RAW264.7 cells with1 µM SB203580 almost completely blocked the induction of TTP protein,as assessed by Western blotting (Fig. 6A, right). Correspondingly,1 µM SB203580 inhibited the formation of C4 (Fig. 6B). LPS stimulationstrongly induced the expression of TTP mRNA, and this inductionwas dose-dependently inhibited by SB203580 (Fig. 6C). Therefore,the MAPK p38 pathway is required for the expression of TTP mRNAfollowing stimulation with LPS.

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FIG. 6. MAPK p38 activity is required for the expression of TTP in response to LPS. (A) RAW264.7 cells preincubated for 15 min with vehicle or 1 µM SB203580 and then stimulated with LPS for the times indicated. Cytoplasmic extracts were prepared and separated by SDS-polyacrylamide gel electrophoresis on a 10% gel and then analyzed by Western blotting using an anti-N-terminal TTP antiserum. The letters at the right (a, b, and c) indicate TTP bands of differing mobility. The positions of molecular size markers are indicated at the left of the gel. (B) RAW264.7 cells preincubated for 15 min with vehicle or 0.1 to 10 µM SB203580, as indicated, and then stimulated with 10 ng of LPS per ml for 2 h. Cytoplasmic extracts were prepared and used in EMSAs with 20 fmol of a full-length human TNF- $alpha$ 3' UTR probe. (C) RAW264.7 cells treated as described for panel B, with RNA then extracted and subjected to Northern blotting using a 1-kb TTP cDNA probe. As a loading control, 28S rRNA was visualized by staining of the gel with Sybr green prior to transfer and Northern blotting.

LPS-induced TTP is expressed in several differentially phosphorylated forms. Changes in the electrophoretic mobility of TTP in LPS-stimulated RAW264.7 cells were not observed in a previous study (50).However, in Western blotting, stimulation of NIH 3T3 cells withserum caused a similar shift in the mobility of TTP, which shiftwas ascribed to the phosphorylation of the protein (50, 51).To test whether the LPS-induced shift of TTP was caused by phosphorylation,cytoplasmic extracts of RAW264.7 cells were treated with phosphatasesin the absence or presence of phosphatase inhibitors, and thensubjected to Western blotting (Fig. 7). Treatment of extractswith the serine/threonine phosphatase PP2A resulted in the disappearanceof TTP bands b and c, leaving only the highest-mobility form,and this alteration in mobility was completely blocked by thePP2A inhibitor microcystin. Calf intestinal phosphatase causedan identical shift from bands b and c to a. LPS treatment of RAW264.7cells therefore causes a strong induction of TTP protein, whichis accompanied by its phosphorylation at serine and/or threonineresidues.

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FIG. 7. TTP is differentially phosphorylated following an stimulation with LPS. RAW264.7 cells were stimulated with 10 ng of LPS per ml for 0 to 2 h, as indicated, and then cytoplasmic extracts were prepared. A 200-µg quantity of extract was treated with recombinant PP2A (72 mU) or calf intestinal phosphatase (CIP [50 U]) in the presence or absence of the phosphatase inhibitor microcystin (PI [10 µM]). The extracts were then subjected to Western blotting as described for Fig. 6A. The letters to the right (a, b, and c) indicate TTP bands of differing mobility.

TTP is a substrate of MAPKAPK2. It is difficult to assess the role of the p38 pathway in the phosphorylation of TTP in vivo, as little TTP protein is synthesizedin the presence of a p38 inhibitor. The TTP protein detected underthese conditions appears to be a lower-mobility form, suggestingthat it is phosphorylated. This phosphorylation could be mediatedby a signal transduction pathway other than the p38 cascade orby residual activity of the p38 pathway under these experimentalconditions. Therefore, two approaches were used to investigatethe phosphorylation of TTP via the p38 pathway invitro.

Firstly, the p38 signal transduction pathway was reconstituted using purified recombinant kinases (Fig. 8A). GST-MKK6 wasexpressed in Sf9 cells (using a baculovirus system) and purifiedby glutathione Sepharose affinity chromatography. GST-p38, GST-TTP,and His₆-tagged MAPKAPK2 were expressed in E. coli and purifiedby glutathione Sepharose chromatography or Ni-NTA chromatography.Purified GST-MKK6 was active, GST-p38 was weakly active, and His₆-taggedMAPKAPK2 was inactive (data not shown). No contaminants of thedifferent preparations were detectable by SDS-PAGE or Coomassieblue staining, but the recombinant GST-TTP was extensively degradedin spite of the presence of protease inhibitors during purification.Reconstitution of the cascade was demonstrated by the strong phosphorylationof hsp27 in the presence of MKK6, p38, and MAPKAPK2 (Fig. 8A,lane 9). Activated p38 did not phosphorylate GST-TTP (Fig. 8A,lane 5); however, strong phosphorylation of GST-TTP was observedin the presence of MKK6, p38, and MAPKAPK2 (Fig. 8A, lane 8),suggesting that TTP is a substrate of MAPKAPK2 in vitro. The onlyother combination of kinases which generated detectable phosphorylationof GST-TTP was that of p38 and MAPKAPK2 (Fig. 8A, lane 6), presumablybecause of the basal activity of the unphosphorylated p38 andthe consequent activation of MAPKAPK2 (G. Sully and J. Saklatvala,unpublished observations).

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FIG. 8. TTP is a substrate of MAPKAPK2. (A) Purified recombinant kinases MKK6, p38, and MAPKAPK2 (MK2) were mixed with the substrate GST-TTP (TTP) or hsp27 in the combinations indicated. Phosphorylation reactions were allowed to proceed for 30 min, and then the phosphorylated products were separated by SDS-PAGE and visualized by phosphorimaging. Lane 1, TTP alone; lane 2, MK2 and TTP; lane 3, p38 and TTP; lane 4, MKK6 and TTP; lane 5, MKK, p38, and TTP; lane 6, p38, MK2, and TTP; lane 7, MKK6, MK2, and TTP; lane 8, MKK6, p38, MK2, and TTP; lane 9, MKK6, p38, MK2, and hsp27. (B) RAW264.7 cells were left untreated ( $-$ ) or stimulated with 10 ng of LPS per ml for 2 h (+), and then lysates were prepared, p38 or MAPKAPK2 was immunoprecipitated, and immune-complex kinase assays were performed using hsp27, His₆-tagged MAPKAPK2 or GST-TTP as substrate (Subst). Phosphorylated products were separated by SDS-PAGE and visualized by phosphorimaging. (C) RAW264.7 cells were stimulated with 10 ng of LPS per ml for the times indicated, and then immune-complex assays of MAPKAPK2 activity were performed as described for panel B, using recombinant hsp27 as the substrate. Phosphorylated products were separated by SDS-PAGE and visualized by phosphorimaging.

The ability of mammalian p38 and MAPKAPK2 to phosphorylate TTP was also assessed by means of immune-complex kinase assays.Active kinases were immunoprecipitated from LPS-stimulated RAW264.7cells (Fig. 8B). Activated p38 phosphorylated MAPKAPK2 but notTTP. Activated MAPKAPK2 phosphorylated both hsp27 and TTP, confirmingthat TTP is a substrate for MAPKAPK2 in vitro. Phosphorylationof GST by immunoprecipitated, active kinases was not observed,nor was GST-TTP phosphorylated by control (immunoglobulin class-matchedirrelevant antibody) immunoprecipitates (data not shown). Identicalresults were obtained using activated kinases immunoprecipitatedfrom IL-1-stimulated HeLa cells (data not shown). In both recombinantand immune-complex kinase assay systems, degradation productsof GST-TTP were phosphorylated by MAPKAPK2. Taking these phosphorylationsinto account, TTP appeared to be a MAPKAPK2 substrate almost aseffective as hsp27. Immune-complex kinase assays were performedto determine whether MAPKAPK2 activity overlaps with TTP proteinexpression in LPS-stimulated RAW264.7 cells. MAPKAPK2 activitionwas sustained for at least 2 h after stimulation with LPS (Fig.8C); therefore, active kinase is present during the period inwhich endogenous TTP becomesphosphorylated.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In order to better understand the regulation of mRNA stability by signal transduction pathways we sought to identify RNA-bindingproteins whose behavior is modulated by the p38 cascade. It waspreviously shown that TTP gene expression is induced by LPS stimulationof myeloid cells and that overexpressed TTP is capable of bindingto TNF- $alpha$ mRNA. Here, we demonstrated that endogenous TTP was presentin a TNF- $alpha$ ARE-binding complex induced following the stimulationof RAW264.7 cells with LPS. The induction of TTP mRNA, proteinexpression and RNA-binding activity was blocked by inhibitionof p38. This establishes a direct connection between an RNA-bindingprotein and a signal transduction pathway, both of which are knownto regulate the expression of TNF- $alpha$ at a posttranscriptionallevel.

Following stimulation with LPS, TTP is expressed in a number of differentially phosphorylated forms. It is difficult to establishwhether the p38 pathway is involved in this phosphorylation invivo, as the phosphorylation status of TTP cannot be assessedin the absence of p38 activity. We demonstrated that recombinantTTP is phosphorylated in vitro by MAPKAPK2 immunoprecipitatedfrom LPS-stimulated RAW264.7 cells and that the kinetics of inductionof MAPKAPK2 activity and TTP expression overlap in LPS-stimulatedRAW264.7 cells. It is therefore likely that TTP is a substrateof MAPKAPK2 in vivo, although the functional significance of thisphosphorylation remains unclear. In mouse spleen cells lackingfunctional MAPKAPK2, steady-state TNF- $alpha$ mRNA levels and mRNA stability,measured at a single time point after LPS stimulation, do notappear to be altered (26). The kinetics of TNF- $alpha$ mRNA expressionare altered by deletion of the AU-rich element in mice (25)or by inhibition of the p38 pathway in human monocytes (53).A role for MAPKAPK2 in the regulation of TNF- $alpha$ mRNA stabilitycannot be ruled out without determining both the expression ofTTP and the kinetics of TNF- $alpha$ mRNA induction in mouse cells lackingMAPKAPK2activity.

The accumulation of the hyperphosphorylated form of TTP is relatively slow, peaking approximately 4 h after stimulation withLPS. The dynamic nature of TNF- $alpha$ mRNA stability regulation isillustrated by the decrease in half-life of the mRNA at late timepoints following stimulation with LPS (23). It is an interestingpossibility that phosphorylation of TTP may be required for TNF- $alpha$ mRNA destabilizing activity. In longer exposures of Western blots,small quantities of phosphorylated TTP can be detected as earlyas 1 h after stimulation with LPS, coinciding with the appearanceof binding activity in the EMSA. The EMSA is exquisitely sensitiveand may detect extremely low concentrations of RNA-binding factors.These observations leave open the question of whether phosphorylationis necessary for the interaction of TTP with the TNF- $alpha$ 3' UTR.Our failure to detect TTP-binding activity in extracts preparedwithout phosphatase inhibitors suggests that this may be the case.It is also possible that phosphorylation by MAPKAPK2 influencesother aspects of TTP biology, such as subcellular localization,stability, or interaction with other proteins. TTP may also bephosphorylated by MAPK p42 (51), which is stimulated by LPSstimulation of RAW264.7 cells (18). The principal site of phosphorylationof TTP by p42 has been mapped; however, the functional significanceof this phosphorylation remains to be demonstrated (29, 51).It is possible that phosphorylation of TTP via different MAPKpathways modulates TNF- $alpha$ biosynthesis in response to differentenvironmental cues. Clearly, the role of phosphorylation in theregulation of TTP function merits further investigation. We intendto map the site or sites of phosphoryation by MAPKAPK2 and todevelop an appropriate myeloid cell system in which to test theeffects of phosphorylation sitemutations.

TTP regulates the stability of TNF- $alpha$ , granulocyte-macrophage colony-stimulating factor and IL-3 mRNAs (6, 7, 29, 48),yet the specificity of binding of TTP to AU-rich RNA is not known.In our hands, clustered AUUUA pentamers appeared to be insufficientfor high-affinity binding of TTP, which requires additional sequencesfrom the TNF- $alpha$ 3' UTR. These distal sequences are well conservedbetween eight mammalian species, from human to bottle-nosed dolphin,and include an absolutely conserved AUUUA motif (Fig. 2A). Itis possible that distal 3' sequences provide additional RNA-bindingcontacts for TTP or contribute to secondary structures of theTNF- $alpha$ 3' UTR which favor TTP binding. It has been shown that theTNF- $alpha$ 3' UTR forms higher-order structures which influence itsinteraction with RNA-binding proteins (54). A more detailedanalysis of the RNA-binding specificity of TTP may provide insightsinto its cellularfunction.

The pattern of expression of TTP has not been studied in detail; however, the pathology of the TTP knockout mouse appearsto be restricted to myeloid and lymphoid cells (5, 6, 49).We did not detect the protein in HeLa cells (data not shown),which are able to stabilize ARE-containing transcripts in responseto activation of the p38 pathway (2, 33, 34, 55). Stimulationof RAW264.7 cells with LPS leads to a rapid and p38-dependentstabilization of TNF- $alpha$ mRNA, at a time preceding the appearanceof detectable TTP antigen (2; M. Brook and A. R. Clark, unpublishedobservations). It is thus unlikely that TTP is involved in theactive stabilization of labile mRNAs via the p38 pathway. Theproperties described here and elsewhere are consistent with acell type-specific role in the off-phase of expression of TNF- $alpha$ and other genes. It is intriguing that the p38 pathway stabilizesTNF- $alpha$ mRNA but is also required for the expression of TTP, a TNF- $alpha$ mRNA destabilizing protein. Such a dual function of the p38 pathwaycould represent a mechanism for the restraint of TNF- $alpha$ biosynthesis,in which an LPS-induced signal transduction cascade is intimatelyinvolved in both the on phase and the off phase of TNF- $alpha$ geneexpression. According to this model, the stabilization phase iscontrolled by rapid phosphorylation of a preexisting factor ofunknown identity and the destabilization phase is controlled bythe more gradual synthesis and perhaps phosphorylation of a secondfactor,TTP.

	ACKNOWLEDGMENTS

M.B. and J.L.E.D. contributed equally to thiswork.

K.R.M. was supported by a Ph.D. studentship from the Charing Cross HospitalTrustees.

We are grateful to Cathleen Ciesielski for assistance with purification and culture of human monocytes, to Simon Sarsfieldfor preparation of recombinant PP2A, and to Andrew Finch and SimonLumb for provision ofreagents.

	FOOTNOTES

^* Corresponding author. Mailing address: Kennedy Institute of Rheumatology Division, Imperial College School of Medicine, 1Aspenlea Rd., Hammersmith, London W6 8LH, United Kingdom. Phone:(0044) 208 383 4430. Fax: (0044) 208 383 4499. E-mail: andy.clark{at}ic.ac.uk.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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