Mutant Cells That Do Not Respond to Interleukin-1 (IL-1) Reveal a Novel Role for IL-1 Receptor-Associated Kinase

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Molecular and Cellular Biology, July 1999, p. 4643-4652, Vol. 19, No. 7
0270-7306/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Mutant Cells That Do Not Respond to Interleukin-1 (IL-1) Reveal a Novel Role for IL-1 Receptor-Associated Kinase

Xiaoxia Li,¹ Mairead Commane,¹ Carmel Burns,¹ Kalpa Vithalani,¹ Zhaodan Cao,² and George R. Stark¹^,^*

Department of Molecular Biology, Lerner Research Institute, Cleveland Clinic Foundation, Cleveland, Ohio 44195,¹ and Tularik, Incorporated, South San Francisco, California 94080²

Received 25 November 1998/Returned for modification 28 January 1999/Accepted 22 March 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Mutagenized human 293 cells containing an interleukin-1 (IL-1)-regulated herpes thymidine kinase gene, selected in IL-1 andgancyclovir, have yielded many independent clones that are unresponsiveto IL-1. The four clones analyzed here carry recessive mutationsand represent three complementation groups. Mutant A in complementationgroup I1 lacks IL-1 receptor-associated kinase (IRAK), while themutants in the other two groups are defective in unknown componentsthat function upstream of IRAK. Expression of exogenous IRAK inI1A cells (I1A-IRAK) restores their responsiveness to IL-1. NeitherNF $kappa$ B nor Jun kinase is activated in IL-1-treated I1A cells, butthese responses are restored in I1A-IRAK cells, indicating thatIRAK is required for both. To address the role of the kinase activityof IRAK in IL-1 signaling, its ATP binding site was mutated (K239A),completely abolishing kinase activity. In transfected I1A cells,IRAK-K239A was still phosphorylated upon IL-1 stimulation and,surprisingly, still complemented all the defects in the mutantcells. Therefore, IRAK must be phosphorylated by a different kinase,and phospho-IRAK must play a role in IL-1-mediated signaling thatdoes not require its kinaseactivity.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Interleukin-1 (IL-1), a proinflammatory cytokine produced mainly by macrophages and monocytes in response to inflammation,infection, and other challenges, stimulates a wide spectrum ofresponses, including fever, lymphocyte activation, and leukocyteinfusion to the site of injury or infection (16). IL-1 stimulatesthe expression of several genes by activating the transcriptionfactors NF- $kappa$ B, ATF, and AP-1 (6, 51, 52).

The activation of NF- $kappa$ B has been studied extensively (4, 6, 16). NF- $kappa$ B is kept in the cytoplasm through interactionwith $kappa$ B inhibitory proteins. Following stimulation with cytokines(e.g., IL-1 and tumor necrosis factor alpha [TNF- $alpha$ ]) or otheragents (e.g., lipopolysaccharide, phorbol ester, and double-strandedRNA), I $kappa$ B undergoes phosphorylation on specific serine residuesand is rapidly ubiquitinated and degraded. The liberated NF- $kappa$ Btranslocates to the nucleus, where it activates transcription(5, 63, 66, 69). Recent studies have provided a modelfor how NF- $kappa$ B is activated in response to IL-1 (Fig. 1). First,a complex is formed between the type 1 receptor (IL-1R1) and thereceptor accessory protein (IL-1RAcP) (21, 24, 29, 70).The cytosolic myeloid differentiation protein (MyD88) (36) isthen recruited to the complex, where it functions as an adaptor,recruiting IL-1R-associated kinase (IRAK) in turn (10, 48,71, 75). IRAK is phosphorylated and then leaves the receptorcomplex to interact with TRAF6 (11). IRAK2, an IRAK homolog,was shown to interact with the IL-1R complex, MyD88, and TRAF6in transfected cells, but how IRAK and IRAK2 function in IL-1signaling is not understood (48). Six TRAFs (TNF receptor-associatedfactors) have been described so far (2, 17, 22, 23, 25,31, 49, 58). TRAF2 and TRAF5 have been implicated in activatingNF- $kappa$ B in response to the activation of members of the TNF- $alpha$ receptorsuperfamily (2, 17, 22, 23, 25, 31, 49, 58).The TRAFs interact with NF- $kappa$ B-inducing kinase (NIK), another serine-threoninekinase believed to be a common downstream component in activatingNF- $kappa$ B in response to IL-1, TNF- $alpha$ , and other stimuli (41). TRAFsmight also activate mitogen-activated protein kinase/ERK kinasekinase 1 (MEKK1) (30, 32, 35, 64, 76). Recently, twoI $kappa$ B kinases (IKK $alpha$ and IKK $beta$ ) have been implicated in signal-inducedphosphorylation of the I $kappa$ B proteins (15, 44, 57, 73, 78).Both NIK and MEKK1 activate the IKKs by serine phosphorylation(34, 50). The activated IKKs then phosphorylate I $kappa$ Bs on specificserine residues, resulting in the degradation of I $kappa$ B and activationof NF- $kappa$ B. The IKKs are components of a large complex (15, 44,78). Two additional components, NEMO (NF- $kappa$ B essential modulatoror IKK $gamma$ ) and IKAP are also part of the IKK complex and are requiredfor its formation (12, 59, 74).

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FIG. 1. A model for the IL-1 signaling pathway. See the text for details. PC, phosphatidylcholine.

Recent studies provide evidence for a second signaling pathway parallel to the cascade leading to I $kappa$ B degradation and specificallyrequired for NF- $kappa$ B-dependent transcriptional competency (Fig.1). Protein kinase C, protein kinase A, and phosphatidylinositol-3kinase (PI3K) have been implicated in this pathway, possibly throughthe phosphorylation of the p65 subunit (7, 14, 19, 20,26, 38, 55, 56, 62, 63a, 80, 81). In addition tothe activation of NF- $kappa$ B, IL-1 and TNF- $alpha$ also activate the transcriptionfactors ATF and AP-1, through the activation of Jun kinase (8,45, 51, 52). Signal-induced activation of Jun kinase (Fig.1) may diverge from NF- $kappa$ B activation at the level of the TRAFproteins (64). The activated TRAFs activate MEKK1, which inturn activates Jun kinase (32, 35, 50, 64).

Although much progress has been made in understanding signaling in response to IL-1, many questions remain and the proposedroles of many components in the pathway need to be confirmed genetically.For example, we do not know how NIK is activated in response tothe activation of IRAK and TRAF6, how NIK activates IKK, or howMEKK1 and Jun kinase are activated. To help resolve these andother issues, we have taken a genetic approach to analyze IL-1signaling, generating mutant cell lines lacking specific componentsof the pathway. In the human embryonic kidney cell line 293, anupstream region of the human IL-1-responsive gene E-selectin (alsocalled ELAM-1 [61]) was used to drive the expression of thymidinekinase (TK) and a protein providing resistance to zeocin (Zeo).Negative selection against the expression of TK (39) and positiveselection for the expression of Zeo provide a powerful dual systemfor isolating mutants unresponsive to IL-1 signaling and for complementingthem. With this new selection scheme, we now have isolated fourindependent mutant cell lines that fail to respond to IL-1, inthree complementation groups. While mutants in two of the complementationgroups are defective in unknown components that lie upstream ofIRAK, mutant cell line I1A (I denotes IL-1 unresponsive; 1 denotescomplementation group 1; A denotes independent isolate A) lacksIRAK mRNA and protein. Using I1A cells, we show that IRAK is requiredfor the activation of both NF- $kappa$ B and Jun kinase by IL-1 and thatIRAK functions between MyD88 and TRAF6 in the pathway. Furthermore,we find that the kinase activity of IRAK is not required for IL-1-mediatedsignaling.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Biological reagents and cell culture. Recombinant human IL-1 $beta$ was provided by the National Cancer Institute. Recombinant human TNF- $alpha$ was from Becton Dickinson (Paramus,N.J.). Antibodies recognizing IL-1R, IL-RAcP, MyD88, IRAK, IRAK2,TRAF6, NIK, IKK1, and IKK2 were described elsewhere (11, 24,34, 57, 71). Anti-Jun was from Santa Cruz Biotechnology(Santa Cruz, Calif.). Human embryonic kidney 293 cells transfectedwith human IL-1R (10) were maintained in Dulbecco's modifiedEagle's medium supplemented with 10% fetal calf serum, penicillinG (100 µg/ml), and streptomycin (100 µg/ml).

Recombinant plasmids. The NF- $kappa$ B-dependent E-selectin-luciferase (Luc) reporter gene plasmid pE-selectin-luc was described by Schindler and Baichwal(61). E-selectin-TK and E-selectin-Zeo were constructed by cloningthe E-selectin promoter ( $-$ 730 to +53) in front of the TK cDNA(3) or the Zeo resistance gene (Invitrogen). Mammalian expressionvectors encoding IRAK (driven by the TK promoter), IRAK-K293A(driven by the TK promoter), MyD88 (driven by the cytomegalovirus[CMV] promoter), TRAF6 (driven by the CMV promoter), and the controlexpression plasmid pRK5 were described elsewhere (11).

Mutagenesis and selection. The mutagenesis protocol was modified slightly from the one used by Pellegrini et al. (54). 293-TK/Zeo cells were expandedinto pools of 10⁷ cells each. One day after the cells in each pool had been splitonto two 150-mm-diameter plates, they were treated with ICR191(54) for 3 h, rinsed twice in serum-free medium, and culturedin complete medium. The concentration of ICR191 used was determinedempirically to achieve 50 to 70% killing after each round of mutagenesisand was varied between 1 and 5 µg/ml. After recovery, the cellswere subjected to a total of five rounds of mutagenesis, and cellsin each mutagenized pool were split onto six 150-mm-diameter platesfor selection. To isolate IL-1-unresponsive mutants, the cellswere selected in gancyclovir (5 µg/ml) (Hoffmann-La Roche, Inc.)plus IL-1 (100 U/ml). Fresh gancyclovir and IL-1 were added every3 days for 23 weeks. Clones were picked, expanded in nonselectivemedium, and analyzed by selection with gancyclovir, either alone,with IL-1 and Zeo (100 µg/ml; Invitrogen) or with IL-1.

Transfection and reporter assay. For stable transfections, 2 × 10⁵ cells were seeded onto a 10-cm-diameter plate and cotransfected the following day by thecalcium phosphate method (60) with 10 µg of each expressionconstruct plus 1 µg of pBabePURO. After 48 h, the cells were selectedwith 1 µg of puromycin per ml until clones appeared. For reportergene assays, 2 × 10⁵ cells were transfected by the same procedure with 1 µg of pE-selectin-luc,1 µg of pSV2- $beta$ -gal, and 2,150 ng of each expression construct.After 48 h, the cells were split into three 35-mm-diameter platesand, the next day, stimulated with IL-1 and TNF- $alpha$ for 4 h beforeharvest. Luciferase and $beta$ -galactosidase activities were determinedby using the Promega luciferase assay system and chemiluminescencereagents (Promega),respectively.

Gel shift assay. An NF- $kappa$ B binding site (5'-GAGCAGAGGGAAATTCCGTAACTT-3') from the IP-10 gene (40) was used as a probe. Complementary oligonucleotides,end labeled with polynucleotide kinase (Boehringer Mannheim) and[ $gamma$ -³²P]ATP, were annealed by slow cooling. Approximately 20,000 cpmof probe were used per assay. Cytoplasmic extracts were preparedas described by Kessler et al. (27) and Levy et al. (33).The binding reaction was carried out at room temperature for 20min in a total volume of 20 µl containing 20 mM HEPES buffer (pH7.0), 10 mM KCl, 0.1% Nonidet P-40, 0.5 mM dithiothreitol, 0.25mM phenylmethanesulfonyl fluoride, and 10%glycerol.

Immunoblotting, immunoprecipitation, in vitro kinase, and Northern assays. For immunoprecipitation and immunoblotting, cells at 80% confluency were harvested from 10-cm-diameter dishes, washed oncewith phosphate-buffered saline, and lysed for 10 min at 4°C in0.5 ml of 0.5% Nonidet P-40 lysis buffer containing 50 mM Tris-Cl(pH 8.0), 100 mM NaCl, 10% glycerol, 0.1 mM EDTA, 20 mM sodiumfluoride, 1 mM sodium orthovanadate, 1 mM dithiothreitol, 0.4mM phenylmethanesulfonyl fluoride, aprotinin (3 µg/ml), pepstatin(2 µg/ml), and leupeptin (1 µg/ml). Cellular debris was removedby centrifugation at 10,000 × g for 5 min. For immunoblotting,cell extracts were fractionated by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) and transferred to a nitrocellulosemembrane. Immunoblot analysis was performed with rabbit polyclonalantibodies, visualized with horseradish peroxidase-coupled goatanti-rabbit immunoglobulin, using the Amersham ECL (enhanced chemiluminescenceWestern blotting detection system. For immunoprecipitation andin vitro kinase assays, cell extracts were incubated with 1 µlof the polyclonal antibody for 2 h and then incubated with 50µl of protein A-Sepharose beads for 1 h. The beads were washedthree times with lysis buffer and once with kinase reaction buffer(20 mM HEPES [pH 7.0], 20 mM MgCl₂). In vitro kinase reactionswere performed in 50 µl of buffer containing 20 mM HEPES (pH 7.0),20 mM MgCl₂, 1 mM ATP, and 10 µCi of [ $gamma$ -³²P]ATP at 30°C for 30 min. For the Jun kinase assay, 2 µg of glutathioneS-transferase-Jun (Alexis Corporation) was included in the reaction.Samples were analyzed by SDS-PAGE (10% gel) followed byautoradiography.

For Northern analysis, total RNA was isolated by using the TRIzol reagent (GIBCO BRL). Appropriate gene-specific probes weremade with a random priming kit (Amersham). Transfers to the positivelycharged nylon membrane Hybond-N were performed according to theprocedure provided byAmersham.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Attempts to isolate mutants by using established strategies and development of a novel approach. Mutant clones defective in the induction of cell surface marker CD2 or CD4, or both, driven by an IL-1-responsive promoter,were obtained by cell sorting but were too unstable to work with.They reverted to wild type after being cultured for three to fourpassages. To allow lethal selection with promoters that drivesignificant basal expression of marker genes, a new double drugselection was set up, with the Zeo and herpesvirus TK genes. Cellsdie in gancyclovir when TK is expressed, and cells that expressthe Zeo gene survive exposure to zeocin. The previously used negativeselection with 6-thioguanine in cells carrying a signal-regulatedgpt gene (13, 65, 68) works well only when the promotergives very low basal expression (for example, the interferon-responsive6-16 promoter). A major advantage of gancyclovir-TK selectionover 6-thioguanine-gpt selection is that the concentration ofgancyclovir can be manipulated to allow cells with a low levelof constitutive TK expression to survive but still to kill cellswith an induced level of expression. Also, since gancyclovir isa poor substrate for mammalian TK, the selection does not requirea TK-null cellline.

To construct plasmids in which TK and Zeo can be induced by IL-1 or TNF- $alpha$ , an upstream fragment ( $-$ 730 to +52) of the E-selectingene (Fig. 2A) was cloned upstream of TK and Zeo. The E-selectinpromoter contains binding sites for both NF- $kappa$ B and ATF, and mutationof either site abolishes the IL-1-induced promoter activity (72).The E-selectin-TK and E-selectin-Zeo constructs were cotransfectedinto 293 cells, in which the E-selectin promoter has a low basalactivity and a high induced activity (Fig. 3B). The transfectedcells were selected for clones that survive in gancyclovir, diecompletely in gancyclovir plus IL-1, die in Zeo, and survive inZeo plus IL-1 (Fig. 2B). The clone used for mutagenesis is called293-TK/Zeo.

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FIG. 2. Double drug selection with TK and Zeo under control of the E-selectin promoter. (A) E-selectin-TK and E-selectin-Zeo. An upstream fragment of the E-selectin gene ( $-$ 730 to +52), containing one ATF and three NF- $kappa$ B binding sites and a TATA box, was cloned in front of the TK cDNA or the Zeo gene. (B) Drug selection. E-selectin-TK and E-selectin-Zeo were cotransfected into 293 cells, and the transfected cells were selected in Zeo plus IL-1. Individual clones were assayed for survival in gancyclovir (GCV), death in gancyclovir plus IL-1, death in Zeo, and survival in Zeo plus IL-1. One such clone was expanded and subjected to five rounds of mutagenesis. IL-1-unresponsive mutants were isolated by selecting the mutagenized pools in gancyclovir plus IL-1. Putative mutants were then tested for survival in gancyclovir and gancyclovir plus IL-1 and for death in Zeo and Zeo plus IL-1.

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FIG. 3. Analyses of IL-1-unresponsive mutants. (A) NF- $kappa$ B gel shift assay. Cell extracts were made from 293-TK/Zeo cells (WT [wild type]) and the IL-1-unresponsive mutants treated for 15 min with IL-1 (100 U/ml) or TNF- $alpha$ (20 ng/ml) or untreat. The NF- $kappa$ B binding site from the IP-10 gene was used as a probe. The two bands in the gel shift assay are due mainly to p50-p65 heterodimers (bottom) and p65-p65 homodimers (top) (63a). (B) Luciferase reporter assay. E-selectin-Luc (1 µg/10-cm-diameter plate) was transiently transfected into 293-TK/Zeo cells (WT) and the IL-1-unresponsive mutants. Thirty-six hours later, the cells were either left untreated or stimulated for 4 h more with IL-1 (100 U/ml; closed bars) or TNF- $alpha$ (20 ng/ml; hatched bars). Luciferase activities were normalized to $beta$ -galactosidase. Data are presented as the fold induction of luciferase activity in the treated cells. Shown are the averages and standard deviations from three independent experiments. (C) Northern analysis of IL-8 gene expression. Total RNAs were made from 293-TK/Zeo cells (WT) and the IL-1-unresponsive mutants treated for 6 h with IL-1 (100 U/ml) or TNF- $alpha$ (20 ng/ml) or untreated. Human IL-8 cDNA was used as a probe, and the signals were normalized after reprobing with a glyceraldehyde-3-phosphate dehydrogenase (GAPDH) cDNA.

Isolation of IL-1-unresponsive mutants. For mutagenesis, 293-TK/Zeo cells were expanded to pools of 10⁷ cells each, subjected to five rounds of mutagenesis with ICR191(an intercalating agent that induces frameshift mutations), andselected in gancyclovir plus IL-1. Clones picked from each ofsix separately mutagenized pools (Table 1) were expanded in nonselectivemedium and analyzed by drug selection. Over 90% of the clonessurvived in gancyclovir plus IL-1 and died in Zeo plus IL-1. Tento thirty percent of the clones from each of four pools had lostthe ability to activate NF- $kappa$ B in a gel shift assay after IL-1treatment (Table 1, pools 1 to 4). Clones from the other twopools still retained IL-1-induced NF- $kappa$ B activation and thus eitherare defective in IL-1-mediated pathways that do not affect theliberation of NF- $kappa$ B from I $kappa$ B or are cis mutants in which the TKconstruct is inactivated (Table 1, pools 5 and 6). Since clonesfrom the same mutagenized pool may be siblings, only one mutantclone from each pool was used for further study. The mutant cloneswere named according to their complementation groups as describedbelow. IL-1 failed to activate NF- $kappa$ B substantially in all fourmutant clones (Fig. 3A and data not shown for clone I2B). An E-selectin-drivenluciferase plasmid was transfected transiently into each mutantcell line. Both IL-1 and TNF- $alpha$ induced luciferase in wild-type(293-TK/Zeo) cells (Fig. 3B). The response to IL-1 was absentin all four mutant clones, while their TNF- $alpha$ response was intact,revealing that these four clones are specifically defective inIL-1 signaling. We also studied the endogenous IL-1-responsiveIL-8 gene, which is induced by both IL-1 and TNF- $alpha$ in wild-type293-TK/Zeo cells. In the mutant cells, IL-1-induced IL-8 geneexpression was reduced greatly, while the response to TNF- $alpha$ wasintact (Fig. 3C). In Fig. 3C, clones I1A and I2A show an enhancedTNF response compared to wild-type or I3A cells. However, thisdifference was not observed consistently.

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TABLE 1. Clones that do not respond to IL-1

Dominance and complementation. Puromycin-resistant populations were made from each of the four mutant clones and fused with hygromycin-resistant 293-TK/Zeocells. After selection with both drugs, the IL-1-induced activationof NF- $kappa$ B was restored in all of the heterokaryons (Fig. 4, lanes1 to 6 and 10 to 12, and data not shown), indicating that themutations are all recessive. To assign complementation groups,puromycin-resistant and hygromycin-resistant populations fromeach mutant clone were fused pairwise, and IL-1-induced NF- $kappa$ Bactivation was examined. Clones I2A and I2B are in the same complementationgroup since IL-1-induced NF $kappa$ B activation was not restored in theheterokaryons (data not shown). I1A and I3A are in different complementationgroups (Fig. 4, lanes 4 to 9 and 13 to 15, and data not shown).The isolation of mutants in three different complementation groupsstrongly suggests that these cell lines are defective in differentsignaling components.

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FIG. 4. NF- $kappa$ B gel shift assay for dominance and complementation. Extracts were made from 293-TK/Zeo cells (WT [wild type]), clones I1A and I2A, and heterokaryons WT/I1A and I1A/I2A, treated for 15 min with IL-1 (100 U/ml) or TNF- $alpha$ (20 ng/ml) or untreated. The NF- $kappa$ B binding site from the IP-10 gene was used as a probe.

Loss of IRAK accounts for the phenotype of I1A cells. All four mutant clones were assayed with antibodies against the known signaling components IL-1R1, IL-1RAcP, MyD88, IRAK,IRAK2, TRAF6, NIK, IKK1, and IKK2. I1A cells lack IRAK (Fig. 5A,lane 2), a serine-threonine kinase recruited to the IL-1R complexupon IL-1 stimulation. This result was confirmed by Northern analysis,showing that IRAK mRNA is also absent in I1A cells (Fig. 5B, lanes3 and 4). No other known component was missing in I1A cells, andno known component was missing in the other three mutant clones(data not shown). To determine whether IRAK can complement thedefect in I1A cells, increasing amounts of TK-driven IRAK cDNAwere cotransfected transiently with E-selectin-Luc into I1A cells.With an optimal amount of DNA (50 to 100 ng), IL-1-induced expressionof luciferase was restored in the IRAK-transfected I1A cells (Fig.6A and B), whereas expression was not observed in I1A cells transfectedwith vector DNA (data not shown). TK-IRAK was also transfectedstably into I1A cells (Fig. 6C). Although constitutive activationof NF- $kappa$ B was observed in these I1A-IRAK cells, IL-1 induces theactivation of NF- $kappa$ B further (data not shown). Taken together,the results show that IRAK can complement the defect in I1A cells,indicating that their failure to respond to IL-1 is likely duesolely to the lack of this protein.

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FIG. 5. Clone I1A lacks IRAK. (A) Analysis of the IRAK protein. Extracts were made from 293-TK/Zeo (WT [wild type]) cells and from the IL-1-unresponsive mutants. Aliquots were analyzed with anti-IRAK after Western transfer. The same blot was probed with anti-IL-1R1. (B) Analysis of IRAK and IRAK2 mRNAs. Total RNA made from 293-TK/Zeo cells (WT) and mutant I1A was analyzed by the Northern procedure with IRAK or IRAK2 cDNA as the probe.

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FIG. 6. Analysis of I1A cells complemented with IRAK or IRAK-K239A. (A) Cells were cotransfected transiently with E-selectin-Luc and increasing amounts of a TK promoter-driven IRAK expression vector or TK promoter-driven IRAK-K239A expression vector. Thirty-six hours later, the cells were either left untreated or stimulated for 4 h more with IL-1 (100 U/ml) before harvest. Luciferase activities were normalized to $beta$ -galactosidase. Data are presented as fold induction of luciferase activity in the treated cells. The experiments were repeated four times. Shown are the data from a typical experiment. (B) Western analysis with anti-IRAK of extracts from I1A cells transiently transfected with increasing amounts of IRAK or IRAK-K239A. (C) Western analysis of extracts from 293-TK/Zeo (WT [wild type]), I1A, or I1A cells stably transfected with IRAK or IRAK-K239A.

Functions of IRAK in IL-1 signaling. IL-1 stimulation also leads to the activation of Jun kinase, and previous studies have suggested that IRAK may be involved(57). Both IL-1 and UV treatment activated Jun kinase in wild-type293-TK/Zeo cells (Fig. 7A, lanes 1 to 3), and the activation ofJun kinase induced by IL-1 but not by UV treatment was abolishedin I1A cells (Fig. 7A, lanes 4 and 5). The IL-1-induced activationof Jun kinase was restored in I1A-IRAK cells (Fig. 7A, lanes 7to 9). Taken together, these results show that IRAK is requiredfor IL-1-induced but not UV-induced activation of Jun kinase.

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FIG. 7. IL-1-induced activation of Jun kinase in mutant cells. Immunoprecipitates were prepared from cell extracts with anti-Jun kinase, followed by an in vitro kinase assay. (A) Analysis of extracts from 293-TK/Zeo (WT [wild type]) cells and I1A cells, untransfected or stably transfected with IRAK or IRAK-K239A, untreated, stimulated with IL-1, or treated with UV (40 J/m²). (B) Analysis of extracts from clones I1A, I2A, and I3A untreated, stimulated with IL-1, or treated with UV (40 J/m²).

Previous studies have shown that ectopic expression of MyD88 induces NF- $kappa$ B activation strongly even in the absence of IL-1(48, 71). When MyD88 was cotransfected with E-selectin-Lucinto wild-type 293-TK/Zeo cells, promoter activity was dramaticallyincreased compared to cells cotransfected with the vector control,but constitutive activation of the E-selectin promoter in responseto overexpression of MyD88 was not observed in I1A cells, whichlack IRAK (Fig. 8). In I1A cells stably transfected with IRAK,the effect of MyD88 was restored (Fig. 8). We conclude that MyD88cannot interact with downstream components in the pathway in theabsence of IRAK. Overexpression of TRAF6 can also constitutivelyinduce NF- $kappa$ B activation (11). When TRAF6 was cotransfected withE-selectin-Luc into either wild-type 293-TK/Zeo cells or I1A cells,promoter activity was increased in the absence of IL-1 (Fig. 8).Therefore, TRAF6 interacts with components of the signaling pathwaydownstream of IRAK, as previously proposed by Cao et al. (11).Taken together, our results confirm that IRAK functions betweenMyD88 and TRAF6.

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FIG. 8. Constitutive stimulation of signaling by MyD88 or TRAF6 in I1A cells. 293-TK/Zeo (WT [wild type]) cells and I1A cells stably transfected with IRAK or IRAK-K239A were cotransfected transiently with E-selectin-Luc, with a vector control, or with a MyD88 or TRAF6 expression vector. Luciferase activities were normalized to $beta$ -galactosidase. Data are presented as fold induction of luciferase in cells transfected with MyD88 (solid bars) or TRAF6. Shown are the averages and standard deviations from three independent experiments.

The kinase activity of IRAK is not required for its function in IL-1 signaling. IRAK, a serine-threonine kinase, is recruited to the receptor complex upon IL-1 stimulation, where it becomes highly phosphorylated(10). Phosphorylated IRAK then leaves the receptor to interactwith TRAF6 and propagate the signal (11). The phosphorylationsites of IRAK have not yet been identified, and it is also notclear whether IRAK phosphorylates itself or is phosphorylatedby another kinase. To examine whether the kinase activity of IRAKis required for signaling, its ATP binding site was inactivatedby changing the lysine at amino acid 239 to alanine (K239A mutation).IRAK-K239A, driven by the TK promoter, was transfected into I1Acells (I1A-IRAK-K239A). As expected, the K239A mutation inactivatesthe kinase activity of IRAK (Fig. 9). Surprisingly, however, IRAK-K239Afunctions about as well as wild-type IRAK in vivo. The luciferasereporter assay showed that activation of the E-selectin promoterby IL-1 was restored in I1A-IRAK-K239A cells as well as in I1A-IRAKcells (Fig. 6A and B). The K239A mutation in IRAK does not affectits ability to restore the IL-1-induced activation of NF- $kappa$ B (datanot shown) or the activation of Jun kinase in I1A cells (Fig.7A, lanes 10 to 12). Finally, the constitutive activation of E-selectin-Lucin response to overexpression of MyD88 was also restored in I1A-IRAK-K239Acells (Fig. 8), revealing that the kinase activity of IRAK isnot required for its interaction with MyD88 either.

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FIG. 9. IRAK kinase assay. Cell extracts were made from 293-TK/Zeo (WT [wild type]), I1A, and I1A stably transfected with IRAK or IRAK-K239A. Immunoprecipitates were prepared with anti-IRAK, followed by an in vitro kinase assay. Short and long exposures are presented. The immunoprecipitated samples were also analyzed with anti-IRAK (bottom panel).

Phosphorylation of IRAK by another kinase. Previous work has shown that the majority of IRAK translocates to the IL-1R complex following IL-1 stimulation, where it becomesmultiply phosphorylated and subsequently degraded by proteosomes(75). We observed the same phenomenon in 293-TK/Zeo cells. IRAKwas phosphorylated and degraded upon IL-1 treatment (Fig. 10A,lanes 2 to 5). Some of the upper bands appearing after IL-1 stimulationmay represent ubiquitinated forms of IRAK (9a). IL-1R was notdegraded upon IL-1 stimulation in 293-TK/Zeo cells (Fig. 10A, bottom).In stably transfected I1A cells, IRAK was phosphorylated and ubiquitinatedbefore IL-1 stimulation, probably due to its overexpression (Fig.10B, lane 1, and data not shown). However, IRAK was still degradedafter IL-1 treatment, possibly due to further phosphorylationafter stimulation (Fig. 10B, lanes 2 to 5). The loss of severalshifted IRAK bands following treatment with calf intestinal phosphataseconfirmed that they are phosphorylated forms (Fig. 10D, lanes 3and 4). IRAK-K239A was not phosphorylated or ubiquitinated beforestimulation (Fig. 10B, lane 6) but was still phosphorylated, ubiquitinated,and degraded after IL-1 treatment (Fig. 10B, lanes 7 to 10). Thephosphorylation of IRAK-K239A following IL-1 stimulation was alsoconfirmed by the loss of several phosphorylated bands of IRAK-K239Afollowing phosphatase treatment (Fig. 10E, lanes 4 to 6). SinceIRAK-K239A cannot phosphorylate itself (Fig. 9), its phosphorylationin response to IL-1 must be due to another kinase. It is possiblethat IRAK is phosphorylated both by itself and by a differentkinase upon IL-1 treatment. Since IRAK-K239A complements I1A cellsjust as well as wild-type IRAK (Fig. 6, 7A, and 8 and data notshown), it is likely that the phosphorylation of IRAK by a differentkinase plays a more important role in signaling than does IRAKautophosphorylation. Further work is needed to determine the residuesmodified in each situation.

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FIG. 10. Western analysis of IRAK as a function of time after stimulation with IL-1. Shown are results for wild-type 293TK/Zeo (WT) cells and I3A cells (A), I1A cells transfected with IRAK or IRAK-K239A (B), and I1A/I3A heterokaryons (C), either untreated or treated with IL-1. Cell extracts were analyzed by the Western procedure with anti-IRAK. P-IRAK, phosphorylated IRAK; U-IRAK, ubiquitinated IRAK. The top portions of panels A and B are short exposures, and the bottom portions are long exposures. The same transfers were probed with anti-IL-1R1 to control for loading. (D and E) Extracts of I1A cells transfected with IRAK or IRAK-K239A, with or without IL-1 stimulation, were either untreated or treated with calf intestinal phosphatase (CIP).

IRAK2 can also complement mutant I1A cells. IRAK2, identified as a homologue of IRAK, has also been implicated in IL-1 signaling (48). Although IRAK2 interacts withthe IL-1R complex and forms complexes with MyD88 and TRAF6 (48),its exact role in signaling is not clear. IRAK2 was expressedin both wild-type and IRAK-deficient I1A cells, but its mRNA wasat a much lower level than the mRNA for IRAK (Fig. 5B). Westernanalysis indicated that the level of IRAK2 protein is also relativelylow in 293-TK/Zeo cells (data not shown). IRAK2 restored responsivenessto IL-1 when overexpressed in IRAK-deficient I1A cells (Fig. 11).Constitutive activation of the pathway in response to overexpressionof MyD88 was also restored in I1A cells transfected with IRAK2(Fig. 11), showing that MyD88 can also signal through IRAK2.

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FIG. 11. Complementation of I1A cells with IRAK2. E-selectin-Luc was cotransfected transiently with control vector, MyD88, or TRAF6 into I1A cells stably transfected with CMV-IRAK2 (I1A-IRAK2 cells). The I1A-IRAK2 cells transfected with E-selectin-Luc and the control vector were treated with IL-1 (100 U/ml, 4 h). Data are presented as the fold induction of luciferase activity in IL-1-treated or untreated cells transfected with MyD88 or TRAF6 compared to cells transfected with the control vector. Shown are the averages and standard deviations from three independent experiments.

Mutants in complementation groups I2 and I3 are defective in components upstream of IRAK. The IL-1-induced activation of NF- $kappa$ B is greatly reduced in mutant clones I2A and I3A (Fig. 3A). Western analyses of IL-1R,IL-1RAcP, MyD88, IRAK, IRAK2, TRAF6, NIK, IKK1, and IKK2 revealedthat none of these components is missing in any of the three mutantclones (data not shown). IL-1-induced Jun kinase activation wascompletely absent in all three clones, whereas UV-induced Junkinase activation was normal (Fig. 7B). Therefore, all three clonesare defective in components required for the activation of bothNF- $kappa$ B and Jun kinase. In response to IL-1, IRAK is phosphorylated,ubiquitinated, and degraded in wild-type cells (Fig. 10A, lanes1 to 5). Interestingly, IRAK was not phosphorylated, ubiquitinated,or degraded upon IL-1 stimulation in any of the three mutants.(Data for clone I3A are presented in Fig. 10A, lanes 6 to 10; datafor clones I2A are not shown.) However, IRAK was phosphorylatedand degraded in the I1A/I3A heterokaryons, suggesting that theIRAK in I3A cells is intact (Fig. 10C). These results suggest thatthe defects in these mutant clones are upstream of IRAK, a conclusionfurther supported by the results of an experiment in which MyD88was cotransfected with E-selectin-Luc into the mutant clones.The E-selectin promoter was activated constitutively in all threemutants (data not shown). Therefore, the defects in these mutantsare upstream of both IRAK andMyD88.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Roles of IRAK and IRAK2 in IL-1 signaling. Although biochemical studies have yielded important information concerning the IL-1 signaling pathway (10, 11, 48, 70,71, 75), genetic information is still largely lacking. Wehave now obtained the IRAK-null cell line I1A, allowing a detailedevaluation of the role of this protein in the IL-1 response. IRAKwas cloned originally through its association with IL-1R (10).Upon IL-1 stimulation, IRAK associates rapidly with the receptorcomplex and becomes highly phosphorylated (10). Our work nowshows that the IL-1-induced activation of both NF- $kappa$ B and Jun kinaseis abolished in IRAK-deficient I1A cells, providing strong geneticevidence that IRAK indeed is essential for these two pathways.How IRAK is activated upon IL-1 stimulation and how it functionsremain to be determined. Recently, IRAK has also been implicatedin the IL-18 and Toll-dependent signaling pathways (1, 28,43, 47). How IRAK is activated in these pathways and the roleplayed by IRAK also need to beelucidated.

MyD88 coprecipitates with IL-1R1, IL-1RAcP, and IRAK and has a high affinity for hypophosphorylated IRAK, suggesting thatIRAK might be recruited to the receptor complex through an interactioninvolving MyD88 (71). The ectopic expression of MyD88 stronglyinduces NF- $kappa$ B activation in wild-type cells (48, 71). We nowfind that the constitutive activity of MyD88 is lost in the absenceof IRAK, suggesting that MyD88 cannot signal to downstream componentsof the pathway without IRAK. MyD88 may interact with IRAK directlyand may indeed function as an adaptor to recruit IRAK to the receptorcomplex.

IRAK leaves the receptor after activation and forms a complex with TRAF6 (11). Overexpression of TRAF6 can also lead toconstitutive activation of NF- $kappa$ B (11). We find that the constitutiveactivation of NF- $kappa$ B by TRAF6 is the same in IRAK-deficient I1Acells as in wild-type controls, confirming that TRAF6 can interactwith downstream components of the pathway in the absence of IRAK.An important downstream target for TRAFs is likely to be NIK,a common mediator in the activation of NF- $kappa$ B in response to IL-1,TNF- $alpha$ , and other stimuli (41). As shown in Fig. 1, TRAFs mayalso activate MEKK1, which in turn activates Jun kinase and IKK(30, 32, 35, 50, 64, 76). However, it is not yet clearhow the TRAFs are activated. Since our study shows that the overexpressionof TRAF6 can activate NF- $kappa$ B constitutively even in the absenceof IRAK, IRAK might activate TRAF6 simply by facilitating itsaggregation.

The kinase activity of IRAK is not necessary for it to function in IL-1 signaling. Although this result is somewhat surprising,it was not totally unexpected since a similar observation hasbeen made for receptor interacting protein, a serine-threoninekinase in TNF- $alpha$ signaling (67). The ability of mutant kinaseswithout catalytic activity still to function has also been observedin interferon signaling. Although the receptor-associated proteintyrosine kinase JAK1 is required for the gamma interferon (IFN- $gamma$ )response, a kinase-dead mutant of JAK1 can restore IFN- $gamma$ -inducedgene expression but not the antiviral state to a JAK1-null mutantcell line (9). Also, although Tyk2 is required for the IFN- $alpha$ response, a kinase-dead mutant of Tyk2 can restore IFN- $alpha$ -inducedgene expression in Tyk2-null cells (18).

It is not known whether IRAK is phosphorylated at the receptor by itself, another kinase, or both. Using IRAK-deficient cells,we show that a kinase-dead mutant of IRAK can still be phosphorylatedupon IL-1 stimulation (Fig. 10B and E), revealing that anotherkinase must be capable of phosphorylating IRAK at least in part.Although the mechanistic role of IRAK phosphorylation is not clear,its state of phosphorylation does affect its affinity for MyD88(71). The high affinity of MyD88 for underphosphorylated IRAKis consistent with its role in recruiting IRAK to the receptor,and the inability of MyD88 to bind to phosphorylated IRAK mayexplain how IRAK leaves the receptor complex afteractivation.

IRAK2, a homolog of IRAK lacking apparent kinase activity, may also be involved in IL-1 signaling since it interacts withIL-1R and forms a complex with MyD88 and TRAF6 (48). The levelof IRAK2 expression in 293 cells seems to be much lower than thatof IRAK. Since overexpression of IRAK2 restores IL-1 responsivenessto I1A cells (Fig. 11), it is possible that IRAK and IRAK2 aredifferentially expressed functional alternatives, explaining thesmall residual IL-1 response that we sometimes observe in IRAK-deficientcells since these cells have a small amount of IRAK2. However,we still cannot exclude the possibility that IRAK and IRAK2 havesomewhat differentfunctions.

Novel components in IL-1 signaling. Analyses of three mutant cell lines in complementation groups I2 and I3 show that in response to IL-1, that the activationof both NF $kappa$ B and Jun kinase is abolished, that IRAK is neitherphosphorylated nor degraded, and that overexpressed MyD88 canstill activate NF- $kappa$ B constitutively, probably by interacting withIRAK. These results strongly suggest that these mutants are likelydefective in components upstream of IRAK. However, the known upstreamcomponents IL-1R1, IL-1RAcP, and MyD88 are all expressed normallyin all three mutant cell lines. ICR191 is a frameshift mutagen,and we have found that it rarely leads to mutations that allowthe protein to be expressed; almost always, both the target mRNAand protein are missing (unpublished results). Therefore, it isvery likely that mutants in complementation groups I2 and I3 aredefective in components of the IL-1 signaling pathway that havenot yet been identified. One possibility is an additional receptorcomponent. IL-1R is a member of a family that includes IL-1Rrp2,T1/ST2, and rsc786/TIL (37, 42, 46, 53, 77). MyD88,also a member of this family, was only recently found to playa role in IL-1 signaling (71). It is also possible that themutation in complementation group I2 or I3 affects the kinasethat phosphorylates IRAK-K239A. In such a mutant, IRAK would stillbe recruited to the receptor complex but not phosphorylated. Complementationof these mutant cell lines with expression libraries will advanceour understanding of IL-1 signalingconsiderably.

IL-1-unresponsive mutants not defective in NF- $kappa$ B activation. Since the E-selectin promoter contains binding sites for both NF- $kappa$ B and ATF, and since mutation of either site abolishes IL-1-inducedpromoter activity, one would expect to isolate IL-1-unresponsivemutant clones that are defective in activating NF- $kappa$ B or ATF, orboth. Mutants defective in both pathways would most likely havedefects in upstream components, whereas mutants defective onlyin one pathway would most likely have defects in downstream components.Furthermore, it has been shown recently that the liberation ofNF- $kappa$ B from I $kappa$ B and its translocation into the nucleus may notbe sufficient for the full activation of NF- $kappa$ B. The transcriptionalactivity of NF- $kappa$ B is also regulated by I $kappa$ B-associated proteinkinase A, leading to phosphorylation of the NF- $kappa$ B p65 subunitand to its binding to the transcriptional coactivator CBP/p300(Fig. 1 and references 20, 55, 79, and 80). Phosphatidylcholine-specificphospholipase C and protein kinase C have also been implicatedin regulating the transcriptional activity of NF- $kappa$ B (7, 14,19, 26, 38, 62, 81). Recently, Sizemore and Stark (63b)have found that inhibitors of PI3K block NF $kappa$ B-dependent transcriptionby blocking the IL-1-stimulated phosphorylation of NF- $kappa$ B but donot affect the IL-1-stimulated degradation of I $kappa$ B $alpha$ , the nucleartranslocation of NF- $kappa$ B, or the ability of NF- $kappa$ B to bind to DNA.Therefore, mutant clones in which NF- $kappa$ B is activated for DNA bindingmay still be defective in activating transcription through thephosphorylation of NF- $kappa$ B itself. Only 10 to 30% of the clonesselected from each of four mutagenized pools have lost the abilityto activate NF- $kappa$ B after IL-1 treatment; the remaining clones stillinduce the DNA binding activity of NF- $kappa$ B (as shown by gel shiftanalysis), and some of these may be defective in other IL-1-mediatedpathways.

Current state of obtaining recessive mammalian cell mutants. In this report, we have described a novel genetic approach to generate mutant cell lines defective in specific componentsof IL-1 signaling, employing a double drug selection with theZeo and herpesvirus TK genes as markers. Cells die in gancyclovirwhen TK is expressed, and cells that express the Zeo gene surviveexposure to zeocin. An obvious advantage of lethal selection overusing the fluorescence-activated cell sorter to separate cellson the basis of surface expression of CD2 or CD4 is the savingof time and money. A more important advantage is that we havenot encountered any metastable mutants with the lethal selection,a serious problem with IL-1-unresponsive mutants obtained by cellsorting. Another major advantage of the TK-gancyclovir selectionis that, in contrast to the gpt-6-thioguanine selection, the concentrationof selective drug can be manipulated to allow cells with a lowerlevel of constitutive marker gene expression to survive but stillto kill cells with an induced level of expression. Also, sincegancyclovir is a poor substrate for mammalian TK, the selectiondoes not require the use of a TK-null cell line. Therefore, theTK selection has the potential to become a general method forisolating mammalian cell mutants in different signalingpathways.

As illustrated here by the IRAK-null cells, mutant cell lines become extremely valuable when they can be complemented by aspecific cDNA since one then can pursue a detailed structure-functionanalysis of a single protein in a null background. Complementationof mutant cell lines defective in unknown components will enableus to identify new participants of the pathway and is a majorgoal of the genetic approach. Successful complementation requiresintroducing libraries into mutant cells with high efficiency,an appropriate level of expression of the transfected gene, andstringent selection of the complemented cells. Retroviral cDNAexpression libraries used very successfully by others (74) areour first choice in attempting to complement the IL-1-unresponsivemutant cell lines. The genetic system described here also haslimitations. For example, it would be very difficult to isolatemutants in redundant branches of a pathway unless the redundantmolecules are expressed differentially, as are IRAK and IRAK2.Finally, extensive development will be required to set up a systemthat would enable one to isolate mutant mammalian cell lines defectivein essentialgenes.

	ACKNOWLEDGMENTS

We thank Stewart Leung for helpful discussion, Mary B. Stark and Michael Haag for technical assistance, members of the Starklab for scientific input, and Jan Vilcek for the IL-8cDNA.

This work was supported by a Human Frontiers of Science Program grant and by NIH/NCI grant P01-CA62220.

	FOOTNOTES

^* Corresponding author. Mailing address: Lerner Research Institute, The Cleveland Clinic Foundation, 9500 Euclid Ave., Cleveland,OH 44195. Phone: (216) 444-3900. Fax: (216) 444-3279. E-mail address:starkg{at}cesmtp.ccf.org.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
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