Inhibiting TRAF2-mediated Activation of NF-κB Facilitates Induction of AP-1*

The compound 5-(4-methoxyarylimino)-2-N-(3,4-dichlorophenyl)-3-oxo-1,2,4-thiadiazolidine (P3-25) is known to possess anti-bacterial, anti-fungal, and anti-tubercular activities. In this report, we provide evidence that P3-25 inhibits NF-κB, known to induce inflammatory and tumorigenic responses. It activates AP-1, another transcription factor. It inhibits TRAF2-mediated NF-κB activation but not TRAF6-mediated NF-κB DNA binding by preventing its association with TANK (TRAF for NF-κB). It facilitates binding of MEKK1 with TRAF2 and thereby activates JNK and AP-1. We provide evidence, for the first time, that suggests that the interaction of P3-25 with TRAF2 leads to inhibition of the NF-κB pathway and activation of AP-1 pathway. These results suggest novel approaches to design of P3-25 as an anti-cancer/inflammatory drug for therapy through regulation of the TRAF2 pathway.

Regulation of nuclear transcription factor B (NF-B) 3 has a role in oncogenesis and cancer therapy (1). Various inflammatory stimuli, including cytokines, mitogens, bacterial products, viral proteins, and apoptosis-inducing agents, activate NF-B via expression of several genes, including adhesion molecules, cox-2 (cyclooxygenase 2), and matrix metalloproteinases (2,3). AP-1 (activator protein 1), another transcription factor like NF-B, is involved in inflammation, oncogenesis, lymphoid differentiation, embryonic development, and apoptosis (4 -6). AP-1 consists of Fos and Jun families of proteins. The heterodimer of Jun and Fos binds to AP-1 promoter site with high affinity and expresses cyclin D1 as cell proliferator (7). Higher activity of NF-B is a common characteristic of many tumor cells (1,2,8,9). The phosphoryl and acetyl forms of p65 (RelA) subunit of NF-B is the important determinant for its multifold gene expression and tumorigenic activity (10,11). Inhibiting constitutively expressed NF-B in tumor cells, the cell growth has been shown to be reduced dramatically both in vitro and in vivo (12)(13)(14). The growing evidence of the role of NF-B in tumorigenesis and resistance to chemotherapy prompt a study on the mechanism and regulation of constitutive activity of NF-B in tumor cells.
TNF superfamily members convey signals that elicit diverse cellular responses. Trimerization of TNF receptors recruits adapter proteins (members of the TNF receptor-associated factor family) to the cytoplasmic domain to initiate signaling pathways that regulate apoptosis, tumorigenesis, viral replication, etc. (15). TNF-mediated signaling thus has become a prominent target for therapeutic intervention. Interaction of TNFR1 with TNF receptor-associated death domain (TRADD) and TRAF2 (TNF receptor-associated factor 2) leads to activation of NF-B and cell death (16,17). Although interaction of TRAF2 with TANK (TRAF for NF-B) leads to activation of IB␣ kinases (IKKs) via NF-B-inducing kinase, followed by NF-B activation (18). Interaction of TRAF2 with TANK also activates JNK (18). Interaction of TRAF2 with MEKK1 (mitogen-activated protein kinase kinase kinase 1) has been shown to activate JNK and AP-1 (19). Interaction of TRAF2 with MEKK1 activates not only the JNK but also IKK␤ via recruitment of receptor-interacting protein (20).
In this report, for the first time, we provide evidence that the dimethyl form of 1,2,4-thiadiazolidine (P 3 -25) interacts with TRAF2-TANK and thereby prevents NF-B activity and inhibits downstream signaling. P 3 -25 facilitated AP-1 activation via TRAF2-MEKK1 interaction, which might explain the regulated cell cycle through AP-1-mediated gene expression. The twin effects of P 3 -25 would contribute to the therapeutic value of inhibition of TNF-mediated signaling as well as high basal expressed tumor cells. Overall, multiple effects of P 3 -25 to block NF-B completely might cut the life line of tumor cells by blocking excessive proliferation and metastasis and thereby regulate proliferation through AP-1 activation. By bypassing several side effects due to complete NF-B inhibition, P 3 -25 might prove to be a safe molecule as a chemotherapeutic drug.

EXPERIMENTAL PROCEDURES
Materials-Glycine, 4-methyl umbelliferyl phosphate, Sepharose 4B, cyanogen bromide, and anti-tubulin antibody were obtained from Sigma. 5-aryl TZD was obtained from Merck. Penicillin, streptomycin, neomycin, RPMI 1640 medium, and fetal bovine serum were obtained from Invitrogen. Antibodies against IKK␣, IKK␤, JNK, TRADD, TRAF2, MEKK1, and TANK and double-stranded AP-1 oligonucleotides were purchased from Santa Cruz Biotechnology, Inc. (Santa Cruz, CA). Antibody against phospho-JNK was obtained from Cell Signaling Technologies (Danvers, MA). Recombinant IL-8 and TNF were purchased from Peprotech. Plasmids for NF-B-SEAP, AP-1-luciferase, TRAF2, TRADD, TRAF2-DN, TRADD-DN, and GFP were kindly supplied by Prof. B. B. Aggarwal (University of Texas M. D. Anderson Cancer Center (Houston, TX)). The P 3 -25 was prepared from 1-(4-methoxyaryl)thiocarbamide as described previously (21,22) (also see supplemental Cell Lines and Treatment with P 3 -25-The cell lines used in this study were Jurkat (T-cell) and HuT-78 (modified T-cell) obtained from the American Type Culture Collection (Manassas, VA). Cells were cultured in RPMI 1640 medium containing 10% fetal bovine serum, penicillin (100 units/ml), and streptomycin (100 g/ml). P 3 -25 was chemically synthesized as described previously (21). A stock solution of 10 mM in DMSO was prepared and added to the cell culture medium to give the mentioned concentrations. Culture supernatant from HuT-78 cells, treated with 100 nM P 3 -25 for 0, 12, and 24 h, when assayed for lactate dehydrogenase activity by incubating with substrate solution (23 mM sodium pyruvate and HuT-78 cells were treated with 100 nM P 3 -25 for different times, and nuclear extracts were prepared. NF-B (A1) and AP-1 (B1) DNA binding was measured by a gel shift assay. Cells were co-transfected with plasmids for NF-B promoter DNA that had been linked to SEAP (NF-B-SEAP) or AP-1 promoter DNA that was linked to the luciferase reporter gene (AP-1-luciferase) and GFP. After washing, cells were cultured for 12 h and then treated with P 3 -25 (100 nM) for different times. The GFP-positive cells were counted, and transfection efficiency was calculated. Culture supernatant was assayed for SEAP activity. The results are represented as -fold activation over the nontransfected control (A2). After treatment, the cell pellet was extracted and assayed for luciferase activity (B2). Cells were treated with 100 nM P 3 -25 for different times. The whole cell extracts (300 g of protein) were immunoprecipitated with anti-IKK␣ and IKK␤ (1 g each) antibodies, and kinase was assayed using GST-IB␣ as a substrate (C). The IKK␣ was assayed from 100 g of protein extract by Western blot. The amount of phospho-JNK was measured from 100 g of whole cell extracts by Western blot using anti-phospho-JNK antibody (D, top). The whole cell extracts (300 g of protein) were immunoprecipitated with 1 g of anti-JNK antibody, and JNK activity was assayed using GST-Jun as substrate (D, bottom). HuT-78 cells, transfected with the NF-B-SEAP construct were treated with 100 pM P 3 -25 or 5-aryl TZD for different times, and activity of SEAP was measured from culture supernatant (E). 0.05 mM NADH in 0.1 M phosphate buffer, pH 7.5), showed 1.22 Ϯ 0.08, 1.18 Ϯ 0.09, and 1.16 Ϯ 0.078 absorbance, respectively, at 340 nm, indicating little cytolysis during incubation with the compound.
NF-B and AP-1 DNA Binding Assay-DNA binding of AP-1 and NF-B was determined by gel shift assay (24). Briefly, the cells were subjected to different treatments as described, and cytoplasmic and nuclear extracts were prepared. Nuclear extract (8 g of protein) was incubated with 32 P-end-labeled double-stranded NF-B oligonucleotide of HIV-LTR, 5Ј-TTG-TTACAAGGGACTTTCCGCTGGGGACTTTCCAGGGAG-GCGTGG-3Ј, for 30 min at 37°C, and the DNA-protein complex was separated from free oligonucleotide on 6.6% native PAGE. AP-1 DNA binding was assayed similarly using specific double-stranded labeled oligonucleotide. Visualization of radioactive bands was done in a phosphor imager (Fuji, Japan).
Assay of NF-B-dependent Secretory Alkaline Phosphatase (SEAP) Reporter Gene-Cells were transiently transfected with Qiagen SuperFect transfection reagent (Hilden, Germany) with reporter plasmid containing the NF-B binding site cloned upstream of heat-stable SEAP, designated as NF-B-SEAP and GFP (0.5 g each) constructs, for 3 h and cultured for 12 h. GFP-positive cells were counted and evaluated for transfection efficiency. These cells were treated with P 3 -25 for different time periods. Cell culture-conditioned medium (25 l) was analyzed for SEAP activity essentially as per the Clontech (Palo Alto, CA) protocol, and results are reported as -fold activation with respect to vector-transected cells as described previously (25).
Assay of AP-1-dependent Luciferase Gene Transcription-The expression of the AP-1-dependent luciferase reporter gene was carried out as described previously (26). Cells, transiently transfected with 0.5 g of reporter plasmid containing an AP-1 binding site cloned upstream of luciferase (designated as AP-1-luciferase) and GFP constructs, were washed and cultured for 12 h, followed by treatment with P 3 -25 for different time periods. The cell pellets were extracted with lysis buffer (part of the luciferase assay kit from Promega), and the extracts were incubated with the firefly luciferin substrate (Promega). Light emission was monitored with a Luminometer, and values were calculated as -fold activation over vector-transfected value.
Immunoprecipitation of MEKK1, TRAF2, and TANK and Detection by Western Blot-Sepharose 4B beads were coupled with anti-TRAF2 or anti-TANK antibody by cyanogen bromide. HuT-78 cells were transfected with vector, TRAF2, or TRAF2-DN constructs for 3 h and then cultured for 12 h. Cells were treated with 100 nM P 3 -25 for 12 h. Cells extracts were prepared and precleared with IgG, followed by removal by protein A-Sepharose beads and incubation with antibody-coupled beads for 6 h. The column was prepared with these beads and washed and eluted with high salt solution. Elutes were used to measure the amounts of TRAF2, TANK, and MEKK1 by Western blot.
Assay of IKK and JNK-The IKK and JNK assays were performed by a method described previously (25). Briefly, IKK FIGURE 2. Effect of P 3 -25 on TNF-or IL-8-induced NF-B activation and PKA␣ activity. Jurkat cells were treated with 100 nM P 3 -25 for different times and then stimulated with 100 pM TNF or 100 ng/ml IL-8 for 2 h. NF-B DNA binding was measured from nuclear extracts (A). The whole cell extracts (300 g of protein), prepared from P 3 -25-treated but TNF-or IL-8-stimulated cells for 1 h, were immunoprecipitated with anti-PKA␣ (1 g) antibody. PKA␣ activity was assayed using GST-p65 as substrate (C). The amount of PKA␣ was detected in the cell extract by Western blot. Jurkat cells were transfected with NF-B-SEAP and GFP constructs cultured for 12 h and treated with P 3 -25 for different times. Cells were then stimulated with TNF (100 pM) or IL-8 (100 ng/ml) for 12 h. Culture supernatants were used to detect SEAP activity, and activity is indicated as -fold activation relative to vector-transfected cells (B).
complex or JNK from whole-cell extract (300 g) was precipitated with anti-IKK␣ and anti-IKK␤ or anti-JNK antibodies (1 g each), followed by incubation with protein A/G-Sepharose beads (Pierce). After a 2-h incubation, the beads were washed with lysis buffer and assayed for IKK or JNK activity using 2 g of GST-IB␣ (amino acids 1-54) or GST-Jun (amino acids 1-100) as substrate proteins, respectively.
Preparation of Ligands and Docking-For docking experiments with the AutoDock 4 suite of programs, ligand molecules P 3 -25 and 5-aryl TZD were drawn, optimized, and saved in the mol2 format with the aid of Hyperchem programs. Full hydrogens were added to the ligands, and Gasteiger partial atomic charges were computed using the VEGA program in the required format (27,28). The x-ray structure of TRADD in the bound state with TRAF2 was taken from the Protein Data Bank (29) (accession number 1FV3) (30). For the building of the complex structure of TRAF2 with TANK or MEKK1, the crystal structures of TANK or MEKK1 co-ordinates were inserted into the experimental model of TRAF2. All bound waters, polar hydrogens, and the Kollman-united charges were added to the proteins. Protein pockets and cavities were located and measured using the program CastP Server (31). AutoDock requires a precalculated electrostatic grid map for each atom type present in the complex molecules. Affinity (grid) maps of 150 ϫ 150 ϫ 200 grid points and 0.375 Å (roughly a quarter of the length of a carbon-carbon single bond) spacing between grid points were utilized. The grids (one for each atom type in the ligand plus one for electrostatic interactions) were generated using the Autogrid program, and maps were centered on the protein center. AutoDock parameter set and distance-dependent dielectric functions were used in the calculation of the van der Waals and the electrostatic terms, respectively. Docking simulations were performed using the Lamarckian genetic algorithm and the Solis and Wets local search method (30). Initial position, orientation, and torsions of the ligand molecules were set randomly. All rotatable torsions were released during docking. Each docking experiment was derived from 100 different runs that were set to terminate after a maximum of 2,500,000 energy evaluations. The population size was set to 250. During the search, a translational step of 0.2 Å, and Jurkat cells were transfected with plasmids for NF-B-SEAP or AP-1-luciferase and GFP. After washing, cells were cultured for 12 h and then treated with P 3 -25 (100 nM) for different times. Nuclear extracts were prepared, and NF-B (A1) and AP-1 (B1) DNA binding was measured by gel shift assay. Culture supernatant was assayed for SEAP activity (A2). Cell pellet was extracted and assayed for luciferase activity (B2). The results are represented as -fold activation over the nontransfected control. TRAF2-and/or TRAF6-transfected cells were treated with P 3 -25 for different times. The whole cell extract (300 g of protein) was immunoprecipitated with anti-IKK␣ and IKK␤ (1 g of each) antibodies, and IKK was assayed using GST-IB␣ as substrate (C). The IKK␣ was assayed from 100 g of protein extract by Western blot. The amounts of phospho-JNK were measured from 100 g of whole cell extracts by Western blot (D, top). The whole cell extracts (300 g of protein) were immunoprecipitated with anti-JNK antibody (1 g), and JNK activity was measured using GST-Jun as substrate (D, bottom). quaternion and torsion steps of 5 were applied. Binding free energies of each job were collected, and the first rank results were selected. The clusters were ranked by the lowest energy representative of each bunch. All calculations were carried out on PC-based machines running Linux x 64 as the operating system. The resultant structure files were analyzed using PyMOL visualization programs (available on the World Wide Web).
Cluster Details-Cluster analysis or "structure binning" superimposes each final ligand structure with each other structure and measures the r.m.s. deviation between each atom pair. Structures that have an r.m.s. deviation lower than rmstol (listed in ligand.dpf) are automatically assumed to be similar; structures that have an r.m.s. deviation greater than rmstol are assumed to be different. This determines if different families of structures have been produced from multiple runs.
Statistical Analysis-Data were expressed as mean Ϯ S.D. of three independent experiments. Statistical analyses of the samples were done by Student's t test wherever applicable. p Ͻ 0.05 was considered to be significant.

RESULTS
In this study, we examined the effect of P 3 -25 in regulation of DNA binding activity of NF-B and AP-1 in the HuT-78 cell line with constitutive activity of NF-B and AP-1 and Jurkat T-cells. P 3 -25 Inhibits NF-B but Increases AP-1 Activation Pathway-Jurkat and HuT-78 cells were treated with P 3 -25 (100 nM) for different times, and then DNA binding to NF-B was measured by a gel shift assay. P 3 -25 treatment did not alter the amount of DNA bound to NF-B in these cells. HuT-78 cells showed high basal DNA binding to NF-B (Fig. 1A1). A decrease in the high basal activity (3.8-fold, p Ͻ 0.001) of the NF-B-dependent SEAP was observed in NF-B promoter-driven SEAP construct (NF-B-SEAP)-transfected HuT-78 cells (Fig. 1A2).
The amount of DNA binding to AP-1 was enhanced in Jurkat cells with increasing time of P 3 -25 treatment, whereas the high basal DNA binding to AP-1 (5.2-fold, p Ͻ 0.005) remained unaltered upon P 3 -25 treatment in HuT-78 cells (Fig. 1B1). The activity of AP-1-dependent luciferase increased upon P 3 -25 treatment in both Jurkat and HuT-78 cells (Fig. 1B2). These results suggest that P 3 -25 treatment inhibited NF-B activity and enhanced AP-1 activation. The basal activity of IKK in Jurkat and HuT-78 cells was unaltered with increasing time of P 3 -25 treatment (Fig. 1C). The basal activity of JNK in both Jurkat (1-fold, p Ͻ 0.001) and HuT-78 (4.2-fold, p Ͻ 0.005) cells increased with increasing time of P 3 -25 treatment as shown by Western blot and in vitro JNK assay data (Fig. 1D), as expected of activation of AP-1 and inhibition of NF-B.
The high basal SEAP activity in HuT-78 cells (5.8-fold, p Ͻ 0.005) decreased in a time-dependent manner of P 3 -25 treatment (Fig. 1E). The related compound, 5-aryl TZD, was ineffective under these conditions. These results suggest that P 3 -25 specifically blocks NF-B-dependent gene expression.  Fig. 2A). Surprisingly, activity of SEAP (NF-B-dependent reporter gene) was inhibited with increasing time of P 3 -25 treatment under these conditions (Fig. 2B). TNF-or IL-8-induced PKA␣ activity (4-and 5.8-fold, respectively, with p Ͻ 0.005) was inhibited by P 3 -25 treatment as detected by an in vitro kinase assay using GST-p65 as substrate protein (Fig. 2C). These results suggest that NF-B activation induced by IL-8 differs from that of TNF. P 3 -25 inhibits p65 phosphorylation by inhibiting activity of PKA␣ and thereby inhibits NF-B-dependent gene transcription as reported earlier (10,32).

P 3 -25 Inhibits TRAF2-but Not TRAF6-mediated DNA Binding of NF-B and Activity of IKK-The effect of P 3 -25 on
TRAF6-induced NF-B activation was next studied because IL-8 is known to predominantly activate NF-B by recruiting TRAF6 (26). Cells transfected with TRAF2 and also TRAF6 showed higher NF-B-DNA binding (4.4-and 3.6-fold, respectively, with p Ͻ 0.001). Treatment of P 3 -25 showed a decrease in NF-B DNA binding in TRAF2-transfected but not in TRAF6transfected or TRAF2-and TRAF6-co-transfected cells (Fig.  3A1). NF-B-dependent expression of the SEAP gene decreased in all of these transfection conditions upon P 3 -25 treatment (Fig. 3A2). P 3 -25 treatment decreased IKK activity in a time-dependent manner in TRAF2-transfected but not in TRAF6-transfected cells (Fig. 3C), suggesting that P 3 -25 interfered with TRAF2-mediated signaling upstream of IKK. P 3 -25 Induces TRAF2-or TRAF6-mediated Activation of AP-1 and JNK-P 3 -25 induced AP-1-DNA binding activity in vector-transfected cells, and this remained unaltered in TRAF2-transfected, TRAF6-transfected, or TRAF2-and TRAF6-transfected cells (Fig. 3B1). However, P 3 -25 treatment increased AP-1-dependent luciferase activity in vector-transfected, TRAF2-transfected, TRAF6-transfected, or TRAF2-and TRAF6-transfected cells (Fig. 3B2). These results indicate that interaction of P 3 -25 with TRAF2 leads to activation of AP-1. High basal activity of JNK in TRAF2-transfected (4.2-fold, p Ͻ 0.005) or TRAF6-transfected (3.4-fold, p Ͻ 0.005) cells was enhanced further by P 3 -25 treatment in a time-dependent manner, as shown by an in vitro JNK assay, which was further supported by Western blot data using anti-phospho-JNK antibody (Fig. 3D). These data further suggest AP-1 activation upon P 3 -25 treatment through JNK activation via the TRAF2 and TRAF6 pathway.  Fig. 2A1). Similarly, P 3 -25 treatment had no effect on the changes of the NF-B-dependent reporter gene SEAP activity in NF-B-SEAP-transfected cells (supplemental Fig. 2A2). Treatment of P 3 -25 in TRAF2-DN-or TRADD-DNtransfected cells decreased high basal amount of AP-1 DNA binding (supplemental Fig. 2B1) and AP-1-dependent luciferase activity (supplemental Fig. 2B2). These data suggest that TRAF2 and TRADD are required for P 3 -25-mediated AP-1 activation as well as NF-B inhibition.
High basal activity of IKK decreased in TRADD-DN or TRAF2-DN HuT-78 cells, and this remained unaltered with P 3 -25 treatment with time in both of these transfected cells (supplemental Fig. 2C). The basal activity of JNK, measured by the amount of phospho-JNK, was further increased with increasing time of P 3 -25 treatment. TRADD-DN or TRAF2-DN transfection decreased the basal amount of phospho-JNK, and P 3 -25 treatment of these cells had no effect on these values at any time of treatment (supplemental Fig. 2D). These data further support the role of TRADD and TRAF2 in P 3 -25-mediated cell signaling. P 3 -25 Treatment Blocks TRAF2-TANK and Facilitates TRAF2-MEKK1 Interaction-TRAF2 interacts with TANK (TNF receptor-associated factor for NF-B) and MEKK1 (18). When TRAF2 was immunoprecipitated with anti-TRAF2 antibody from TRAF2-DN-transfected HuT-78 cells, the amount of MEKK1 or TANK was undetected as shown by Western blot. TRAF2 interacted with MEKK1 and TANK as shown by a  The best clusters of a total 100 runs are shown. b The geometry fit was measured by r.m.s. deviation of angles, r.m.s. deviation ϭ (⌺ ␣i Ϫ ␣ ideal )2/n)1/2, where ␣i is the measured angle, ␣ ideal is the angle in ideal coordination geometry, and n is the total number of angles of the corresponding geometry. c Value for the optimal structure in the cluster.  (C2, left). Interaction of 5-aryl TZD with MEKK1 active site residues (magenta) and TRAF2 complex is analyzed (C2, right). The graph shows the lowest binding energies of complexes with P 3 -25 and 5-aryl TZD with different complexes (D).
Western blot from a fraction immunoprecipitated against anti-TRAF2 antibody of TRAF2-or vector-transfected HuT-78 cell extract. P 3 -25 treatment inhibited interaction of TRAF2 with TANK but not with MEKK1 (Fig. 4A). P 3 -25 treatment showed the inhibition of TRAF2 and TANK interaction in vector-or TRAF2-transfected HuT-78 cells, as shown by Western blot from the immunoprecipitated fraction by anti-TANK antibody. The amount of MEKK1 decreased in vector-or TRAF2-transfected HuT-78 cell extracts upon P 3 -25 treatment (Fig. 4B). In TRAF2-DN-transfected cells, the amounts of both MEKK1 and TRAF2 were not detected in immunoprecipitated fractions with anti-TANK antibody. These data further indicate that TRAF2 interacts with TANK and MEKK1 and that P 3 -25 inhibits TRAF2 and TANK interaction. P 3 -25 Interacts with TRAF2 More Potently Than TRAF6-The binding affinities of P 3 -25 with TRAF2 and TRAF6 were evaluated by the binding free energies (⌬Gb, kcal/mol), inhibition constants (K i ), hydrogen bonds, and r.m.s. deviation values. The predicted binding sites for TRAF2 and TRAF6 with P 3 -25 are shown in Fig. 5A. P 3 -25 mostly binds with positive charged basic amino acid residues and the predicted active sites of TRAF2 and TRAF6 (Fig. 5B). The different surface pocket for residues seems to be an important factor in determining the different mode of P 3 -25 interaction with TRAF2 and TRAF6, where the P 3 -25 binds with Arg 393 , Phe 447 , and Asp 399 of TRAF2 and Arg 392 , Lys 469 , and Gly 470 of TRAF6 (Fig. 5B). The binding free energies of these residues, calculated based on their best docking scores, are Ϫ18.43 kcal/mol and Ϫ11.21 kcal/mol for TRAF2 and TRAF6, respectively ( Table 1). The difference between the lowest binding interaction of TRAF2 and TRAF6 with P 3 -25 is shown in Fig. 5C. It revealed the energy difference and cluster runs of the TRAFs. From the above results, it is clear that P 3 -25 interferes with TRAF2 action more efficiently than with that of TRAF6. P 3 -25 Interferes Interaction between TRAF2 and TANK but Not between TRADD and TRAF2 or TRAF2 and MEKK1-TRADD-TRAF2, TRAF2-TANK, and TRAF2-MEKK1 binding sites were identified as described previously (31), and predicted binding sites of P 3 -25 and 5-aryl TZD with these complexes were shown by surface binding in Fig. 6, A1, B1, and C1, respectively. The complex of TRADD-TRAF2 formed a hydrogen bond with P 3 -25 and 5-aryl TZD (Fig. 6A2) with binding free energy of Ϫ11.35 and Ϫ11.55 kcal/mol, respectively ( Table 2, top) suggesting weak interaction for both. The benzene ring of P 3 -25 is surrounded by hydrophobic residues (Ala 466 , Ser 467 , Tyr 395 , and Gly 400 ), and they formed hydrophic interactions in the TRAF2-TANK complex. In addition, the two oxygen atoms of the benzene ring of P 3 -25 formed three hydrogen bonds with Arg 393 , Phe 447 , and Asp 399 . The 5-aryl TZD formed hydrogen bonds with Arg 392 , Lys 446 , and Gly 470 of the TRAF2-TANK complex (Fig. 6B2). The energies of these residues for TRAF2-TANK are Ϫ18.43 and Ϫ15.43 kcal/mol for P 3 -25 and 5-aryl TZD, respectively (Table 2, middle) suggesting that P 3 -25 has higher binding affinity than 5-aryl TZD for forming TRAF2-TANK complex. The TRAF2-MEKK1 electrostatic potential surface showed the possible docking interaction with P 3 -25 and 5-aryl TZD (Fig. 6C1). P 3 -25 formed a single hydrogen bond with the active site Lys 192 residue of the TRAF2-MEKK1 com- The best clusters of a total 100 runs are shown. b The geometry fit was measured by r.m.s. deviation of angles. r.m.s. deviation ϭ (⌺a i Ϫ ␣ ideal )2/n)1/2, where ␣i is the measured angle, ␣ ideal is the angle in ideal coordination geometry, and n is the total number of angles of the corresponding geometry. c Value for the optimal structure in the cluster. d 5-Aryl TZD lacks binding ability with the TRAF2-MEKK1 complex, which gives a negligible value of the inhibition constant (K i ) compared with other ligands. plex (Fig. 6C2). It showed the lowest binding energy (Ϫ4.89 kcal/mol). The 5-aryl TZD showed the lowest binding energy (ϩ157.21 kcal/mol) with residues in the TRAF2-MEKK1 complex ( Table 2, bottom) suggesting no interaction. The docking of the complex of TRAF2-MEKK1 with P 3 -25 showed fewer interactions compared with TRAF2-TANK or TRADD-TRAF2 complex. The above results revealed that synthetic P 3 -25 molecule more potently complexes with TRAF2-TANK than 5-aryl TZD (Fig. 6D), supporting the experimental studies obtained.

DISCUSSION
The present study demonstrated that the dichlorophenyl derivative of 1,2,4-thiadiazolidine (P 3 -25) decreases NF-B activation and enhances AP-1 activation by interacting with TRAF2. It did not inhibit IL-8-or TRAF6-induced NF-B DNA binding but inhibited NF-B-dependent reporter gene expression. IL-8-mediated NF-B activation requires recruitment of TRAF6 (26). We did not observe TRAF6-or IL-8-induced inhibition of IKK activity. P 3 -25 inhibited dependent gene expression of NF-B in cells irrespective of inducers of NF-B, over-expression of upstream molecules, such as TRAFs, or having constitutive NF-B expression. This is in complete agreement with our previous report on P 3 -25 blocking expression of NF-B-dependent genes through inhibition of p65 phosphorylation (10). TNF signals through recruitment of TRAF2 and IKKs via TANK. TNF-induced activation of IKKs was not observed upon P 3 -25 treatment, which was reflected in inhibition of NF-B, supporting our previous observation (21). This suggests that the effect of P 3 -25 lies on TRAF2, but not on IKK. TRAF2 interacts with TANK and MEKK1 (18). P 3 -25 treatment inhibited TANK interaction with TRAF2, which was supported by a pull-down assay as well as AutoDock evidence. P 3 -25 did not interfere with TRAF2-MEKK1 interaction. TRAF2-TANK interaction has been shown to induce JNK and AP-1 (18). Although we observed JNK activation, which may be independent of TRAF2-TANK interaction, in silico data also suggest that P 3 -25 interferes with TRAF2-TANK but not TRADD-TRAF2 or TRAF2-MEKK1 interactions.
AutoDock evidence and the values of lowest binding energy suggest that the binding affinity of P 3 -25 with the TRAF2-TANK complex is stronger than the TRADD-TRAF2 or TRAF2-MEKK1 complex. The 5-aryl thiazolidine-2,4-diones, structurally similar to P 3 -25, having the same backbone, does not interact with TRAF2-MEKK1 at all and weakly interact with TRADD-TRAF2 or TRAF2-TANK. The strong binding ability of P 3 -25 with the TRAF2-TANK complex hinders the recruitment and activation of IKKs, the immediate molecules of such interaction. P 3 -25 is also known to inhibit p65 phosphorylation by blocking upstream kinases, casein kinase 2 and protein kinase A (10). The double sword effect of P 3 -25 on inhibition of NF-B might be important for the potential therapeutic value of P 3 -25 in NF-B-driven inflammatory and tumorigenic responses. Although P 3 -25 induces AP-1 by facilitating MEKK1 recruitment with TRAF2 followed by JNK activation, as shown in the schematic diagram in Fig. 7, the AP-1mediated signaling may be less responsible for such responses than NF-B.
NF-B and AP-1 regulate cell cycle in embryonic development and body growth. Excessive activation of these transcription factors results in inflammatory response and rapid cell cycle progression, the hallmark of tumorigenesis. Regulation of FIGURE 7. Schematic diagram of P 3 -25-mediated interference with cell signaling to inhibit NF-B but to activate AP-1.
these transcription factors is required to control inflammatory diseases and cancer metastasis. Predominantly enhanced NF-B activation through p65 phosphorylation and acetylation via recruitment of several cofactors is a prerequisite for the severalfold NF-B-mediated transcription of genes required for tumorigenesis and tumor metastasis. Knock-out of NF-B has several deleterious effects and is even lethal for embryo. Even T-cell-mediated apoptosis of dendritic cells has been shown to be inhibited through JNK-AP-1 activation when signaling mediated by TNF receptor superfamily members was ligated (33). Thus, deregulation of NF-B function, while allowing AP-1 activation to progress regulated cell division through the interaction of P 3 -25 with TRAF2, would be ideal for many reasons. AP-1 is a mild transcription factor and is mostly involved in regulated cell cycle progression. Initially, it was considered to be a housekeeping transcription factor. In this report, for the first time we provide evidence that P 3 -25, a synthetic derivative, interacts with TRAF2 in such a manner that recruitment of TANK is completely inhibited and thereby inhibits recruitment of IKKs. Thus, P 3 -25 is inhibiting IB␣ degradation, thereby arresting NF-B in cytoplasm. Although TRAF6-or IL-8-mediated IKKs activation is unaffected by P 3 -25 treatment, it blocks NF-B-dependent gene transcription by inhibiting p65 phosphorylation. Thus, the double sword mechanisms of P 3 -25 action are shutting down NF-B functions completely (Fig. 7). Although P 3 -25 binding with TRAF2 inhibited TANK binding, it facilitated binding with MEKK1 required for AP-1 activation via JNK. Thus, P 3 -25 is allowing AP-1 activation. However, P 3 -25 would be an important drug target by blocking NF-B action totally but allowing AP-mediated cell signaling to regulate inflammatory and tumorigenic responses without compromising its regulated cell growth. Thus, P 3 -25 might be a safe molecule as a potential chemotherapeutic drug by avoiding several side effects otherwise obtained upon complete inhibition of NF-B and anticipating the function of NF-B by activation of AP-1 in a regulated fashion.