Activation of Stat3 in v-Src-transformed Fibroblasts Requires Cooperation of Jak1 Kinase Activity

doi:10.1074/jbc.M002383200

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Activation of Stat3 in v-Src-transformed Fibroblasts Requires Cooperation of Jak1 Kinase Activity^*

Yi Zhang^a^b^c, James Turkson^a^c, Christin Carter-Su^d, Thomas Smithgall^e, Alexander Levitzki^f, Alan Kraker^g, John J. Krolewski^h, Peter Medveczky^a^bⁱ, and Richard Jove^a^b^c^j

From the ^a Molecular Oncology Program, H. Lee Moffitt Cancer Center and Research Institute, ^b Institute for Biomolecular Sciences, ^c Department of Biochemistry and Molecular Biology, and ⁱ Department of Medical Microbiology and Immunology, University of South Florida College of Medicine, Tampa, Florida 33612, the ^d Department of Physiology, University of Michigan Medical School, Ann Arbor, Michigan 48109, the ^e Department of Molecular Genetics and Biochemistry, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania 15261, the ^f Department of Biological Chemistry, Alexander Silberman Institute of Life Sciences, The Hebrew University of Jerusalem, Jerusalem 91904, Israel, the ^g Department of Cancer Research, Parke-Davis Pharmaceutical Research, Ann Arbor, Michigan 48105, and the ^h Department of Pathology, University of California, Irvine, California 92697

Received for publication, March 20, 2000, and in revised form, May 15, 2000

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Signal transducers and activators of transcription (STATs) are latent cytoplasmic transcription factors that transduce signalsfrom the cell membrane to the nucleus upon activation by tyrosinephosphorylation. Several protein-tyrosine kinases can induce phosphorylationof STATs in cells, including Janus kinase (JAK) and Src familykinases. One STAT family member, Stat3, is constitutively activatedin Src-transformed NIH3T3 cells and is required for cell transformation.However, it is not entirely clear whether Src kinase can phosphorylateStat3 directly or through another pathway, such as JAK familykinases. To address this question, we investigated the phosphorylationof STATs in baculovirus-infected Sf-9 insect cells in the presenceof Src. Our results show that Src can tyrosine-phosphorylate Stat1and Stat3 but not Stat5 in this system. The phosphorylated Stat1and Stat3 proteins are functionally activated, as measured bytheir abilities to specifically bind DNA oligonucleotide probes.In addition, the JAK family member Jak1 efficiently phosphorylatesStat1 but not Stat3 in Sf-9 cells. By contrast, we observe thatAG490, a JAK family-selective inhibitor, and dominant negativeJak1 protein can significantly inhibit Stat3-induced DNA bindingactivity as well as Stat3-mediated gene activation in NIH3T3 cells.Furthermore, wild-type or kinase-inactive platelet-derived growthfactor receptor enhances Stat3 activation by v-Src, consistentwith the receptor serving a scaffolding function for recruitmentand activation of Stat3. Our results demonstrate that Src kinaseis capable of activating STATs in Sf-9 insect cells without expressionof JAK family members; however, Jak1 and platelet-derived growthfactor receptor are required for maximal Stat3 activation by Srckinase in mammalian cells. Based on these findings, we proposea model in which Jak1 serves to recruit Stat3 to a receptor complexwith Src kinase, which in turn directly phosphorylates and activatesStat3 in Src-transformedfibroblasts.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Signal transducers and activators of transcription (STATs)¹ are a family of latent cytoplasmic transcription factors that areactivated in response to various extracellular polypeptide ligands,including cytokines and growth factors (1, 2). Upon cytokinestimulation, cytokine receptors dimerize and thereby activatereceptor-associated tyrosine kinases of the Janus kinase (JAK)family (3). The activated JAKs induce STAT activation by atwo-step mechanism. First, JAKs phosphorylate receptor tyrosineresidues, which in turn become docking sites for the recruitmentof cytoplasmic STAT proteins. Second, the recruited STAT proteinsare directly phosphorylated by the receptor-associated JAKs. ActivatedSTATs then dimerize and translocate to the nucleus, where theybind to specific promoter sequences of target genes and inducetranscription (4). This signaling mechanism is often referredto as the JAK-STAT pathway (2, 3).

Seven mammalian STAT family members have been identified and characterized, and they share similar structural features aswell as activation mechanism (1, 4). The different STATsare involved in mediating a variety of biological functions indiverse cell types. For example, Stat1 is critical for interferonfunctions as well as innate immunity (5, 6), while Stat3is required for IL-6 signaling in hematopoietic cells as wellas anti-apoptosis (7-9). Targeted disruption of the mouse Stat3gene is embryonic lethal (10), which demonstrates the importanceof Stat3 in the development of mouse embryos. In addition, Stat5has been shown to be important in lactation and hematopoiesis(11-13).

STAT activation has also been observed to be induced by epidermal growth factor and PDGF receptors with intrinsic tyrosinekinase activities (14-17). While receptor tyrosine kinases maydirectly phosphorylate STATs, some reports suggest that JAKs areinvolved in PDGF-induced STAT activation. For example, the JAKfamily kinases, Jak1, Jak2, and Tyk2, are activated in cells stimulatedwith PDGF (18). Furthermore, recent studies suggest that Stat3activation by PDGF receptor is mediated by JAK kinases but thatStat1 activation is not (19). PDGF can also activate the nonreceptortyrosine kinase c-Src (20, 21), and it has been suggestedthat c-Src activates Stat1 and Stat3 in PDGF-stimulated murinefibroblast cells (22). These findings indicate that STAT activationby polypeptide hormones involves nonreceptor tyrosine kinasesin addition to the intrinsic tyrosine kinase of theirreceptors.

We and others have observed the constitutive activation of Stat3 in v-Src-transformed cells (23-25). Further studies demonstratedthat this Stat3 activation results in gene activation and is essentialfor v-Src transformation (26, 27). Although direct activationof Stat3 by Src has been suggested (24, 28), the mechanismof Stat3 activation is not entirely clear (29) and may employdifferent mechanisms that are dependent on the cell type. In v-Src-transformedmouse fibroblasts, Jak1 and, to a much lesser extent, Jak2 arealso constitutively activated (30). To investigate the mechanismof Stat3 activation by Src, we examined STAT activation by Srcand Jak1 expressed from recombinant baculoviruses in Sf-9 insectcells as well as the role of Jak1 in Stat3 activation in mousefibroblasts transformed by v-Src.

Here we report that Stat1 and Stat3 are tyrosine-phosphorylated in Sf-9 cells by activated Src in the absence of other mammaliantyrosine kinases. The phosphorylated STAT proteins bind to specificDNA sequences in gel shift assays, indicating that this phosphorylationinduces functional activation of the STAT proteins. Furthermore,Jak1 enhances activation of Stat1 but not Stat3 when co-expressedwith Src in Sf-9 cells, and the phosphorylation level of Jak1is also increased with the expression of Src. By contrast, inNIH3T3 cells, Jak1 activity is required for maximal Stat3-mediatedgene induction. In addition, activation of Stat3 by Src in mammaliancells is enhanced by the PDGF receptor independently of receptorkinase activity, consistent with a scaffolding function for thereceptor. Our results indicate that, although Src can directlyactivate Stat3 in insect cells, Jak1 plays an important role inthe activation of Stat3 in Src-transformed mouse fibroblasts.These findings support a model in which Src and Jak1 cooperatetogether with the PDGF receptor and possibly other receptors toactivate Stat3 in the context ofoncogenesis.

EXPERIMENTAL PROCEDURES

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Cells and Reagents-- NIH3T3 cells and their Src-transformed counterparts have been described previously (23, 31). The human fibrosarcoma cell,2fTGH (32), was a kind gift from Dr. George Stark (ClevelandClinic Foundation, Cleveland, OH). Expression vectors for wild-typeand kinase-inactive PDGF receptor- $beta$ (33, 34) were generouslyprovided by Dr. Andrius Kazlauskas (The Schepens Eye ResearchInstitute, Boston, MA). Anti-Jak1 antibody (HR-785) was obtainedfrom Santa Cruz Biotechnology, Inc. (Santa Cruz, CA); anti-phosphotyrosine701-Stat1 and anti-phosphotyrosine 694-Stat5 were from Zymed LaboratoriesInc.; anti-phosphotyrosine 705-Stat3 was from New England Biolabs;anti-phosphoserine 727-Stat1 and -Stat3 (35) were kind giftsfrom Dr. David Frank (Dana-Farber Cancer Institute, Boston, MA);anti-Stat1 (E-23), anti-Stat3 (K-15), anti-Stat5A (L-20), andanti-phosphotyrosine (PY-99) for Western blot analyses were fromSanta Cruz Biotechnology; anti-Stat1 (E-23) and anti-Stat3 (H-190)for gel supershift assays were also from Santa Cruz Biotechnology.Peroxidase-free Triton X-100 was obtained from Roche MolecularBiochemicals; recombinant protein A/G-agarose was from Santa CruzBiotechnology; and enhanced chemiluminescence (ECL) detectionassays were from Amersham Pharmacia Biotech. AG490 (36) andPD180970 (37) have been describedelsewhere.

Recombinant Baculoviruses and Protein Expression in Sf-9 Insect Cells-- Stat3 recombinant baculovirus was generated using the Bac-to-Bac Expression System (Life Technologies, Inc.) according tothe supplier's protocol. Briefly, the mouse Stat3 cDNA was clonedinto pFastBac donor plasmid and transformed into competent DH10BacEscherichia coli cells. White colonies were selected, and theinsertion of Stat3 cDNA was verified by polymerase chain reactionwith primers to the 5'- and 3'-ends. High molecular weight DNA(recombinant bacmid DNA) was generated and transfected to Sf-9cells, and recombinant baculoviruses encoding Stat3 were titeredbefore being used for protein expression. Jak1 and Stat1 recombinantbaculoviruses (38) were generous gifts from Dr. James Ihle (St.Jude Children's Hospital, Memphis, TN). The Stat5A and c-Src baculoviruseshave been previously described (39, 40). For infection withbaculoviruses, Sf-9 insect cells were plated at 1 × 10⁶ cells/35-mm dish (six-well plates) in 2 ml of SF-900II serum-freemedium (Life Technologies) and incubated for 1 h. After Sf-9 cellsattached to the dish, the medium was replaced with 500 µl of infectionmixture containing a combination of appropriately diluted baculovirusesin Sf-900II medium. The cells were then incubated for 1 h at 27°C with slow rocking. The medium was replaced with fresh medium,and the cells were further incubated for 48 h prior toharvest.

Preparation of Cytosolic Extracts of Sf-9 Cells-- Cytosolic extracts were made with a modified radioimmune precipitation buffer. Briefly, culture dishes of Sf-9 cells werewashed twice with ice-cold PBS followed by PBS containing 1 mMsodium orthovanadate. The cells were then lysed in Nonidet P-40lysis buffer (50 mM HEPES, pH 7.9, 150 mM NaCl, 1% Nonidet P-40,20 mM sodium fluoride, 1 mM sodium orthovanadate, 1 mM tetrasodiumpyrophosphate, 1 mM dithiothreitol, 0.5 mM phenylmethylsulfonylfluoride, 2 mM EGTA, 2 mM EDTA, 0.1 µM aprotinin, 1 µM leupeptin,and 1 µM antipain) on ice for 10 min. The extract was clarifiedby microcentrification at 13,000 × g, and protein concentrationwas determined with the Bio-Rad Protein Assay. The extract wasfrozen in aliquots at $-$ 80 °C untiluse.

Western Blot Analyses-- Cytosolic extracts or immunoprecipitated proteins were separated on 8% SDS-polyacrylamide gels and transferred to nitrocellulosemembranes. The membranes were blocked with 5% nonfat dried milkfor 1 h and then incubated for 1 h with antibodies against Stat1,Stat3, Stat5, Jak1, or Src at 1 µg/ml in PBS plus 0.1% Tween 20(PBST) containing 3% nonfat dried milk. For anti-phosphotyrosineblots, the membranes were blocked with chicken ovalbumin (gradeIII; Sigma) instead of dried milk for 2 h. The membranes werethen washed in PBST and probed with anti-phosphotyrosine antibodiesand subsequently with appropriate secondary antibodies for 1 h.After another 15-min wash in PBST, the membranes were treatedwith ECL detection solutions and exposed tofilms.

In Vitro Kinase Assays-- For Jak1 kinase assays, we followed the previously published procedure with minor modifications (30). For immunoprecipitationof Jak1, whole-cell lysates were incubated with 2 µg of anti-Jak1antibody for 2 h at 4 °C followed by a 1-h incubation with 20µl of protein A/G-agarose. The immunoprecipitates were then washedtwice with wash buffer and once with phosphorylation buffer asdescribed previously (30). The kinase reactions were carriedout at 30 °C for 40 min in 100 µl of the kinase buffer (100 mMNaCl, 50 mM HEPES, pH 7.6, 0.1% Triton X-100, 0.5 mM dithiothreitol,6.25 mM MnCl₂, 20 µCi of [ $gamma$ -³²P]ATP, 0.1 µM aprotinin, 1 µM leupeptin, and 1 µM antipain). Wheninhibitors were used, AG490 or PD180970 was added to the reactionmix prior to the addition of the kinase buffer. The reactionswere stopped with 10 mM EDTA, and the agarose beads were washedtwice with washing buffer and boiled for 5 min in SDS-PAGE samplebuffer. Proteins were separated by 8% SDS-PAGE, and phosphorylatedJak1 was visualized by autoradiography. In vitro Src kinase assayswere performed as described previously (41, 42). Briefly,whole-cell lysates containing 1 mg of total protein were incubatedwith 2 µg of anti-Src antibody for 4 h at 4 °C followed by 1 hof incubation with protein A/G-agarose beads with rotation. Theimmunoprecipitates were then washed three times with modifiedRIPA-150 buffer (10 mM Tris-Cl, pH 7.5, 150 mM NaCl, 10% glycerol,5 mM EDTA, 1% Triton X-100, 0.1% SDS, 100 µM Na₃VO₄, 0.1 µM aprotinin,1 µM leupeptin, and 1 µM antipain), two times with RIPA-10 buffer(the same as RIPA-150 buffer except with 10 mM NaCl instead of150 mM NaCl), and three times with Tris buffer (40 mM Tris, pH7.4). The immunoprecipitates were then resuspended with 30 µlof kinase reaction buffer (20 mM Tris-HCl, pH 7.4, 5 mM MgCl₂)containing 10 µCi of [ $gamma$ -³²P]ATP and 5 µg of acid-denatured enolase as exogenous substrate.Inhibitors were preincubated for 10 min with kinases or addedimmediately after the kinase reaction buffer. Kinase reactionmixtures were incubated 15 min at room temperature and stoppedby the addition of loadingbuffer.

Electrophoretic Mobility Shift Assay-- The procedures for nuclear extract preparation from mammalian cells and electrophoretic mobility shift assays (EMSAs) wereconducted as previously published (23, 43). The ³²P-radiolabeled oligonucleotide probes are (a) hSIE (high affinitysis-inducible element, m67 variant, 5'-AGCTTCATTTCCCGTAAATCCCTA)for Stat1 and Stat3 (43, 44) and (b) MGFe (mammary gland factorelement from the bovine $beta$ -casein gene promoter, 5'-AGATTTCTAGGAATTCAA)for Stat5 binding (11, 45). For cytosolic extracts from Sf-9cells, 0.05 µg of total protein was used in each reaction. Inthe case of competitions, a 100-fold molar excess of unlabeledprobes was added to each reaction. The FIRE probe (5'-AGCGCCTCCCCGGCCGGGG)was used as nonspecific competitor (23, 43). For supershifts,1 µl of the antibodies against each specific STAT was preincubatedwith the extract for 20 min prior to the addition of radiolabeledprobes (43). The reactions were incubated at 30 °C for 30 minand then resolved on 5% polyacrylamide gels in 0.25× Tris borate-EDTAbuffer. STAT-DNA complexes were detected by autoradiography. Forthe inhibitor treatment, NIH3T3 cells stably transformed withv-Src were treated with fresh inhibitors, AG490 or PD180970, every12 h for a total of 24h.

Transfections and Luciferase Reporter Assays-- NIH3T3 cells were grown in Dulbecco's modified Eagle's medium containing 5% iron-supplemented bovine calf serum. Transienttransfections were performed with calcium phosphate as describedpreviously (26). Briefly, NIH3T3 cells were seeded at 5 × 10⁵ cells/100-mm dish in Dulbecco's modified Eagle's medium (5% bovinecalf serum) at 18 h prior to transfection. 20 µg of total DNAwas used for each plate, which contained typically 4 µg of Stat3reporter construct pLucTKS3, 0.2 µg of $beta$ -galactosidase internalcontrol, and the amounts of expression vector described in thefigure legends. The plates were washed once with PBS and replenishedwith fresh Dulbecco's modified Eagle's medium at 15 h after transfection.The cells were harvested 48 h after transfection, and whole-celllysates were assayed for luciferase as well as $beta$ -galactosidaseactivities.

Human fibrosarcoma cell line, 2fTGH, was cultured in Dulbecco's modified Eagle's medium containing 10% fetal bovine serumas described previously (32). The transfection was performedwith LipofectAMINE Plus according to the supplier's protocol (LifeTechnologies). Six µg of plasmid DNA expressing wild type or kinase-deadPDGF-R $beta$ was transfected into 2fTGH culture in a 60-mm dish. Transfectedcells were then selected against G418 at 400 µg/ml final concentration.After selection, cells stably transfected with the respectiveplasmids were pooled and then used for transient transfectionswith v-Src expression vector using LipofectAMINE Plus asabove.

RESULTS

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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Activation of Stat1 and Stat3 by Src in Sf-9 Cells-- It is now well established that v-Src induces constitutive activation of Stat3 signaling in transformed cells (23-25). However,it is not entirely clear whether Stat3 is activated directly bySrc or through the cooperation of JAK family kinases acting downstreamof Src. To address this question, we utilized a baculovirus/insectcell system to overexpress STATs and Src in the absence of othermammalian tyrosine kinases. Sf-9 insect cells were infected withrecombinant c-Src baculovirus either alone or in combination withStat3 baculovirus. In this system, c-Src is an activated kinasedue to lack of phosphorylation of the negative regulatory Tyr-527residue (46).

Activation of STAT proteins was examined in cytosolic extracts using EMSA with a specific oligonucleotide probe (hSIE) todetect DNA-binding activities. As shown in Fig. 1, co-expressionof activated c-Src kinase and either Stat1, Stat3 $alpha$ , or Stat3 $beta$ protein induced high levels of hSIE-binding activity (lanes 1-9).As previously observed, Stat3 $beta$ -hSIE complexes migrate more slowlythan Stat3 $alpha$ -hSIE complexes, although the Stat3 $beta$ splice varianthas a C-terminal-deletion relative to full-length Stat3 $alpha$ (26,47). Expression of either c-Src or Stat1 alone results in noDNA binding activity, while Stat3 $alpha$ or Stat3 $beta$ expressed individuallyexhibits very low levels of activity, possibly due to basal levelsof phosphorylation. We also expressed c-Src with Stat5A in Sf-9cells; however, Stat5A co-expressed with c-Src did not resultin any detectable MGFe binding activity (Fig. 1, lanes 10-14).These results indicate that Src is capable of efficiently activatingStat1 and Stat3, but not Stat5A, in the absence of additionalmammalian tyrosine kinases.

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Fig. 1. DNA binding activities of STATs induced by Src in Sf-9 insect cells. Sf-9 cells were infected with recombinant baculovirus expression vectors for Stat1, Stat3 $alpha$ , Stat3 $beta$ , or Stat5A, either alone or in combination with c-Src baculovirus as indicated. Cytosolic lysates were used for EMSA with radiolabeled hSIE probe to detect active Stat1, Stat3 $alpha$ , and Stat3 $beta$ (lanes 1-9) or with radiolabeled MGFe probe to detect active Stat5A (lanes 10-14). Positions of the activated STAT-DNA complexes are labeled. The free probe lane contains no protein, and the Sf-9 lane contains lysate from uninfected cells.

To confirm the identities of each protein-DNA complex, we performed competition and supershift analyses as shown in Fig. 2.Shifted radiolabeled hSIE probe was competed by a 100-fold molarexcess of unlabeled hSIE (Fig. 2, lanes 3, 9, and 15) but notthe irrelevant FIRE oligonucleotide, demonstrating specificityof DNA binding. Stat1-hSIE complexes were supershifted only withanti-Stat1 antibody (lane 4). Most of the Stat3-hSIE complexeswere blocked by anti-Stat3 antibody with some supershifted complexesdetected but not affected by antibodies against Stat1 and Stat5A(lanes 10-12 and 16-18). These results suggest that Src is capableof directly activating Stat1 and Stat3 without the presence ofany mammalian JAK family kinase or another intermediate protein-tyrosinekinase in Sf-9 insect cells. This finding is consistent with earlierstudies of Stat3 activation in Src-transformed cells (23-25), whichsuggested that Stat3 is directly activated by v-Src. Interestingly,we and others did not observe the activation of Stat1 in v-Src-transformedfibroblasts (23, 24).

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Fig. 2. Identification of STAT-DNA complexes activated in Sf-9 cells. Cytosolic lysates from Sf-9 cells infected with baculoviruses encoding STATs or Src as indicated were incubated with either nonspecific oligonucleotide competitor, FIRE, or the unlabeled hSIE oligonucleotide at a 100-fold molar excess or with anti-Stat1, anti-Stat3, or anti-Stat5A antibodies. The positions of specific STAT-hSIE complexes are indicated as Stat1, Stat3 $alpha$ , and Stat3 $beta$ . The supershifted STAT-hSIE-antibody complexes are indicated with asterisks.

Src Induces Tyrosine Phosphorylation of Stat1 and Stat3 in Sf-9 Cells-- Phosphorylation of tyrosine residues 701 of Stat1 and 705 of Stat3 are required for STAT dimerization and DNA binding (4,48, 49). To determine whether Stat1 and Stat3 DNA bindingactivities induced by Src are associated with tyrosine phosphorylation,cytosolic extracts used for EMSA were analyzed by SDS-PAGE andimmunoblotting with the anti-phosphotyrosine antibody, PY99. Asshown in Fig. 3A, Stat1, Stat3 $alpha$ , and Stat3 $beta$ are phosphorylatedon tyrosine in the presence of Src but were not phosphorylatedwhen expressed alone. Following stripping and reprobing of thesame blot, total protein levels of Stat1, Stat3 $alpha$ , Stat3 $beta$ , andStat5A were detected with anti-Stat1, anti-Stat3, and anti-Stat5A-specificantibodies. The position of each protein, as determined by comparingthe blots in Fig. 3, A and B, is indicated by an arrow in A. Insome cases, lower molecular weight forms were detected, whichprobably represent proteolytic products of the full-length STATproteins (B). Stat5A did not contain tyrosine phosphorylation,since no band in Fig. 3A aligns with Stat5A protein as detectedby anti-Stat5A, consistent with the EMSA results. As further confirmationof this conclusion, anti-phospho-Stat5A antibody did not detecttyrosine-phosphorylated Stat5A (data not shown), although highlevels of Stat5A protein were co-expressed with Src.

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Fig. 3. Phosphorylation of Stat1 and Stat3 induced by Src in Sf-9 cells. Western blot analysis was performed with the same cytosolic extracts from Sf-9 cells infected with c-Src and/or STAT baculoviruses used for the EMSAs in Figs. 1 and 2. A, the anti-phosphotyrosine antibody PY-99 was used to detect total tyrosine-phosphorylated proteins. B, the immunoblot of A was stripped and reprobed with a mix of antibodies against Stat1, -3, and -5A combined together. The positions of Stat1, -3 $alpha$ , -3 $beta$ , and -5A were identified by overlaying films and are indicated in A. The same immunoblot was stripped and reprobed multiple times using antibodies specifically recognizing phosphorylated Stat1 at serine residue 727 (C) or at tyrosine residue 701 (D) and phosphorylated Stat3 at serine residue 727 (E) or at tyrosine residue 705 (F).

To assess the phosphorylation sites of Stat1 and Stat3 further, we reprobed the membrane with the antibodies specificallyrecognizing either Stat1 phosphorylated at Tyr-701 or Stat3 phosphorylatedat Tyr-705. We detected the phosphorylation of these tyrosineresidues in Stat1 and Stat3 (Fig. 3, D and F). These results indicatethat Src phosphorylates Stat1 and Stat3 (including both Stat3 $alpha$ and Stat3 $beta$ ) at specific tyrosine sites that are required for dimerization.We also observed that Stat1 and Stat3 $alpha$ are phosphorylated at Ser-727of both proteins, as detected by antibodies against phosphoserine727-Stat1 (Fig. 3C, lanes 1 and 2) and phosphoserine 727-Stat3(Fig. 3E, lanes 3 and 4), respectively. Stat3 $beta$ lacks the Ser-727residue (47) and did not show this modification as expected(Fig. 3E, lanes 5 and 6). The constitutive phosphorylation ofserine residues in Stat1 and Stat3 $alpha$ has been observed previously(38), indicating that a constitutively active, endogenous insectcell serine/threonine kinase is involved in this modification.Tyr-701-phosphorylated Stat1 migrates slower than the non-Tyr-701-phosphorylatedStat1 (Fig. 3, B, C, and D, the top bands in lane 2). Tyr-705-phosphorylatedStat3 did not exhibit any shift inmobility.

Jak1 Enhances Stat1 Activation Induced by Src-- Since Jak1 is highly activated in Src-transformed NIH3T3 cells (30), we investigated the involvement of Jak1 in the activationof Stat1 and Stat3 induced by v-Src in Sf-9 insect cells. Stat1was phosphorylated in the presence of either Jak1 or Src in Sf-9cells (Fig. 4A, lanes 4 and 5), indicating that both Src and Jak1can use Stat1 as a substrate. Stat1 phosphorylation was enhancedsignificantly when expressed in combination with both Jak1 andSrc (Fig. 4A, lane 6), and the majority of Stat1 shifted to aslower migrating form (compare lanes 4 and 5 with lane 6 in theStat1 panel). Phosphorylation levels of Jak1 were also increasedin the presence of Src (Fig. 4A, lane 6). This enhanced phosphorylationlevel of Jak1 may result in increased kinase activity toward Stat1,since JAK kinases are activated by transphosphorylation (4).In contrast, Stat3 was weakly activated by Jak1 compared withSrc in Sf-9 cells (Fig. 4B). Co-expression of Jak1 and Src didnot significantly enhance Stat3 phosphorylation compared withSrc alone, although Jak1 was hyperphosphorylated in the presenceof Src (Fig. 4B, lanes 10 and 12). These data indicate the differentialinvolvement of Jak1 in phosphorylation of Stat1 and Stat3 in Sf-9cells. In addition, the EMSA analyses of Stat1 and Stat3 DNA bindingactivities induced by Jak1 in combination with or without Srcare consistent with these phosphorylation results (data not shown).

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Fig. 4. Co-expression of Jak1 with Src enhances Stat1 tyrosine phosphorylation in Sf-9 cells. Stat1, Stat3 $alpha$ , Jak1, and c-Src were expressed from recombinant baculovirus-infected Sf-9 insect cells, either alone or in the combinations indicated at the top. Approximately equal amounts of total Stat1 or Stat3 were used in lanes 4-6 and lanes 10-12, respectively, as estimated by Western blot analysis. The proteins identified by specific antibodies are indicated to the right of the immunoblot. Jak1 was detected with anti-Jak1 antibody, whereas phosphotyrosine-Jak1 (pY-Jak1) was detected after reprobing the membrane with PY-99 anti-phosphotyrosine antibody. Phosphotyrosine-Stat1 (pY-Stat1) and phosphotyrosine-Stat3 (pY-Stat3) were detected with the respective antibodies against Tyr-701-phosphorylated Stat1 and Tyr-705-phosphorylated Stat3. The expression levels of Stat1 and Stat3 were confirmed with antibodies against total Stat1 or Stat3 proteins. Src protein levels were detected with anti-Src antibodies.

Jak1 Is Essential for Stat3 Activation Induced by v-Src In NIH3T3 Cells-- The above results show that Src can activate both Stat1 and Stat3, while Jak1 activates Stat1 efficiently and Stat3 relativelyweakly in Sf-9 cells. Although Src is capable of directly activatingStat3, we investigated if the mechanism of Stat3 activation isthrough direct interaction with Src kinase independent of otherprotein-tyrosine kinases, such as JAK kinases, in mammalian cells.We examined the Stat3 activation by Src in the presence of eithera JAK kinase inhibitor, AG490, or a Src kinase inhibitor, PD180970,in NIH3T3 cells. AG490 has been shown to be selective for JAKfamily kinases and reported to not inhibit Src, Lck, Lyn, Btk,and Syk kinases at the levels tested (36), while PD180970 hasbeen shown to be selective for Src family kinases (37). We firsttested AG490 and PD180970 for their effects on Jak1 and Src kinaseactivities using in vitro kinase assays to which these compoundswere directly added. Normal NIH3T3 cells show a minimal basallevel of Jak1 kinase activity (Fig. 5A, lane 1), which is greatlyincreased in v-Src-transformed cells (lane 2) as previously reported(30). As shown in Fig. 5A, AG490 inhibits in vitro Jak1 autophosphorylationin a dose-dependent manner. At 10 µM of AG490, a majority of Jak1kinase activity is inhibited (Fig. 5A, lane 4), while at 50 µMthe Jak1 kinase activity is nearly completely abolished (lanes5 and 6). In contrast, the Src inhibitor, PD180970, has littleeffect on Jak1 kinase activity even at a high concentration (Fig.5A, lanes 7-9).

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Fig. 5. AG490 and PD180970 specifically inhibit Jak1 and Src kinases in vitro, respectively. Immunoprecipitated Jak1 and Src proteins from whole-cell lysates of normal and v-Src-transformed NIH3T3 cells were used in the in vitro kinase assays to which the JAK-selective inhibitor, AG490, or Src-selective inhibitor, PD180970, was added directly. A, equal amounts of Jak1 immunoprecipitates were incubated in each reaction and preincubated with various concentrations of the inhibitor as indicated for 5 min prior to the addition of 20 µCi of [ $gamma$ -³²P]ATP. The reaction products were then analyzed by SDS-PAGE and autoradiography. B, Src immunoprecipitates from NIH3T3/v-Src cells were divided equally and preincubated with or without various concentrations of PD180970. After a 10-min preincubation, 5 µg of acid-denatured enolase was added to each reaction as an exogenous substrate together with 10 µCi of [ $gamma$ -³²P]ATP. Lane 1 has no enolase added as a control. C, similar to B except that AG490 at various concentrations was used instead of PD180970, and AG1296, a specific inhibitor of PDGF-R, was used as a negative control. The positions of Jak1, Src, and enolase are indicated at the left. DMSO, Me₂SO.

We then tested the effectiveness and specificity of PD180970 using in vitro Src kinase assays to which inhibitor was directlyadded with an exogenous substrate, enolase. PD180970 exhibitsa dose-dependent inhibition of v-Src kinase activity (Fig. 5B),and Src kinase activity is inhibited nearly completely with 1-2µM of PD180970 (Fig. 5B, lanes 6 and 7). In contrast, AG490 hasno effect on Src kinase activity at 10 µM (Fig. 5C, lane 3); however,it does display partial inhibition at 50 µM and significant inhibitoryeffects on Src kinase activity at 100 µM (Fig. 5C, lanes 4 and5). The PDGF receptor tyrosine kinase inhibitor, AG1296, has noeffect on Src kinase even at 100 µM, a concentration at whichit potently inhibits PDGF receptor kinase activity (Fig. 5B, lane8) (42). In summary, AG490 and PD180970 can specifically inhibitJak1 and Src, respectively, within specified concentration rangeswhen added directly to in vitro kinaseassays.

We next examined whether inhibition of JAK kinases in vivo will affect Stat3 DNA-binding activity in fibroblasts stably transformedv-Src. NIH3T3 cells transformed with v-Src were treated in vivowith various concentrations of AG490 or PD180970. As shown inFig. 6, nuclear extracts prepared from v-Src-transformed NIH3T3cells exhibit dose-dependent responses to AG490 and PD180970 treatment.Most of the Stat3-DNA complexes are significantly inhibited byAG490 at 10 µM and totally abolished at 50 µM (Fig. 6, lanes 3and 5). The majority of Stat3 DNA binding ability was decreasedwith PD180970 at 0.5 µM (Fig. 6, lane 8), although no additionaldecrease was observed at 1 µM (Fig. 6, lane 9). These resultsdemonstrate that Stat3 activation is effectively inhibited byAG490 as well as by PD180970 in a dose-dependent manner. Importantly,the majority of Stat3 inhibition by these kinase inhibitors invivo is observed at concentrations of the inhibitors that arespecific for the JAK or Src kinases in vitro (compare Figs. 5and 6), particularly taking into consideration that the actualconcentrations of the inhibitors are probably lower in vivo thanin vitro at any given dosage level. These results suggest thatJAK kinases are required for Stat3 activation and that the activationof Stat3 is not mediated exclusively by Src kinase in v-Src-transformedNIH3T3 cells.

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Fig. 6. AG490 and PD180970 inhibit Stat3 DNA-binding in v-Src-transformed NIH3T3 cells. Nuclear extracts were prepared from v-Src-transformed NIH3T3 cells treated in vivo with AG490 or PD180970 at various concentrations as indicated for 24 h. Equal amounts of total protein from nuclear extracts were used for EMSA with radiolabeled hSIE. The position of Stat3-hSIE complexes is indicated at the left. The control lane has no added inhibitor, and Me₂SO (DMSO) is the solvent alone.

Since Jak1 is constitutively phosphorylated in v-Src-transformed NIH3T3 cells (30) and also phosphorylated in the presenceof the active Src in Sf-9 insect cells (see Fig. 4, lanes 6 and12), we examined the tyrosine phosphorylation of Jak1 in v-Src-transformedNIH3T3 cells after treatment in vivo with Src and Jak inhibitors.We observed that tyrosine phosphorylation of Jak1 in v-Src-transformedcells is effectively inhibited by the Src inhibitor PD180970 (1µM) (Fig. 7, lane 4). These results suggest that Jak1 is directlyphosphorylated by Src in v-Src-transformed NIH3T3 cells. Jak1tyrosine phosphorylation in vivo is only inhibited by AG490 at50 µM, a concentration at which both Jak1 and Src kinase activitiesmay be affected (Fig. 5C, lane 4). Thus, it is possible that bothSrc and Jak1 contribute to Jak1 tyrosine phosphorylation.

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Fig. 7. Jak1 phosphorylation in vivo is inhibited by PD180970 and AG490. NIH3T3/v-Src cells were treated in vivo with the indicated concentrations of PD180970 or AG490 for a total of 36 h with the addition of fresh inhibitor every 12 h. Whole-cell lysates were prepared, and equal amounts of lysates were used for immunoprecipitation with anti-Jak1 antibody. The immunoprecipitates were resolved by SDS-PAGE and transferred to a nitrocellulose membrane. Western blot analysis was performed using antibodies against phosphotyrosine (PY-99, upper row) or Jak1 (lower row). DMSO, Me₂SO.

Inhibition of Jak1 Blocks Gene Expression Induced by v-Src-- We further investigated the role of Jak1 in Stat3-mediated gene regulation induced by v-Src. We transiently transfected NIH3T3cells with a v-Src expression vector and the Stat3 responsivereporter plasmid, pLucTKS3, as described previously (26). pLucTKS3contains multiple copies of a Stat3-specific binding site derivedfrom the promoter of the human C-reactive protein gene (26,50). As shown in Fig. 8A, the JAK inhibitor, AG490, reducedStat3-mediated reporter gene expression induced by v-Src in adose-dependent manner, paralleling the inhibition of Stat3 DNAbinding activity by AG490 (Fig. 6).

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Fig. 8. Stat3-mediated gene regulation is inhibited by AG490 and dominant negative Jak1 cDNA. NIH3T3 cells were transiently transfected with the indicated plasmids. Luciferase activities were measured in cytosolic extracts prepared 48 h post-transfection and normalized to $beta$ -galactosidase activity as an internal control for transfection efficiency. A, NIH3T3 cells were transfected with pLucTKS3 reporter without or with v-Src expression plasmid, pMvSrc, and treated with either Me₂SO (DMSO) or various concentrations of AG490 as indicated. B, cells were transfected with pLucTKS3 reporter, pMvSrc, and either a vector expressing wild-type (wt) Jak1 or one expressing dominant negative (dn) Jak1 as indicated. Values shown in each panel are means ± S.D. of transfections performed in triplicate.

We next examined the effect of dominant negative Jak1 on Stat3-mediated gene expression (Fig. 8B). Transfection of the dominantnegative Jak1 (Jak1-dn) gene with the Src gene significantly reducedthe pLucTKS3 reporter gene expression. This reduction by Jak1-dncorrelated with the inhibition by AG490, suggesting that Jak1has an important role in regulating Stat3-mediated gene expressioninduced by Src. Transfection of the wild-type Jak1 gene alonedid not substantially stimulate the reporter gene expression,indicating that Jak1 is not sufficient without Src to induce Stat3activation, consistent with the finding that overexpression ofJak1 does not activate Stat3 in Sf-9 insect cells. Furthermore,co-transfection of wild-type Jak1 gene with the Src gene resultedin only a slight increase of reporter expression compared withSrc alone, suggesting that the endogenous levels of Jak1 are notlimiting for maximal induction of Stat3 by Src in NIH3T3 cells.Thus, while Jak1 plays a key role in regulating Stat3-mediatedgene activation induced by Src in NIH3T3 cells, the finding thatJak1 does not directly phosphorylate Stat3 efficiently in Sf-9cells suggests an indirect role for Jak1 in enhancing Stat3 phosphorylationbySrc.

Inactivation of Stat1 Is Not Due to Dephosphorylation-- Since Stat1 is phosphorylated by Src in Sf-9 cells, it is surprising that Stat1 activation is not detected in v-Src-transformedNIH3T3 cells. One possible explanation for this is that the phosphorylatedStat1 is rapidly dephosphorylated by a cellular phosphatase. Analternative possibility is that the Stat1 is not phosphorylatedbecause it is not accessible to v-Src or Jak1 (e.g. Stat1 andStat3 may employ different docking sites). To test the possibilitythat the lack of Stat1 activation in v-Src-transformed cells maybe the result of rapid dephosphorylation rather than inaccessibilityto the kinases, we used the phosphatase inhibitor sodium orthovanadate.We reasoned that if a phosphatase is responsible for rapid Stat1-dephosphorylationafter its activation by Src kinase, we should observe a significantincrease of phosphorylated Stat1 in the presence of this generalphosphatase inhibitor. We treated v-Src-transformed NIH3T3 cellswith increasing amounts of Na₃VO₄ for extended periods of timeand then compared the DNA binding activities of Stat1 and Stat3with equal amounts of nuclear extracts (Fig. 9). We did not observea significant increase in the level of the activated Stat1 relativeto Stat3 in v-Src-transformed NIH3T3 cells (Fig. 9, lanes 4 and8). In contrast, normal NIH3T3 cells treated with Na₃VO₄ displayedan equal increase of Stat1 and Stat3 activation. Thus, in v-Src-transformedcells, lack of Stat1 activation is probably due to inaccessibilityto Src kinase rather than to a rapid dephosphorylation by phosphatases.

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Fig. 9. Phosphatase inhibitor does not significantly increase phosphorylated Stat1 relative to Stat3 in v-Src-transformed cells. Normal or v-Src-transformed NIH3T3 cells were treated in vivo with various concentrations of Na₃VO₄ as indicated for 3 h. Equal amounts of protein from nuclear extracts were used for EMSA with radiolabeled hSIE probe. The positions of Stat3-Stat3, Stat3-Stat1, and Stat1-Stat1 dimers bound to DNA are indicated at the left.

PDGF Receptor Is Required for Stat3 Activation by v-Src-- Since our initial observation of the association between Jak1 and Src (30), more recent studies have shown that PDGF receptor(PDGF-R), Src, and Stat3 form a multiprotein receptor complexin fibroblast cells (53). To examine the requirement for PDGF-Rin STAT activation induced by v-Src, we used the cell line 2fTGH,which is derived from the human fibrosarcoma HT1080 cell lineand lacks PDGF-R expression (17, 19). 2fTGH cells do not respondto PDGF stimulation unless transfected with PDGF-R expressionplasmid (17, 19). The 2fTGH cells were transfected with plasmidsexpressing either wild-type or kinase-inactive PDGF $beta$ -receptors(PDGF-R $beta$ ) and subsequently selected with G418 for stable transfectants.The transfected G418-resistant cells were pooled (to eliminateclonal variation) and transiently transfected with v-Src expressionvector. The activation of Stat3 DNA binding activity was measuredby EMSA. As shown in Fig. 10A, Stat3 is activated by v-Src in cellsstably transfected with either wild-type (WT) or kinase-dead (KD)PDGF-R $beta$ expression vectors (lanes 2 and 3). Stat3 was not activatedby v-Src in parental 2fTGH cells that were not transfected withPDGF-R $beta$ vectors (lane 1). Cells transfected with either wild-typeor kinase-dead PDGF-R $beta$ display similar levels of receptor expressionand Stat3 activation (compare lanes 2 and 3, EMSA and Blot). Thus,the presence of PDGF-R protein, independent of receptor kinaseactivity, plays a major role in Stat3 activation induced by v-Srcin human 2fTGH cells.

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Fig. 10. PDGF receptor is required for maximal Stat3 activation induced by v-Src. A, 2fTGH cells were transfected with plasmids expressing either wild-type (WT) or kinase-dead (KD) PDGF-R $beta$ and selected in G418. Pooled, stably transfected G418-resistant cells were then transiently transfected with 4 µg of v-Src expression vector. Nuclear extracts were prepared, normalized, and assayed by EMSA for DNA binding activity with ³²P-labeled hSIE probe (upper panel). The corresponding cytosolic extracts containing 2 mg of total protein were used for immunoprecipitation with anti-PDGF-R $beta$ antibodies, followed by Western blot analysis with antibodies against PDGF-R $beta$ (lower panel). The control (Cont) lane represents empty vector-transfected cells. B, NIH3T3 cells were transiently transfected with pLucTKS3 reporter, v-Src expression vector, and vectors expressing either wild-type (WT) or kinase-dead (KD) PDGF-R $beta$ as indicated. Luciferase activities were measured in cytosolic extracts prepared 48 h post-transfection and normalized to $beta$ -galactosidase activity as an internal control for transfection efficiency. Values shown are means ± S.D. of transfections performed in triplicate.

We next investigated the role of PDGF-R $beta$ in Stat3-mediated gene regulation induced by v-Src in NIH3T3 cells. We transientlytransfected NIH3T3 cells with a v-Src expression vector, the Stat3-responsivereporter plasmid pLucTKS3, and a plasmid expressing either wild-typeor kinase-dead PDGF-R $beta$ . Consistent with the results obtained in2fTGH cells, transfection of both wild-type and kinase-dead PDGF-R $beta$ further enhances the Stat3-mediated reporter activity inducedby v-Src (Fig. 10B). Unlike the 2fTGH cells, NIH3T3 cells expressendogenous levels of PDGF-R $beta$ , and therefore ectopic expressionof the receptor is not essential although it enhances Stat3 activation.This result confirms that maximal activation of Stat3 by v-Srcrequires the expression of PDGF-R $beta$ protein, which may serve ascaffolding function for Stat3 recruitment and activation. However,our results do not exclude the possibility that other receptorsmay substitute for PDGF-R in providing this scaffoldingfunction.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

While constitutive activation of Stat3 signaling has previously been shown to be required for cell transformation by the oncogenicSrc tyrosine kinase (26, 27), the mechanism of Stat3 activationby Src was not entirely clear. Our results presented here demonstratethat maximal activation of Stat3 requires Jak1 and PDGF-R in v-Src-transformedNIH3T3 cells, indicating that the mechanism of Stat3 activationinduced by oncogenic Src is more complex than a simple interactionbetween Stat3 and Src. However, in Sf-9 insect cells, Src is muchmore efficient than Jak1 at phosphorylating Stat3, arguing thatJak1 is not acting as an intermediary kinase between Src and Stat3.Furthermore, the role of PDGF-R in Stat3 activation by Src inNIH3T3 cells does not require the receptor's intrinsic tyrosinekinase activity. Based on our findings, we propose that the oncogenicSrc kinase activates Jak1 kinase, which in turn phosphorylatestyrosine sites on PDGF-R and possibly other receptors that providedocking sites for Stat3 (Fig. 11). In this model, activation ofJak1 is required for the recruitment of Stat3 proteins into areceptor complex with Src kinase, which then directly phosphorylatesStat3 at Tyr-705. Our model is consistent with the earlier findingsthat Stat3 is co-immunoprecipitated with Src (24, 25) andthat Jak1 is constitutively activated in Src transformed cells(30).

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Fig. 11. Model for the cooperative action of Jak1 and Src on Stat3 activation. In this model, Src phosphorylates and activates Jak1 (step 1), activated Jak1 phosphorylates the cytoplasmic tail of a membrane receptor (step 2), phosphotyrosine on the receptor acts as a docking site for recruiting cytoplasmic Stat3 (step 3), Src phosphorylates and activates the recruited Stat3 (step 4), and activated Stat3 dimerizes and translocates to the nucleus (step 5). Note that one candidate receptor for this scaffolding function is PDGF-R, although other receptors may also serve this role.

Our data (Fig. 1) demonstrate that Src can efficiently activate Stat1 and Stat3, but not Stat5A, in Sf-9 cells in the absenceof other mammalian kinases, suggesting that Stat1 and Stat3 areimmediate substrates of Src. Although we cannot quantitativelycompare the phosphorylation levels of Stat1 and Stat3 with eachother, since different antibodies are used for each protein, wecan determine the phosphorylation status of these STAT proteins(Fig. 3). Either Stat5A is not a substrate of Src or else an additionalcomponent is required for its activation. This observation isconsistent with our previous findings that c-Fes activates Stat3but not Stat5A in Sf-9 cells (39) and that v-Src does not activateStat5 in NIH3T3 cells (43). Furthermore, the observation thatbaculovirus-expressed Bcr-Abl can activate Stat5A rules out thepossibility that Stat5A expressed in insect cells is resistantto activation (39). Although we could not exclude the possibleinvolvement of an insect equivalent of mammalian JAK kinase, theendogenous insect JAK counterpart would probably be expressedat very low levels compared with baculovirus-overexpressed STATand Src proteins. We did not observe a rate-limiting step in STATactivation by Src in insect cells, suggesting that low levelsof endogenous insect kinases are not involved in STAT activationby overexpressed Src. Moreover, co-expression of Jak1 did notsignificantly increase Stat3 activation by Src in Sf-9 cells,indicating that JAK family kinases are not a factor in Stat3 activationby Src in insectcells.

Several lines of evidence support our model shown in Fig. 11. First, we show in insect cells that Src is able to activate Stat1and Stat3 selectively, consistent with Src being the immediateupstream kinase for phosphorylation of Stat1 and Stat3. Second,Jak1 is unable to phosphorylate Stat3 efficiently, which is instriking contrast to the result that it phosphorylates Stat1 equallyas well as Src does. This finding suggests that Jak1 is unlikelyto be the kinase for Stat3 activation acting downstream of Srckinase in v-Src-transformed cells. Third, the JAK-selective inhibitor,AG490, and the Src-selective inhibitor, PD180970, significantlyinhibit Stat3 DNA binding activity in v-Src-transformed NIH3T3cells, which indicates a requirement for both Src and JAKs inStat3 activation. Fourth, Jak1 is hyperphosphorylated in the presenceof active Src in insect cells and NIH3T3 fibroblasts. In addition,inhibition of Src kinase activity by PD180970 abolishes Jak1 tyrosinephosphorylation in v-Src-transformed NIH3T3 cells. Since the tyrosinephosphorylation level of Jak1 has been found to correlate withits kinase activity (30), these results suggest that Jak1 isdirectly activated by Src in v-Src transformed NIH3T3 cells. Fifth,both AG490 and dominant negative Jak1 inhibit Stat3-mediated generegulation, further establishing a requirement of Jak1 for Stat3activation by Src in NIH3T3 cells. Sixth, the lack of Stat1 activationin v-Src-transformed fibroblast cells may be due to the inaccessibility(possibly resulting from the lack of Stat1-specific docking sites)to the kinases, which is consistent with the notion that membrane-boundreceptors contribute to the specificity of STAT signaling (4).Previous studies (24) have shown that Stat1 can be activatedby interferon- $gamma$ stimulation of v-Src-transformed NIH3T3 cells,indicating that the normal Jak1-Stat1 pathway is intact in v-Src-transformedfibroblasts. These findings point to different mechanisms foractivation of Stat1 and Stat3. One plausible reason why Stat1signaling is down-regulated in v-Src-transformed cells may bethat Stat1 is involved in growth-inhibitory and proapoptosis functions(51, 52).

In myeloid cells stimulated with interleukin-3, c-Src but not JAKs is required for activation of Stat3 (28), consistentwith a direct role for c-Src in Stat3 activation. Normal c-Srchas been shown to be activated in epidermal growth factor- andPDGF-stimulated cells and to interact with epidermal growth factorand PDGF receptors (17, 21, 29, 53). Furthermore, onerecent study (54) reported that the activation of STAT proteinsinduced by epidermal growth factor receptor is mediated by c-Src.Using a cell-free system, another recent study provided evidencefor differences between Stat1 and Stat3 activation by PDGF (19).In particular, JAK kinases are indispensable for Stat3 activationinduced by PDGF but not for Stat1 activation; however, these studiesdid not address the involvement of c-Src in activation of Stat1and Stat3 in response to PDGF stimulation (19). Other studieshave also suggested that c-Src activates Stat1 and Stat3 in PDGF-stimulatedNIH3T3 cells (22, 53), and a multiprotein complex containingPDGF-R, c-Src, and STAT proteins has been detected (53). Moreover,there is evidence that Src and JAK family kinases are both requiredfor PDGF-mediated Stat3 signaling in normal NIH3T3 cells (Ref.53; our unpublished results). Therefore, cooperation among Src,JAKs, and PDGF-R may be required for Stat3 activation in normalgrowth factor signaling events. We have shown that the expressionof PDGF-R is essential for maximal Stat3 activation induced byv-Src in mammalian cells (Fig. 10). Importantly, the intrinsictyrosine kinase activity of PDGF-R is not required for Stat3 activationby v-Src, consistent with the receptor's proposed role as a scaffoldingcomplex for recruitment of Stat3 into close proximity of Src.However, our findings do not exclude the possibility that otherreceptors may also provide this scaffold function for recruitmentand activation of Stat3 by v-Src.

The requirement of JAK kinases for STAT activation has been previously observed in other oncogenic signaling events (55).The inhibitor of JAK family kinases, AG490, blocks IL-6-dependentStat3 activation in human multiple myeloma tumor cells (8).In human mycosis fungoides tumor cell lines, Jak3 and Tyk2 arein a complex with Stat3 and are required for Stat3 activationas well as for cell growth (56). In the case of v-Abl-transformedcells, Jak1 is required for proliferation in BAF/3 cells (57).Direct interaction of Jak1 and v-Abl has been observed, and thisinteraction is essential for STAT activation (57). In v-Src-transformedNIH3T3 cells, Jak1, but not Jak2 or Tyk2, is important in Stat3activation by v-Src, since dominant negative Jak2 and Tyk2 didnot affect Stat3-mediated gene activation by v-Src.² By contrast, JAK kinases are neither activated nor required forBcr-Abl-induced STAT activation (12), and the activated Lckkinase can directly phosphorylate Stat3 (58). These findingssuggest that the requirement of JAK family kinases is dependenton the specific cell type as well as the particular oncogenicsignalsinvolved.

Consistent with the results presented here, recent studies demonstrate that both Src and JAK tyrosine kinases are requiredfor constitutive Stat3 activation in human breast cancer celllines.³ Inhibition of Src or JAKs by PD180970 or AG490, respectively,results in inactivation of Stat3 DNA binding activity and growthinhibition of these breast cancer cells. Thus, the cooperationbetween Src and JAK tyrosine kinases is important for the constitutiveStat3 activation in various cell types, including human tumorcell lines. Our findings provide evidence for a novel mechanismof Stat3 activation that requires cooperation of Src and Jak1kinase in v-Src-transformed mouse fibroblasts. In this model,Jak1 has a critical role in recruiting Stat3 to a receptor complexwith Src kinase, which in turn directly phosphorylates Stat3.This model may be relevant not only to oncogenic signaling bytyrosine kinases but also to normal growth factor receptorsignaling.

ACKNOWLEDGEMENTS

We thank members of the laboratory for stimulating discussions; Drs. David Frank, George Stark, Andrius Kazlauskas, and JamesIhle for providing valuable reagents; and the Moffitt Cancer Center'sMolecular Biology and Imaging CoreFacilities.

	FOOTNOTES

^* This work was supported by National Institutes of Health Grant CA55652 (to R. J.).The costs of publication of this articlewere defrayed in part by the payment of page charges. The articlemust therefore be hereby marked "advertisement" in accordancewith 18 U.S.C. Section 1734 solely to indicate thisfact.

^j To whom correspondence should be addressed: Molecular Oncology Program, Moffitt Cancer Center, 12902 Magnolia Dr., Tampa,FL 33612. Tel.: 813-979-6725; Fax: 813-632-1436; E-mail: richjove@moffitt.usf.edu.

Published, JBC Papers in Press, May 22, 2000, DOI 10.1074/jbc.M002383200

² Y. Zhang, J. Turkson, C. Carter-Su, T. Smithgall, A. Levitzki, A. Kraker, J. J. Krolewski, P. Medveczky, and R. Jove, unpublishedresults.

³ R. Garcia, J. Sun, T. L. Bowman, G. Niu, Y. Zhang, S. Minton, C. A. Muro-Cacho, N. N. Ku, R. Falcone, C. Cox, A. Kraker, A.Levitzki, S. Parsons, S. M. Sebti, and R. Jove, submitted forpublication.

ABBREVIATIONS

The abbreviations used are: STAT, signal transducers and activators of transcription; JAK, Janus kinase; PDGF, platelet-derived growth factor; PDGF-R, PDGF receptor; PBS, phosphate-buffered saline; EMSA, electrophoretic mobility shift assay.

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Activation of Stat3 in v-Src-transformed Fibroblasts Requires Cooperation of Jak1 Kinase Activity*

Activation of Stat3 in v-Src-transformed Fibroblasts Requires Cooperation of Jak1 Kinase Activity^*