Protein Tyrosine Phosphatase 2 (SHP-2) Moderates Signaling by gp130 but Is Not Required for the Induction of Acute-Phase Plasma Protein Genes in Hepatic Cells

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Kim, H.
	Articles by Baumann, H.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Kim, H.
	Articles by Baumann, H.

Previous Article | Next Article

Mol Cell Biol, March 1998, p. 1525-1533, Vol. 18, No. 3
0270-7306/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Protein Tyrosine Phosphatase 2 (SHP-2) Moderates Signaling by gp130 but Is Not Required for the Induction of Acute-Phase Plasma Protein Genes in Hepatic Cells

Hongkyun Kim,¹ Teresa S. Hawley,² Robert G. Hawley,² and Heinz Baumann¹^,^*

Department of Molecular and Cellular Biology, Roswell Park Cancer Institute, Buffalo, New York 14263,¹ and Oncology Gene Therapy Program, The Toronto Hospital, Toronto, Ontario M5G 2M1, Canada²

Received 29 August 1997/Returned for modification 30 September 1997/Accepted 17 November 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Signals propagated via the gp130 subunit of the interleukin-6 (IL-6)-type cytokine receptors mediate, among various cellularresponses, proliferation of hematopoietic cells and inductionof acute-phase plasma protein (APP) genes in hepatic cells. Hematopoieticgrowth control by gp130 is critically dependent on activationof both STAT3 and protein tyrosine phosphatase 2 (SHP-2). To investigatewhether induction of APP genes has a similar requirement for SHP-2,we constructed two chimeric receptors, G-gp130 and G-gp130(Y2F),consisting of the transmembrane and cytoplasmic domains of gp130harboring either a wild-type or a mutated SHP-2 binding site,respectively, fused to the extracellular domain of the granulocytecolony-stimulating factor (G-CSF) receptor. Rat hepatoma H-35cells stably expressing the chimeric receptors were generatedby retroviral transduction. Both chimeric receptors transmitteda G-CSF-induced signal characteristic of that triggered by IL-6through the endogenous gp130 receptor; i.e., both activated theappropriate JAK, induced DNA binding activity by STAT1 and STAT3,and up-regulated expression of the target APP genes, those for $alpha$ -fibrinogen and haptoglobin. Notwithstanding these similaritiesin the patterns of signaling responses elicited, mutation of theSHP-2 interaction site in G-gp130(Y2F) abrogated ligand-activatedreceptor recruitment of SHP-2 as expected. Moreover, the tyrosinephosphorylation state of the chimeric receptor, the associatedJAK activity, and the induced DNA binding activity of STAT1 andSTAT3 were maintained at elevated levels and for an extended periodof time in G-gp130(Y2F)-expressing cells following G-CSF treatmentcompared to that in cells displaying the G-gp130 receptor. H-35cells ectopically expressing G-gp130(Y2F) were also found to displayan enhanced sensitivity to G-CSF and a higher level of inductionof APP genes. Overexpression of the enzymatically inactive SHP-2enhanced the signaling by the wild-type but not by the Y2F mutantG-gp130 receptor. These results indicate that gp130 signalingfor APP gene induction in hepatic cells differs qualitativelyfrom that controlling the proliferative response in hematopoieticcells in not being strictly dependent on SHP-2. The data furthersuggest that SHP-2 functions normally to attenuate gp130-mediatedsignaling in hepatic (and, perhaps, other) cells by moderatingJAK action.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

The engagement of the JAK/STAT pathway by gp130, the common signal-transducing subunit of interleukin-6 (IL-6)-type cytokinereceptors, has been well established (30, 42, 43). The ligand-mediatedoligomerization of receptor subunits leads to the activation ofgp130-associated Janus protein tyrosine kinases (JAKs). This processis in part determined by the Box B1 and Box B2 motifs in the cytoplasmicgp130 domain. The activated JAKs mediate cross-phosphorylationas well as phosphorylation of gp130, in particular, at the fourBox B3 motifs, which then serve as docking elements for STAT1and STAT3 (42). The receptor-recruited STAT proteins are inturn subject to tyrosine phosphorylation, causing their dimerization,acquisition of DNA binding activity, and nuclear translocationfor action as transcriptional inducers of IL-6-responsive genes.Phosphorylation of additional receptor or JAK tyrosine residuesprovides binding sites for other SH-2 domain-containing signalingmolecules, such as protein tyrosine phosphatase 2 (SHP-2), SHC,and Src-related kinases (16, 25, 31, 32, 42, 47, 49).

Deletions and residue substitutions have defined the functional relevance of the Box B1, B2, and B3 motifs for controllingcellular functions. Some of these analyses have utilized the experimentalmodel of chimeric gp130 subunits, granulocyte colony-stimulatingfactor receptor (G-CSFR)-gp130 (5) or IL-5 receptor-gp130 (6),which permitted characterization of the signaling response independentof endogenous gp130. The data suggest that gp130 acts throughat least two separate pathways, one that depends on the Box B3element and involves STAT3 as a mediator and another that is independentof STAT3, appears to engage STAT5, and induces a restricted setof genes (27).

Analyses of gp130 domains involved in controlling proliferation and differentiation of hematopoietic cells have provided supportfor a model of multiple signaling pathways. The membrane-proximalregion, including Box B1 and B2, was noted to be sufficient forcell survival, whereas proliferation as well as differentiationrequires minimally one Box B3 motif and the activation of STAT3(14, 36). Additional mutations in gp130 have identified tyrosine759 (the second tyrosine located further downstream from Box B1and B2, termed Y2) as part of the binding sequence for SHP-2 (14).SHP-2 is a ubiquitous enzyme of 72 kDa that contains two SH-2domains and has been found to interact with a broad spectrum ofsignal-transducing molecules (1, 9, 11, 12, 19, 20,24, 28, 48). gp130-recruited SHP-2 has also proved to beinvolved in the transmission of a proliferative signal in varioushematopoietic cell model systems (8, 14, 36). These findingssuggested that STAT3 and SHP-2 are critical mediators of gp130signaling. A role of SHP-2 in mitogenic signaling was also demonstratedfor other hematopoietin receptors (48) and growth factor receptors(7, 51).

A major function of IL-6-type cytokine receptors in hepatic cells is the induction of acute-phase plasma protein (APP) genes(3, 15). The requirement of Box B3 of gp130 in this processhas been shown previously (26), but the relevance of the Y2-dependentsignaling function for the APP response has not yet been demonstrated.Therefore, by retroviral transduction, we established rat hepatomacells stably expressing chimeric G-CSFR-gp130 proteins with orwithout an intact SHP-2 binding site. Here, we report that theinduction of APP genes by gp130 signaling differs from gp130-mediatedgrowth control in that it is not abrogated by the Y2 mutation;instead, prevention of SHP-2 recruitment enhances the signalingreaction and responsiveness of the cells to the cytokine, in partby prolonging the activity of JAKs.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Cytokines and antibodies. Human recombinant IL-6 and G-CSF were gifts from Genetics Institute and Immunex (Seattle, Wash.), respectively. Insulin wasobtained from Sigma. Antisera against JAK1, JAK2, and TYK2 werepurchased from Upstate Biotechnology, Inc. (Lake Placid, N.Y.);anti-FLAG antibody (M2) was from Eastman Kodak (Rochester, N.Y.);anti-SHP-1 antibody (C-19) and anti-SHP-2 antibody (C-18) werefrom Santa Cruz Biotechnology, Inc. (Santa Cruz, Calif.); antiphosphotyrosine(PY20) and anti-STAT3 antibodies were from Transduction (Lexington,Ky.); and anti-phospho-STAT3 antibody was from New England Biolabs(Beverly, Mass.).

Plasmid construction and cell lines. To change tyrosine 759 to phenylalanine (Y2F) in the cytoplasmic domain of gp130, a substitution mutation was introduced byoverlap extension PCR with an oligonucleotide containing the desiredamino acid codon sequence. A C-terminal epitope (DYKDDDDK) ingp130 was created by introducing the FLAG sequence and terminationcodon at the end of gp130. All mutations were confirmed by sequenceanalysis. The chimeric receptors were constructed by insertingthe EcoRI-NotI fragment encoding the FLAG-tagged gp130 (aminoacid residues 561 to 874) into the EcoRI-NotI site of pSVsport1-G-CSFR,encoding the extracellular domain of G-CSFR (amino acid residues1 to 623), as previously described (5). The construct G-CSFR-gp130(wildtype)-FLAG was termed G-gp130, and G-CSFR-gp130(Y2F)-FLAG wastermed G-gp130(Y2F). To generate cell lines stably expressingthe chimeric receptors, G-gp130 and G-gp130(Y2F) were cloned intothe retroviral vector MINV (17). The receptor cDNA is expressedfrom the murine stem cell virus (MSCV) long terminal repeat ona bicistronic transcript which contains a downstream neomycinphosphotransferase (neo) gene linked via an internal ribosomeentry site from encephalomyocarditis virus. Recombinant MINV-G-gp130retroviruses were produced in PA317 packaging cells (33) (CRL9078; American Type Culture Collection). Rat hepatoma H-35 cells(clone T-7-18) (4) were transduced and selected by culturingin Dulbecco's modified essential medium containing 10% fetal calfserum and G418 (2 mg/ml) (50). Proliferating cells were clonedby limiting dilution. The initial pools of transduced H-35 cellsand individual clonal lines were screened for chimeric receptorexpression by immunoblotting with anti-FLAG antibodies and forG-CSF-stimulated APP expression. All cytokine treatments werecarried out in serum-free minimal essential medium.

To test the influence of overexpressed SHP-2 on gp130 signaling, the two chimeric constructs, G-gp130 and G-gp130(Y2F), wereinserted into the expression vector pDC containing the human cytomegalovirusimmediate-early gene promoter (35). The pcDNA3 vector (Invitrogen)containing the full-length murine phosphatase-inactive SHP-2 (SHP-2*),was generously provided by Gen-Sheng Feng (Walther Oncology Center,Indiana University School of Medicine, Indianapolis) and has beendescribed previously (52).

CAT assay. HepG2 cells were transfected by the calcium phosphate method (38). The DNA mixture consisted of the IL-6-responsive reportergene constructs of pHPX(5×IL-6RE)-CAT containing five tandem copiesof the STAT3-sensitive regulatory elements from the rat hemopexingene (18) (15 µg/ml) and the expression vectors for G-gp130or G-gp130(Y2F) (1 µg/ml) and for SHP-2* (4 µg/ml). The plasmidpIE-MUP (1 µg/ml) was included in all transfections as an internalmarker (39). The transfected subcultures were treated for 24h either with serum-free medium alone (control) or with mediumcontaining 100 ng of G-CSF or IL-6 per ml. The chloramphenicolacetyltransferase (CAT) activities were determined in seriallydiluted cell extracts to ensure measurements in the linear rangeof the enzyme assay. The activities were normalized to the amountsof immunodetectable major urinary protein derived from the transfectionmarker in each culture (5, 34). The normalized values forCAT activities were then expressed relative to the values in controlcultures in each experimental series (fold stimulation).

¹²⁵I-G-CSF binding assay. G-CSF was labeled with ¹²⁵I by the Iodobead method according to the instructions of the manufacturer (Pierce) and purified ona Sephadex G-25 column. The labeled G-CSF had a specific activityof 81,000 cpm/ng and was fully functional as judged from the abilityto induce APP expression in G-gp130-expressing H-35 cells. Bindingwas determined on confluent cell monolayers in six-well clusterplates by using 50 pM ¹²⁵I-G-CSF in phosphate-buffered saline with 1% bovine serum albuminalone or in the presence of 100 nM unlabeled G-CSF. After incubationfor 4 h at 4°C, the cultures were washed four times with 2 mlof binding buffer and two times with 2 ml of phosphate-bufferedsaline. The cells were solubilized in 0.1 N NaOH-0.1% sodium dodecylsulfate (SDS), and the radioactivity was measured in a gamma counter(Beckman). The radioactivity specifically competed for by coldG-CSF was taken as a measure of specific G-CSF binding activityand was calculated as ¹²⁵I-G-CSF molecules bound per cell. In each experimental series,the average number of cells per well was counted in extra wellsnot used for the radioactive-ligand binding assay but which hadbeen subjected to the same procedures as the assay cells. Thenumber of H-35 cells per confluent monolayer in one well was 2.1× 10⁶ ± 0.2 × 10⁶ (n = 36) and was highly consistent from experiment to experiment.

Electrophoretic mobility shift assay. (EMSA). Whole-cell extracts were prepared as described previously (40). The double-stranded DNA probe SIEm67 was used for detectingbinding activity of STAT1 and STAT3 (34, 40).

Immunoprecipitation and Western blotting. Before cytokine treatment, cells were incubated for 6 h in serum-free minimal essential medium. Then, cells were treated withmedium alone (control) or medium containing G-CSF (50 ng/ml) orIL-6 (10 ng/ml) for various lengths of time and lysed in modifiedradioimmunoprecipitation assay (RIPA) buffer (50 mM Tris-HCl [pH7.4], 1% Nonidet P-40, 0.25% sodium deoxycholate, 1 mM NaF, 1mM sodium orthovanadate, 1 µg of leupeptin and 1 µg of aprotininper ml, 1 mM phenylmethylsulfonyl fluoride, 10% glycerol). Thesoluble fraction after centrifugation at 15,000 × g for 10 minwas used for immunoprecipitation with the appropriate antibodies.The immune complexes were recovered with protein A-Sepharose orprotein G-Sepharose (Pharmacia) by incubating for 16 h and thenwere washed five times with modified RIPA buffer. Immunoprecipitatedproteins were separated on an SDS-7.5% polyacrylamide gel andtransferred to polyvinylidine difluoride membranes (Bio-Rad).Proteins on membranes were then reacted with antibodies, and immunecomplexes were visualized with horseradish peroxidase-conjugatedanti-mouse or anti-rabbit immunoglobulin G (Cappel) and enhancedchemiluminescence reagent (Amersham). Sequential immunoblottingreactions were performed following stripping of the membranesin 0.1 N glycine (pH 2.7) for 4 h. All data on coimmunoprecipitatedproteins shown in the figures in this paper were obtained by usingthe modified RIPA buffer containing Nonidet P-40 as the detergent.We have, however, performed complementary immunoprecipitationsby using RIPA buffer that contains 1% of the milder detergentBrij 96. The immunoprecipitates recovered with Brij-containingbuffers were comparable to those described below, but the electrophoreticgel analyses showed more-complex patterns, probably due to less-stringentwashing conditions achieved with Brij 96 (data not presented).

Northern hybridization. Total cellular RNA (25 or 5 µg) was separated on a 1.5% agarose-formaldehyde gel and blotted onto a positively charged nylonfilter (Schleicher and Schuell). cDNAs encoding the extracellulardomain of G-CSFR, rat haptoglobin, or rat $alpha$ -fibrinogen (3)were labeled with ³²P by using an oligolabeling kit (Pharmacia). Hybridizations wereperformed for 16 h at 65°C, and filters were washed in 2× SSC(1× SSC is 0.15 M NaCl plus 0.015 M sodium citrate)-0.2% SDS at65°C four times for 30 min each.

Quantitation of secreted plasma proteins. Aliquots (25 µl) of medium from H-35 cells treated with medium alone, G-CSF, or IL-6 for 24 h were analyzed by immunoelectrophoresisfor rat fibrinogen (2). The precipitation peaks were measuredby scanning and integrated by using the National Institutes ofHealth Image program, version 1.6. The data are expressed in arbitraryimmunoelectrophoretic units. The detection limit of the methodis <1 immunoelectrophoretic unit.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Stable expression of G-gp130 in hepatoma cells. H-35 cells transduced with retroviral vectors for G-gp130 and G-gp130(Y2F) yielded significant expression of the chimericreceptors. From several hundred individual clones tested, we selectedfor functional characterization those clones that showed an inductionof APP production by G-CSF treatment that was equal to or greaterthan that by IL-6. By comparing receptor expression detectableby anti-FLAG antibodies and induction of APP genes in the initialpools of transduced and G-418-selected cells and in individualclones, we noted that the magnitudes of APP gene induction weregenerally correlated with receptor levels (for example, see Fig.7). Similarly, clonal cell lines with different amounts of expressedreceptors showed a DNA binding activity of STAT proteins followingG-CSF treatment that correlated in most instances with the relativereceptor level and APP induction (data not shown). The few clonallines (<5% of all clones) that did not respond to G-CSF treatmentby a measurable induction of APPs had also undetectable amountsof transduced receptors. Interestingly, the cell lines with G-gp130(Y2F)showed consistently less receptor expression than those with G-gp130.This difference is demonstrated in Fig. 1 for two representativelines chosen for this study and termed H-35 G-gp130 and H-35 G-gp130(Y2F).The lines had been initially selected because of their comparablelevels of maximally G-CSF-induced APP expression. Parental H-35cells showed a low level of ¹²⁵I-G-CSF binding, although no G-CSFR mRNA could be detected byNorthern blot analysis (data not shown). The receptor-transducedcells displayed a significantly increased ligand binding activity,with cells expressing G-gp130 binding on average four times moreG-CSF than those expressing G-gp130(Y2F). Northern blot analysisconfirmed the differences in expression determined by the ligandbinding assay. However, there was only a twofold difference inthe mRNA hybridization signals (Fig. 1, upper panel), suggestingsome effect of the Y2F mutation on posttranslational receptorprocessing (see also the severalfold difference in immunodetectablereceptor proteins in Fig. 2B).

View larger version (32K):
[in this window]
[in a new window]

FIG. 1. Expression of G-gp130 forms in H-35 cells. (Upper panel) Total cellular RNAs (5 µg) from parental H-35 cells and from the transduced clonal lines G-gp130 and G-gp130(Y2F) were analyzed by Northern blot hybridization. The hybridization of the G-CSFR probe to the fusion transcripts MSCV-G-gp130/IRES-neo at 7 kb (3-day exposure) and ethidium bromide (EtBr)-stained 18S rRNA of the separated RNA are shown. (Lower panel) Binding of ¹²⁵I-G-CSF to the same cell cultures was determined by the single-point binding assay. The specific ¹²⁵I-G-CSF binding was calculated as sites per cell (means ± standard deviations of three separate measurements).

The expression of functional receptor proteins was assessed by the G-CSF-induced activation of STAT proteins (Fig. 2A) andphosphorylation of receptor and binding of SHP-2 to G-gp130 butnot G-gp130(Y2F) (Fig. 2B). The specificity of the cell responseand of the biochemical analytical techniques was demonstratedby comparing the transduced cells with parental H-35 cells andby comparing the effects of G-CSF and IL-6. Although parentalH-35 cells exhibited a low level of G-CSF binding, treatment withG-CSF did not result in any detectable activation of DNA bindingactivity of STAT1 and STAT3 (Fig. 2A). In both transduced celllines, a strong STAT activation that was comparable to that elicitedby IL-6 was observed. Immunoprecipitation of cell lysates withanti-FLAG antibody yielded receptor proteins with the expectedsize of 130 kDa. The antibody also recognized an endogenous cross-reactingprotein (Fig. 2B) with an apparent molecular size of 190 kDa.This protein conveniently served as internal marker for proteinloading (see Fig. 4). The immunoblot detection of G-gp130 proteinsby anti-FLAG antibody verified a severalfold-lower level of G-gp130(Y2F)compared to G-gp130.

View larger version (62K):
[in this window]
[in a new window]

FIG. 2. Identification of gp130 proteins and functions. (A) Parental and transduced H-35 cells were treated for 15 min as indicated. Whole-cell extracts were subjected to EMSA. Binding complexes with the SIE probe and positions of the specific STAT combinations are shown. (B) Lysates from the same cell cultures used in panel A were immunoprecipitated (IP) with anti-FLAG antibodies, and the recovered proteins were separated by SDS-polyacrylamide gel electrophoresis and sequentially reacted in Western blotting (WB) with antibodies against FLAG, phosphotyrosine, and SHP-2 (FLAG, PY, and SHP-2, respectively). H-35 cells contain a protein of 190 kDa (CRM) that cross-reacts with anti-FLAG antibodies.

G-CSF treatment led to tyrosine phosphorylation of the chimeric receptor that was detected by phosphotyrosine immunoblottingand recognized by the slower electrophoretic mobility of the anti-FLAG-detectedG-gp130 proteins (Fig. 2B). A similar phosphorylation-inducedchange in electrophoretic mobility was reported for the nativegp130, which showed an increase in the apparent molecular massfrom ~ 155 to ~170 kDa (30). As expected, G-CSF induced associationof SHP-2 with G-gp130 but not G-gp130(Y2F). Moreover, the dataalso demonstrated that there was no constitutive binding of SHP-2to G-gp130 and no IL-6-mediated modification of the G-gp130 forms.H-35 cells express immunodetectable amounts of SHP-1; however,we could not detect the phosphorylation of SHP-1 by G-CSF or IL-6treatment, nor was the association of SHP-1 with anti-FLAG-immunoprecipitatedproteins from either G-gp130 or G-gp130(Y2F) cells observed (datanot shown).

Activation of signaling reaction. G-gp130-initiated signaling was compared to those of the endogenous receptors for IL-6 and insulin. The insulin response wasselected because, while ineffective at inducing the JAK/STAT pathway,insulin prominently activates the mitogen-activated protein kinase(MAPK) pathway (45) and involves SHP-2 (24). H-35 cells expressingG-gp130 and G-gp130(Y2F) responded to G-CSF and IL-6 by engagementof JAK1, STAT1, and STAT3 as detected by immunoprecipitation withantiphosphotyrosine antibodies (Fig. 3A). The somewhat strongerG-CSF response of the G-gp130 cells was attributed to the higherlevel of chimeric receptors in these cells. Phosphorylation ofSHP-2 was observed in G-gp130 but not G-gp130(Y2F) cells followingG-CSF treatment; this was higher than seen after IL-6 treatment,in correlation with the stronger signaling response. By comparison,insulin treatment did not yield significant tyrosine phosphorylationof the analyzed proteins or a significant association of theseproteins. However, SHP-2, probably through association with insulinreceptor substrate 1/2 (24), could be recovered from antiphosphotyrosineimmunoprecipitates of insulin-treated H-35 cells when these precipitateshad been prepared in Brij 96-containing buffers and subjectedto less-stringent washing conditions (data not shown; see alsoFig. 3B). SHP-2 receptor recruitment by each treatment was investigateddirectly by immunoprecipitation with anti-SHP-2 antibody (Fig.3B). The association of SHP-2 with G-gp130, but not with G-gp130(Y2F),was further demonstrated by the coprecipitation of only G-gp130with SHP-2 (Fig. 3B). The same analysis also illustrated thatthe cross-reactive material observed in the anti-FLAG immunoprecipitates(Fig. 2B) was not associated with the proteins recovered withthe anti-SHP-2 antibody.

View larger version (66K):
[in this window]
[in a new window]

FIG. 3. Comparison of the signaling reactions initiated by G-CSF, IL-6, and insulin. Monolayers of G-gp130 and G-gp130(Y2F) cells were treated for 10 min as indicated. (A) One half of the cell lysate was immunoprecipitated (IP) with antiphosphotyrosine antibody (PY). The immunoprecipitated proteins were analyzed sequentially by immunoblotting (WB) with antibodies against SHP-2, JAK1, STAT3, and STAT1. (B) The other half of the cell lysate was reacted with anti-SHP-2 antibodies, and the immunoprecipitated proteins were analyzed by sequential immunoblotting with antibodies against phosphotyrosine, FLAG, and SHP-2. In the upper panel, the positions of the several proteins are indicated only for reference. It is not proven whether the antiphosphotyrosine-immunoreactive bands shown represent the comigrating proteins. IgG, immunoglobulin G; IRS, insulin receptor substrate.

Loss of SHP-2 recruitment correlates with prolonged JAK action. To assess the potential effect of the Y2F mutation on signaling, we compared time-dependent changes of JAK phosphorylationin G-gp130 and G-gp130(Y2F) cells (Fig. 4A). In G-gp130 cells,maximal tyrosine phosphorylation of the receptors, JAK1, JAK2,and TYK2 was attained after a 5-min treatment with G-CSF, withrapid loss of signal by 30 min. A similar time course was obtainedfor JAK1 activation by IL-6 (Fig. 4A, bottom, and data not shown).In contrast, in G-CSF-treated G-gp130(Y2F) cells, elevated levelsof tyrosine-phosphorylated receptors and JAKs persisted for 30min before declining to basal levels.

View larger version (64K):
[in this window]
[in a new window]

FIG. 4. Time course of signaling by G-gp130 and G-gp130(Y2F). (A) Monolayers of the two transduced H-35 cell lines were treated for the indicated lengths of time with either G-CSF or IL-6. Separate cell lysates were immunoprecipitated (IP) with antibodies against FLAG, JAK1, or JAK2. The proteins were immunoblotted (WB) as indicated. PY, phosphotyrosine. (B) To determine turnover of G-gp130 proteins, monolayers of the two transduced cell lines were preincubated with cycloheximide (30 µg/ml) for 10 min, and then the cells were treated for the indicated lengths of time in the presence of cycloheximide with or without G-CSF. Cell lysates from each time point were immunoprecipitated with anti-FLAG antibodies, followed by immunoblot analysis of the proteins with anti-FLAG antibodies. The gel areas of G-gp130 proteins and cross-reacting material (CRM) are shown.

Since the distinct patterns of temporal changes in the phosphorylation of receptors and JAKs (Fig. 4A) could conceivably becaused by differences in ligand-induced receptor turnover, wemeasured immunodetectable G-gp130 proteins during the course ofcycloheximide treatment (Fig. 4B). In so far as this techniqueallowed an estimate of receptor amounts, the cellular concentrationsof both G-gp130 and G-gp130(Y2F) appeared to decline with roughlythe same kinetics, regardless of whether the cells had been treatedwith G-CSF. Most of the receptor proteins were lost by 90 min.Thus, relatively fast turnover of the chimeric receptors, ratherthan the specific action of a tyrosine phosphatase, may accountfor the loss of tyrosine-phosphorylated proteins noted after 1h of cytokine treatment (Fig. 4A).

Prolonged JAK activity enhances STAT activation. Observing that the inability of G-gp130(Y2F) to recruit SHP-2 resulted in prolonged JAK activity, we expected a correspondingprolongation or even an enhancement of STAT activation. Time courseanalysis of G-CSF treatment indeed indicated that the DNA bindingactivity of STAT1 and STAT3 (Fig. 5A) and the relative amountsof tyrosine-phosphorylated STAT3 (Fig. 5B) persisted longer inG-gp130(Y2F) cells than in G-gp130 cells. IL-6 treatment elicitedthe same relative temporal changes in STAT activity in both celltypes, which were essentially identical to those produced by G-CSFin G-gp130 cells. The higher STAT3 activity following a 24-h G-CSFtreatment in G-gp130 cells was tentatively attributed to the relativelyhigh level of the chimeric receptor in these cells.

View larger version (46K):
[in this window]
[in a new window]

FIG. 5. Time course of STAT protein activation and degradation. (A and B) Monolayers of the two transduced H-35 cell lines were treated for the indicated lengths of time with either G-CSF or IL-6. Whole-cell extracts were prepared and subjected to EMSA (A) or Western blot analysis for proteins reacting to anti-phosphotyrosine (PY)-STAT3 and STAT3 antibody (B). (C) Parental H-35 cells and H-35 cells expressing G-gp130 or G-gp130(Y2F) were preincubated for 10 min with cycloheximide (30 µg/ml) (0-h time point), and then treatment was started and continued for the indicated lengths of time in the presence of cycloheximide with or without cytokines. The cells were solubilized directly in SDS buffer. Equal aliquots of extracts were analyzed by immunoblotting by reaction first with anti-STAT3 antibody and, after stripping of the membrane, then with anti-phospho-STAT3 antibody.

The prolonged high STAT activity in G-gp130(Y2F) cells could be explained by (i) a prolonged tyrosine phosphorylation throughthe receptor-associated kinases that was not suppressed by SHP-2,(ii) a reduced dephosphorylation of receptor-recruited STATs bySHP-2, or (iii) a change in STAT protein turnover. Using the sameexperimental procedure for G-gp130 (Fig. 4B) except that cycloheximidetreatment was for 4 h, we determined the effect of SHP-2 recruitmenton the turnover of STAT3 and phospho-STAT3 proteins (Fig. 5C).The kinetic analysis indicated a half-life of immunodetectableSTAT3 of approximately 100 min in H-35 cells treated with or withoutcytokines. Although the measured STAT3 half-life was likely influencedby the prolonged treatment of cells with cycloheximide and showedno statistically significant differences, a minor IL-6- or G-CSF-inducedenhanced turnover of STAT3 seems to take place within the firsthours of treatment in cells not exposed to cycloheximide, as evidentfrom the reduced immunoblot signal for STAT3 in the extract fromcells after a 2-h treatment (Fig. 5B). Essentially the same timecourse of STAT3 reduction was detected in G-gp130 and G-gp130(Y2F)cells after either G-CSF or IL-6 treatment. The analysis alsorevealed that the cellular level of STAT3 increased again followingextended hours of treatment and even exceeded the level detectedin cells at 0 h. This increase was previously shown to be theresult of cytokine-induced STAT3 expression (10). Taking thesedata together, we interpret the elevated DNA binding activityof STATs (Fig. 5A) and the phosphotyrosine STAT3 level (Fig. 5B)to be the result of prolonged kinase activity and not of a slowerSTAT3 turnover.

Gene induction is enhanced in G-gp130(Y2F) cells. Regardless of the mechanism by which the level of activated STAT3 was enhanced in G-gp130(Y2F) cells, a corresponding effectwith regard to the regulation of APP genes was expected. Sincethe relative difference in activated STAT3 protein between G-gp130and G-gp130(Y2F) cells was most prominent after the initial phaseof cytokine treatment, we determined the mRNA levels of the markerAPPs, $alpha$ -fibrinogen and haptoglobin, after a 2-h treatment thatallowed for accumulation of sufficient mRNA to be detected byNorthern blot hybridization (Fig. 6A). Whereas IL-6 induced $alpha$ -fibrinogenand haptoglobin mRNAs in both cell lines to the same levels, G-CSFwas approximately twice as effective in G-gp130(Y2F) cells thanin G-gp130 cells, in agreement with the noted difference in STAT3activation in these cells. The greater induction of APP mRNA inG-gp130(Y2F) cells was also manifested in an enhanced sensitivityof the cells to G-CSF (Fig. 6B). For instance, 10 ng of G-CSFper ml induced a strong APP mRNA signal in G-gp130(Y2F) cellsbut not in G-gp130 cells. The comparison also indicated that theAPP genes were not identically regulated, in that $alpha$ -fibrinogenattained the same maximal mRNA level in both cell types afterG-CSF treatment, whereas the haptoglobin mRNA level in G-gp130(Y2F)cells was approximately twice that in G-CSF-treated G-gp130 cells.

View larger version (45K):
[in this window]
[in a new window]

FIG. 6. Induction of APP mRNA and CAT gene expression. (A) The two transduced H-35 cell lines were treated for 2 h with serum-free medium alone (control) or medium containing G-CSF or IL-6. Total cellular RNA (20 µg per lane) was analyzed by sequential Northern blot hybridization for the mRNAs for $alpha$ -fibrinogen ( $alpha$ -FB) and haptoglobin (HP). The autoradiograms are after a 24-h (HP) or 6-h ( $alpha$ -Fb) exposure. Equal RNA loading is indicated by the ethidium bromide (EtBr)-stained 18S rRNA bands. (B) Receptor-transduced H-35 cells were treated for 24 h with increasing doses of G-CSF. Total cellular RNAs (5 µg per lane) were analyzed as for panel A. In order to demonstrate the quantitative differences in hybridization signals, the autoradiographic image after a 6-h exposure is shown. (C) HepG2 cells were transfected with pHPX(5×IL-6RE)-CAT and the expression vectors for the chimeric receptors and SHP-2* as indicated. Subcultures were treated with the appropriate cytokines, and the fold inductions of the CAT activity were determined (means ± standard deviations of three determinations).

The data thus far suggested that the APP gene-inducing action of wild-type gp130 was moderated by the recruitment of SHP-2.Recently, Symes et al. (46) demonstrated that the phosphataseactivity of SHP-2 was necessary to achieve this moderating effecton gene induction in neuroblastoma cells. To assess whether thecatalytic activity of SHP-2 was also critical for G-gp130-mediatedinduction of genes via the STAT3-sensitive IL-6-responsive APPgene elements, we overexpressed the phosphatase-inactive SHP-2*together with the chimeric receptors and the pHPX(5×IL-6RE)-CATreporter gene in transfected HepG2 cells (Fig. 6C). HepG2 cellswere chosen for this assay because in this cell line, in contrastto in H-35 cells, a significantly larger overexpression of transfectedvectors can be achieved (22, 26, 27, 34). In agreementwith the prediction that enzymatically inactive SHP-2 acts asa dominant-negative protein (46), overexpression of SHP-2* enhancedthe gene-regulatory effects by endogenous IL-6 receptor and G-gp130.Also, as expected, SHP-2* was ineffective on the signaling bythe G-gp130(Y2F). The rather modest effects of the overexpressedSHP-2* may in part be explained by the relatively high levelsof endogenous SHP-2 proteins, which, based on comparative Westernblot data, were similar in HepG2 and H-35 cells (data not shown).The endogenous SHP-2 protein likely prevented an effective competitionby the transfected SHP-2* and thus yielded a result that was lessprominent than that seen in neuroblastoma cells (46).

The mRNA analysis, as well as the CAT regulation (Fig. 6), indicated a more prominent signaling action by G-gp130(Y2F) thanby G-gp130. The difference in the G-CSF dose response betweenthe two G-gp130 cell lines was more clearly seen in the amountsof APP secreted into the culture medium over the 24-h treatmentperiod (Fig. 7 shows fibrinogen as an example). The IL-6 responsesof the parental and the transduced cell lines proved to be essentiallyindistinguishable (Fig. 7 shows only the parental H-35 cells).While the G-CSF responses in the two transduced cell lines weresimilar, in that approximately 5 ng of G-CSF per ml was requiredfor half-maximal stimulation, the production of fibrinogen wasalready detectable in G-gp130(Y2F) cells at the lowest concentrationtested (0.01 ng/ml), and the maximal level of expression was somewhathigher. The data strongly suggest that the Y2F mutation of gp130had not appreciably altered the affinity of the chimeric receptorfor G-CSF interaction (i.e., the same concentration of G-CSF inducedthe half-maximal response) but enhanced the signaling activityof the receptor such that many fewer receptors were needed toattain the level of APP induction mediated by the wild-type receptor.This higher signaling action was highlighted by the comparisonof the APP response of the G-gp130(Y2F) cells with that of a separateclonal line of G-gp130 cells (clone 2 in Fig. 7) that expressedthe same amount of G-gp130 proteins as the G-gp130(Y2F) cells.While showing essentially the same G-CSF dose response as clone1 or the G-gp130(Y2F) cells, the magnitude of induction of fibrinogenwas threefold lower in this cell line.

View larger version (21K):
[in this window]
[in a new window]

FIG. 7. Cytokine-regulated production of fibrinogen. Parental H-35 cells and H-35 cell lines transduced with G-gp130(wild type) (clone 1 represents the line used in all previous experiments; clone 2 represents a separate line with four-times-lower G-gp130 expression) and G-gp130(Y2F) were grown to confluency in 24-well cluster plates. The cells were treated for 24 h with serum-free medium containing increasing concentrations of G-CSF or IL-6. Aliquots from the culture media were analyzed for the concentration of fibrinogen by immunoelectrophoresis (expressed in arbitrary immunoelectrophoretic units). The means ± standard deviations for three separate treatment series are shown.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

In this study, we attempted to identify the specific contribution of SHP-2 to the signaling by gp130 that controls inductionof IL-6-responsive APP genes in hepatic cells. The experimentalapproach was to examine the effect of mutating the suggested SHP-2binding site in the chimeric G-gp130 constructs that could betested in hepatoma cells independently of the endogenous gp130.The results showed that SHP-2 is recruited to gp130 upon activationby ligand binding. Prevention of this binding by the Y2F mutationled to an enhanced signaling response that was associated withprolonged phosphorylation of the receptors, JAK, and STATs, extendedDNA binding of the STAT proteins, and elevated transcription ofAPP genes. From this information, we conclude that in the wild-typegp130 the recruited SHP-2 attenuates the signaling intensity butthat SHP-2 is not essential for APP gene expression. A similarconclusion has been reached about the gp130-recruited SHP-2 inneuroblastoma cells to induce ciliary neurotrophic factor-sensitivegene constructs (46).

SHP-1, expressed exclusively in hematopoietic and epithelial cells, is thought to play a negative role in signal transductionof growth factors or cytokines, whereas SHP-2 has been suggestedas a positive regulator, in particular of proliferation (8,9, 14, 23, 28, 29, 48). Surprisingly, our data showthat SHP-2 recruited into gp130 can act as a negative regulatorof JAK in hepatoma cells. The specific effects of SHP-2 were determinedby eliminating its docking site on the receptor. The loss of SHP-2from immunoprecipitated G-gp130(Y2F) attested to the relevanceof the tyrosine residue (Y2) as being critical for binding ofSHP-2 through its SH-2 domain (14). It is less certain whetherthe G-gp130(Y2F) signaling in transduced H-35 cells is indeedindependent of SHP-2. An indirect recruitment of SHP-2 by tyrosine-phosphorylateddownstream substrates of gp130 action is conceivable, such asthat suggested in the case of insulin receptor action (12, 24).In fact, we noted a low-level recovery of a G-CSF-induced associationof SHP-2 with tyrosine-phosphorylated protein in G-gp130(Y2F)cells (Fig. 3B) that may arise from such an indirect pathway.

It has been suggested that SHP-2 serves as a link between the hematopoietin or growth factor receptors and the control ofcell proliferation. This connection is invariably associated withthe activation of the Raf-MAPK (ERK1 and -2) pathway. Abrogationof SHP-2 recruitment by gp130 has been seen to negatively affectproliferation of hematopoietic cells, which was in part correlatedwith lower MAPK activity (8, 14). However, truncated gp130forms that lack the SHP-2 binding site still deliver a detectableMAPK activation (36, 41) that is interpreted to account forminimal growth stimulation (36). Similarly, analysis of transducedG-gp130(Y2F) cells showed detectable ERK1 and ERK2 tyrosine phosphorylationfollowing G-CSF treatment, although the magnitude of activationwas much lower than that observed for G-gp130 cells (22a). Hence,while SHP-2 may play a role in engaging the MAPK pathway as partof the gp130 signaling, a critical contribution of the gp130-regulatedMAPK pathway to the induction of APP genes appears unlikely.

What is a conceivable mechanism of SHP-2 action in our more restricted experimental model of APP gene induction? Upon receptorengagement, the gp130 cytoplasmic domain, including the Y2 site,is phosphorylated in a ligand-dependent manner. The gp130-associatedJAKs are probably the principal kinases in this process. However,it has also been observed that members of other cellular proteintyrosine kinase families, including Fyn, Fes, and Tec, are associatedwith ligand-activated gp130 and may contribute to the gp130 phosphorylationprocess (30, 31, 48). After SHP-2 binds to the phosphorylatedY2 site, it may exert a phosphatase action on phosphorylated siteson gp130 and its associated factors, including JAKs and STATs.However, at present, there is no convincing experimental evidencethat the negative regulation is achieved by the phosphatase actionof SHP-2 on JAKs. Although the direct association of SHP-2 withJAK1 and JAK2 has been demonstrated in COS-1 cells overexpressingthese proteins, a reduced tyrosine phosphorylation of the JAKproteins was not evident in those analyses (52). Substrate specificityof SHP-2 appears to be determined by its association with thereceptor rather than by direct binding to a JAK or STAT, sincewe did not observe in our receptor-transduced hepatoma cell linean association of the endogenous SHP-2 with STAT3 or JAKs (datanot shown). Moreover, it is likely that SHP-2 is also a targetfor phosphorylation by gp130-associated kinases. Since the SHP-2that coprecipitated with gp130 barely reacted with antiphosphotyrosineantibody (22a), which is in contrast to the relatively strongsignal seen for tyrosine-phosphorylated SHP-2 recovered from thefraction that was not associated with gp130, we assume that SHP-2,once phosphorylated at the receptor site, disassociates from gp130and may associate with various cellular and membrane proteins(9, 19, 21, 28, 29).

Based on the observation that phosphorylation of JAKs is maintained longer in G-gp130(Y2F) cells (Fig. 4A), we intuitivelyassume that SHP-2 acts soon after signal initiation and explainsthe effects on the downstream targets of JAKs, e.g., STAT recruitmentand activation by phosphorylation. In fact, the consequence ofthe proposed SHP-2 action is equivalent to the negative-feedbackaction demonstrated for the JAK-associated protein inducible byIL-6 (13, 37, 44). The difference is that the moderatingaction of SHP-2 is practically immediate, whereas the JAK-associatedprotein first requires protein synthesis.

SHP-2 is not crucial for APP gene induction or for eventual down-regulation of the gp130 signal. Since IL-6 induction of APPgenes can be maintained for days (i.e., long after the dramaticchanges in phosphorylation of gp130, JAKs, and STATs are observedat signal initiation) (Fig. 4A and 5A), the influence of SHP-2on gp130 action is expected to continue, albeit at a much lower,barely detectable level. The fact that this process does takeplace is highlighted by the striking effect of the Y2F mutationon the APP level (Fig. 7). Even slightly enhanced gp130 signalingthat is maintained for 24 h leads to a significantly elevatedaccumulation of stable APP mRNA and, consequently, to a correspondingaccumulation of plasma protein in the medium. In conclusion, thisstudy has defined a component of the gp130 signal pathway thatdistinguishes the regulation of "differentiated" genes from thatof those that control cell proliferation.

	ACKNOWLEDGMENTS

We are greatly indebted to Immunex Corporation and Genetics Institute for their generous supply of cytokines, to D. Gearingfor providing the original chimeric G-CSFR-gp130 construct, toG.-S. Feng for the SHP-2* expression vectors, to Olivier Robledofor ¹²⁵I-G-CSF, and to Marcia Held for secretarial assistance.

This work was supported by NIH grant CA26122 to H.B. and by NCI grant 8398 to R.G.H.

	FOOTNOTES

^* Corresponding author. Mailing address: Roswell Park Cancer Institute, Department of Molecular and Cellular Biology, Elm andCarlton St., Buffalo, NY 14263. Phone: (716) 845-4587. Fax: (716)845-8389. E-mail: baumann{at}sc3101.med.buffalo.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Adachi, M., M. Ishino, T. Torigoe, Y. Minami, T. Matozaki, T. Miyazaki, T. Taniguchi, Y. Hinoda, and K. Imai. 1997. Interleukin-2 induces tyrosine phosphorylation of SHP-2 through IL-2 receptor beta chain. Oncogene 14:1629-1633[Medline].

2. Baumann, H., R. E. Hill, D. M. Sauder, and G. P. Jahreis. 1986. Regulation of major acute-phase plasma proteins by hepatocyte-stimulating factors of human squamous carcinoma cells. J. Cell. Biol. 102:370-383[Abstract/Free Full Text].

3. Baumann, H., C. Richards, and J. Gauldie. 1987. Interaction among hepatocyte-stimulating factors, interleukin 1 and glucocorticoid for regulation of acute phase plasma proteins in human hepatoma (HepG2) cells. J. Immunol. 139:1422-1428.

4. Baumann, H., K. R. Prowse, S. Marinkovic, K.-A. Won, and G. P. Jahreis. 1989. Stimulation of hepatic acute phase response by cytokines and glucocorticoids. Ann. N.Y. Acad. Sci. 557:280-295[Medline].

5. Baumann, H., A. J. Symes, M. R. Comeau, K. K. Morella, Y. Wang, D. Friend, S. F. Ziegler, J. S. Fink, and D. P. Gearing. 1994. Multiple regions within the cytoplasmic domains of the leukemia inhibitory factor receptor and gp130 cooperate in signal transduction in hepatic and neuronal cells. Mol. Cell. Biol. 14:138-146[Abstract/Free Full Text].

6. Behrmann, I., C. Janzen, C. Gerhartz, de L. H. Schmitz-Van, H. Hermanns, B. Heesel, L. Graeve, F. Horn, J. Tavernier, and P. C. Heinrich. 1997. A single STAT recruitment module in a chimeric cytokine receptor complex is sufficient for STAT activation. J. Biol. Chem. 272:5269-5274[Abstract/Free Full Text].

7. Bennett, A. M., S. F. Hausdorff, A. M. O'Reilly, R. M. Freeman, Jr., and B. G. Nell. 1996. Multiple requirements for SHPTP2 in epidermal growth factor-mediated cell cycle progression. Mol. Cell. Biol. 16:1189-1202[Abstract].

8. Berger, L. C., and R. G. Hawley. 1997. Interferon- $beta$ interrupts interleukin-6 dependent signaling events in myeloma cells. Blood 89:261-271[Abstract/Free Full Text].

9. Bone, H., U. Dechert, F. Jirik, J. W. Schrader, and M. J. Welham. 1997. SHP1 and SHP2 protein-tyrosine phosphatases associate with betac after interleukin-3-induced receptor tyrosine phosphorylation. J. Biol. Chem. 272:14470-14476[Abstract/Free Full Text].

10. Campos, S. P., Y. Wang, and H. Baumann. 1996. Insulin modulates STAT3 protein activation and gene in hepatic cells. J. Biol. Chem. 271:24418-24424[Abstract/Free Full Text].

11. Carlberg, K., and L. R. Rohrschneider. 1997. Characterization of a novel tyrosine phosphorylated 100-kDa protein that binds to SHP-2 and phosphatidylinositol 3'-kinase in myeloid cells. J. Biol. Chem. 272:15943-15950[Abstract/Free Full Text].

12. Case, R. D., E. Piccione, G. Wolf, A. M. Benett, R. J. Lechleider, B. G. Neel, and S. E. Shoelson. 1994. SH-PTP2/Syp SH2 domain binding specificity is defined by direct interactions with platelet-derived growth factor beta-receptor, epidermal growth factor receptor, and insulin receptor substrate-1-derived phosphopeptides. J. Biol. Chem. 269:10467-10474[Abstract/Free Full Text].

13. Endo, T. A., M. Masuhara, M. Yokouchi, R. Suzuki, H. Sakamoto, K. Mitsui, A. Matsumoto, S. Tanimura, M. Ohtsubo, H. Misawa, T. Miyazaki, N. Leonor, T. Taniguchi, T. Fujita, Y. Kanakura, S. Komiya, and A. Yoshimura. 1997. A new protein containing an SH2 domain that inhibits JAK kinases. Nature 387:921-924[Medline].

14. Fukada, T., M. Hibi, Y. Yamanaka, M. Takahashi-Tezuka, Y. Fujitani, T. Yamaguchi, K. Nakajima, and T. Hirano. 1996. Two signals are necessary for cell proliferation induced by a cytokine receptor gp130: involvement of STAT3 in antiapoptosis. Immunity 5:449-460[Medline].

15. Gauldie, J., C. Richards, D. Harnish, P. Lansdorp, and H. Baumann. 1987. Interferon- $beta$ ₂/BSF-2 shares identity with monocytoe derived hepatocyte stimulating factor (HSF) and regualtes the major acute phase protein response in liver cells. Proc. Natl. Acad. Sci. USA 84:7251-7255[Abstract/Free Full Text].

16. Giordano, V., G. De Falco, R. Chiari, I. Quinto, P. G. Pelicci, L. Bartholomew, P. Delmastro, M. Gadina, and G. Scala. 1997. Shc mediates IL-6 signaling by interacting with gp130 and Jak2 kinase. J. Immunol. 158:4097-4103[Abstract].

17. Hawley, R. G., F. H. Lieu, A. Z. Fong, S. J. Goldman, J. P. Leonard, and T. S. Hawley. 1996. Retroviral vectors for production of interleukin-12 in the bone marrow to induce a graft-versus-leukemia effect. Ann. N.Y. Acad. Sci. 795:341-345[Medline].

18. Immenschuh, S., Y. Nagae, H. Satoh, H. Baumann, and U. Muller-Eberhard. 1994. The rat and human hemopexin genes contain an identical interleukin-6 response element that is not a target of CAT enhancer-binding protein isoforms. J. Biol. Chem. 269:12654-12661[Abstract/Free Full Text].

19. Jackson, D. E., C. M. Ward, R. Wang, and P. J. Newman. 1997. The protein-tyrosine phosphatase SHP-2 binds platelet/endothelial cell adhesion molecule-1 (PECAM-1) and forms a distinct signaling complex during platelet aggregation. J. Biol. Chem. 272:6986-6993[Abstract/Free Full Text].

20. Kazlauskas, A., G.-S. Feng, T. Pawson, and M. Valius. 1993. The 64-kDa protein that associates with the platelet-derived growth factor receptor $beta$ subunit via Tyr-1009 is the SH-2 containing phosphotyrosine phosphatase Syp. Proc. Natl. Acad. Sci. USA 90:6939-6942[Abstract/Free Full Text].

21. Kharitonenkov, A., Z. Chen, I. Sures, H. Wang, J. Schilling, and A. Ullrich. 1997. A family of proteins that inhibit signalling through tyrosine kinase receptors. Nature 386:181-186[Medline].

22. Kim, H., and H. Baumann. 1997. The carboxyl-terminal region of STAT3 controls gene induction by the mouse haptoglobin promoter. J. Biol. Chem. 272:14571-14579[Abstract/Free Full Text].

22a. Kim, H., and H. Baumann. Unpublished data.

23. Klingmuller, U., U. Lorenz, L. C. Cantley, B. G. Neel, and H. F. Lodish. 1995. Specific recruitment of SH-PTP1 to the erythropoietin receptor causes inactivation of JAK2 and termination of proliferative signals. Cell 80:729-738[Medline].

24. Kuhne, M. R., T. Pawson, G. E. Lienhard, and G.-S. Feng. 1993. The insulin receptor substrate 1 associates with the SH-2 containing phophotyrosine phosphatase Syp. J. Biol. Chem. 268:11479-11481[Abstract/Free Full Text].

25. Kumar, G., S. Gupta, S. Wang, and E. Nel. 1994. Involvement of Janus kinases, p52^shc, Raf-1, and MEK-1 in the IL-6 induced mitogen-activated protein kinase cascade of growth responsive B cell line. J. Immunol. 152:4436-4447.

26. Lai, C.-F., J. Ripperger, K. K. Morella, Y. Wang, D. P. Gearing, G. H. Fey, and H. Baumann. 1995. Separate signaling mechanisms are involved in the control of STAT protein activation and gene regulation via the interleukin 6 response element by the box 3 motif of gp130. J. Biol. Chem. 270:14847-14850[Abstract/Free Full Text].

27. Lai, C.-F., J. Ripperger, K. K. Morella, Y. Wang, D. P. Gearing, N. D. Horseman, S. P. Campos, G. H. Fey, and H. Baumann. 1995. STAT3 and STAT5B are targets of two different signal pathways activated by hematopoietin receptors and control transcription via separate cytokine response elements. J. Biol. Chem. 270:23254-23257[Abstract/Free Full Text].

28. Li, W., R. Nishimura, A. Kashishian, A. G. Batzer, W. J. Kim, J. A. Cooper, and J. Schlessinger. 1994. A new function for a phosphotyrosine phosphatase: linking GRB2-Sos to a receptor tyrosine kinase. Mol. Cell. Biol. 14:509-517[Abstract/Free Full Text].

29. Liu, L., J. E. Damen, M. D. Ware, and G. Krystal. 1997. Interleukin-3 induces the association of the inositol 5-phosphatase SHIP with SHP2. J. Biol. Chem. 272:10998-11001[Abstract/Free Full Text].

30. Lutticken, C., U. M. Wegenka, J. Yuan, J. Buschmann, C. Schindle, A. Ziemiecki, A. G. Harpur, A. F. Wilks, K. Yasukawa, T. Taga, and T. Kishimoto. 1994. Association of transcription factor APRF and protein kinase Jak1 with the interleukin-6 signal transducer gp130. Science 263:89-92[Abstract/Free Full Text].

31. Matsuda, T., T. Fukada, M. Takahashi-Tezuka, Y. Okuyama, Y. Fujitani, Y. Hanazono, H. Hirai, and T. Hirano. 1995. Activation of Fes tyrosine kinase by gp130, an interleukin-6 family cytokine signal transducer, and their association. J. Biol. Chem. 270:11037-11039[Abstract/Free Full Text].

32. Matsuda, T., M. Takahashi-Tezuka, T. Fukada, Y. Okuyama, Y. Fujitani, S. Tsukada, H. Mano, H. Hirai, O. N. Witte, and T. Hirano. 1995. Association and activation of Btk and Tec tyrosine kinases by gp130, a signal transducer of the interleukin-6 family of cytokines. Blood 85:627-633[Abstract/Free Full Text].

33. Miller, A. D., and C. Buttimore. 1986. Redesign of retrovirus packaging cell lines to avoid recombination leading to helper virus production. Mol. Cell. Biol. 6:2895-2902[Abstract/Free Full Text].

34. Morella, K. K., C.-F. Lai, S. Kumaki, N. Kumaki, Y. Wang, E. M. Bluman, B. A. Witthuhn, J. N. Ihle, J. Giri, D. P. Gearing, D. Cosman, S. F. Ziegler, D. J. Tweardy, S. P. Campos, and H. Baumann. 1995. The action of interleukin-2 receptor subunits defines a new type of signaling mechanism for hematopoietic receptors in hepatic cells and fibroblasts. J. Biol. Chem. 270:8298-8310[Abstract/Free Full Text].

35. Mosley, B., M. P. Beckmann, C. J. March, R. L. Idzerda, S. D. Gimpel, T. Vanden Bos, D. Friend, D. Anderson, J. Jackson, J. M. Wignall, C. Smith, B. Gallis, J. E. Sims, D. Urdal, M. B. Widmer, and D. Cosman. 1989. The murine interleukin-4 receptor: molecular cloning and characterization of secreted and membrane bound forms. Cell 59:335-348[Medline].

36. Murakami, M., M. Narazaki, M. Hibi, H. Yawata, K. Yasukawa, M. Hamaguchi, T. Taga, and T. Kishimoto. 1991. Critical cytoplasmic region of the interleukin 6 signal transducer gp130 is conserved in the cytokine receptor family. Proc. Natl. Acad. Sci. USA 88:11349-11353[Abstract/Free Full Text].

37. Naka, T., M. Narazaki, M. Hirata, T. Matsumoto, S. Minamoto, A. Aono, N. Nishimoto, T. Kajita, T. Taga, K. Yoshizaki, S. Akira, and T. Kishimoto. 1997. Structure and function of a new STAT-induced STAT inhibitor. Nature 387:924-929[Medline].

38. O'Mahoney, J. V., and T. E. Adams. 1994. Optimization of experimental variables influencing reporter gene expression in hepatoma cells following calcium phosphate transfection. DNA Cell Biol. 13:1227-1232[Medline].

39. Prowse, K. R., and H. Baumann. 1988. Hepatocyte-stimulating factor, beta-2 interferon, and interleukin-1 enhance expression of the rat alpha 1-acid glycoprotein gene via a distal upstream regulatory element. Mol. Cell. Biol. 8:42-51[Abstract/Free Full Text].

40. Sadowski, H. B., K. Shuai, J. E. Darnell, Jr., and M. Z. Gilman. 1993. A common nuclear signal transduction pathway activated by growth factor and cytokine receptors. Science 261:1739-1744[Abstract/Free Full Text].

41. Schiemann, W. P., J. L. Bartoe, and N. M. Nathanson. 1997. Box 3-independent signaling mechanisms are involved in leukemia inhibitory factor receptor alpha- and gp130-mediated stimulation of mitogen-activated protein kinase. J. Biol. Chem. 272:16631-16636[Abstract/Free Full Text].

42. Stahl, N., T. J. Farruggella, T. G. Boulton, Z. Zhong, J. E. Darnell, Jr., and G. D. Yancopoulos. 1995. Choice of STATs and other substrates specified by modular tyrosine-based motifs in cytokine receptors. Science 267:1349-1353[Abstract/Free Full Text].

43. Stahl, N., T. G. Boulton, T. Farruggella, N. Y. Ip, S. Davis, B. A. Witthuhn, F. W. Quelle, O. Silvennoinen, G. Barbieri, S. Pellegrini, et al. 1994. Association and activation of Jak-Tyk kinases by CNTF-LIF-OSM-IL-6 beta receptor components. Science 263:92-95[Abstract/Free Full Text].

44. Starr, R., T. A. Willson, E. M. Viney, L. J. Murray, J. R. Rayner, B. J. Jenkins, T. J. Gonda, W. S. Alexander, D. Metcalf, N. A. Nicola, and D. J. Hilton. 1997. A family of cytokine-inducible inhibitors of signalling. Nature 387:917-921[Medline].

45. Sturgill, T. W., L. B. Ray, E. Erikson, and J. L. Maller. 1988. Insulin-stimulated MAP-2 kinase phosphorylates and activates ribosomal protein S6 kinase II. Nature 334:715-718[Medline].

46. Symes, A., N. Stahl, S. A. Reeves, T. Farruggella, T. Servidei, T. Gearan, G. Yancopoulos, and J. S. Fink. 1997. The protein tyrosine phosphatase SHP-2 negatively regulates ciliary neurotrophic factor induction of gene expression. Curr. Biol. 7:697-700[Medline].

47. Takahashi-Tezuka, M., M. Hibi, Y. Fujitani, T. Fukada, T. Yamaguchi, and T. Hirano. 1997. Tec tyrosine kinase links the cytokine receptors to PI-3 kinase probably through JAK. Oncogene 14:2273-2282[Medline].

48. Tauchi, T., J. E. Damen, K. Toyama, G. S. Feng, H. E. Broxmeyer, and G. Krystal. 1996. Tyrosine 425 within the activated erythropoietin receptor binds Syp, reduces the erythropoietin required for Syp tyrosine phosphorylation, and promotes mitogenesis. Blood 87:4495-4501[Abstract/Free Full Text].

49. Wang, X. Y., D. K. Fuhrer, M. S. Marshall, and Y. C. Yang. 1995. Interleukin-11 induces complex formation of Grb2, Fyn, and Jak2 in 3T3L1 cells. J. Biol. Chem. 270:27999-28002[Abstract/Free Full Text].

50. Wang, Y., K. K. Kuropatwinski, D. W. White, T. S. Hawley, R. G. Hawley, L. A. Tartaglia, and H. Baumann. 1997. Leptin receptor action in hepatic cells. J. Biol. Chem. 272:16216-16223[Abstract/Free Full Text].

51. Xia, S., D. W. Rose, T. Sasuoka, H. Maegawa, T. R. Burke, P. P. Roller, S. E. Shoelson, and J. M. Olefsky. 1994. SYP(SH-PTP2) is a positive mediator of growth factor-stimulated signal transduction. J. Biol. Chem. 269:21244-21248[Abstract/Free Full Text].

52. Yin, T., R. Shen, G.-S. Feng, and Y.-C. Yang. 1997. Molecular characterization of specific interactions between SHP-2 phosphatase and JAK tyrosine kinases. J. Biol. Chem. 272:1032-1037[Abstract/Free Full Text].

This article has been cited by other articles:

Kalliolias, G. D., Ivashkiv, L. B. (2008). IL-27 Activates Human Monocytes via STAT1 and Suppresses IL-10 Production but the Inflammatory Functions of IL-27 Are Abrogated by TLRs and p38. J. Immunol. 180: 6325-6333 [Abstract] [Full Text]
Chattopadhyay, S., Tracy, E., Liang, P., Robledo, O., Rose-John, S., Baumann, H. (2007). Interleukin-31 and Oncostatin-M Mediate Distinct Signaling Reactions and Response Patterns in Lung Epithelial Cells. J. Biol. Chem. 282: 3014-3026 [Abstract] [Full Text]
Bard-Chapeau, E. A., Yuan, J., Droin, N., Long, S., Zhang, E. E., Nguyen, T. V., Feng, G.-S. (2006). Concerted Functions of Gab1 and Shp2 in Liver Regeneration and Hepatoprotection. Mol. Cell. Biol. 26: 4664-4674 [Abstract] [Full Text]
Sommer, U., Schmid, C., Sobota, R. M., Lehmann, U., Stevenson, N. J., Johnston, J. A., Schaper, F., Heinrich, P. C., Haan, S. (2005). Mechanisms of SOCS3 Phosphorylation upon Interleukin-6 Stimulation: CONTRIBUTIONS OF Src- AND RECEPTOR-TYROSINE KINASES. J. Biol. Chem. 280: 31478-31488 [Abstract] [Full Text]
Arnaud, M., Crouin, C., Deon, C., Loyaux, D., Bertoglio, J. (2004). Phosphorylation of Grb2-Associated Binder 2 on Serine 623 by ERK MAPK Regulates Its Association with the Phosphatase SHP-2 and Decreases STAT5 Activation. J. Immunol. 173: 3962-3971 [Abstract] [Full Text]
Jenkins, B. J., Grail, D., Inglese, M., Quilici, C., Bozinovski, S., Wong, P., Ernst, M. (2004). Imbalanced gp130-Dependent Signaling in Macrophages Alters Macrophage Colony-Stimulating Factor Responsiveness via Regulation of c-fms Expression. Mol. Cell. Biol. 24: 1453-1463 [Abstract] [Full Text]
Bode, J. G., Schweigart, J., Kehrmann, J., Ehlting, C., Schaper, F., Heinrich, P. C., Haussinger, D. (2003). TNF-{alpha} Induces Tyrosine Phosphorylation and Recruitment of the Src Homology Protein-Tyrosine Phosphatase 2 to the gp130 Signal-Transducing Subunit of the IL-6 Receptor Complex. J. Immunol. 171: 257-266 [Abstract] [Full Text]
Mahboubi, K., Kirkiles-Smith, N. C., Karras, J., Pober, J. S. (2003). Desensitization of Signaling by Oncostatin M in Human Vascular Cells Involves Cytoplasmic Tyr Residue 759 in gp130 but Is Not Mediated by Either Src Homology 2 Domain-containing Tyrosine Phosphatase 2 or Suppressor of Cytokine Signaling 3. J. Biol. Chem. 278: 25014-25023 [Abstract] [Full Text]
Lehmann, U., Schmitz, J., Weissenbach, M., Sobota, R. M., Hortner, M., Friederichs, K., Behrmann, I., Tsiaris, W., Sasaki, A., Schneider-Mergener, J., Yoshimura, A., Neel, B. G., Heinrich, P. C., Schaper, F. (2003). SHP2 and SOCS3 Contribute to Tyr-759-dependent Attenuation of Interleukin-6 Signaling through gp130. J. Biol. Chem. 278: 661-671 [Abstract] [Full Text]
Cebo, C., Durier, V., Lagant, P., Maes, E., Florea, D., Lefebvre, T., Strecker, G., Vergoten, G., Zanetta, J.-P. (2002). Function and Molecular Modeling of the Interaction between Human Interleukin 6 and Its HNK-1 Oligosaccharide Ligands. J. Biol. Chem. 277: 12246-12252 [Abstract] [Full Text]
Mahboubi, K., Pober, J. S. (2002). Activation of Signal Transducer and Activator of Transcription 1 (STAT1) Is Not Sufficient for the Induction of STAT1-dependent Genes in Endothelial Cells. COMPARISON OF INTERFERON-gamma AND ONCOSTATIN M. J. Biol. Chem. 277: 8012-8021 [Abstract] [Full Text]
Tanuma, N., Shima, H., Nakamura, K., Kikuchi, K. (2001). Protein tyrosine phosphatase epsilon C selectively inhibits interleukin-6- and interleukin- 10-induced JAK-STAT signaling. Blood 98: 3030-3034 [Abstract] [Full Text]
Deon, D., Ahmed, S., Tai, K., Scaletta, N., Herrero, C., Lee, I.-H., Krause, A., Ivashkiv, L. B. (2001). Cross-Talk Between IL-1 and IL-6 Signaling Pathways in Rheumatoid Arthritis Synovial Fibroblasts. J. Immunol. 167: 5395-5403 [Abstract] [Full Text]
Miura, K., Saini, S. S., Gauvreau, G., MacGlashan, D. W. Jr (2001). Differences in Functional Consequences and Signal Transduction Induced by IL-3, IL-5, and Nerve Growth Factor in Human Basophils. J. Immunol. 167: 2282-2291 [Abstract] [Full Text]
Bode, J. G., Fischer, R., Haussinger, D., Graeve, L., Heinrich, P. C., Schaper, F. (2001). The Inhibitory Effect of IL-1{beta} on IL-6-Induced {alpha}2-Macroglobulin Expression Is Due to Activation of NF-{kappa}B. J. Immunol. 167: 1469-1481 [Abstract] [Full Text]
Watanabe, S., Zeng, R., Aoki, Y., Itoh, T., Arai, K.-i. (2001). Initiation of polyoma virus origin-dependent DNA replication through STAT5 activation by human granulocyte-macrophage colony-stimulating factor. Blood 97: 1266-1273 [Abstract] [Full Text]
Stofega, M. R., Herrington, J., Billestrup, N., Carter-Su, C. (2000). Mutation of the SHP-2 Binding Site in Growth Hormone (GH) Receptor Prolongs GH-Promoted Tyrosyl Phosphorylation of GH Receptor, JAK2, and STAT5B. Mol. Endocrinol. 14: 1338-1350 [Abstract] [Full Text]
Anhuf, D., Weissenbach, M., Schmitz, J., Sobota, R., Hermanns, H. M., Radtke, S., Linnemann, S., Behrmann, I., Heinrich, P. C., Schaper, F. (2000). Signal Transduction of IL-6, Leukemia-Inhibitory Factor, and Oncostatin M: Structural Receptor Requirements for Signal Attenuation. J. Immunol. 165: 2535-2543 [Abstract] [Full Text]
Auernhammer, C. J., Melmed, S. (2000). Leukemia-Inhibitory Factor--Neuroimmune Modulator of Endocrine Function. Endocr. Rev. 21: 313-345 [Abstract] [Full Text]
Schmitz, J., Weissenbach, M., Haan, S., Heinrich, P. C., Schaper, F. (2000). SOCS3 Exerts Its Inhibitory Function on Interleukin-6 Signal Transduction through the SHP2 Recruitment Site of gp130. J. Biol. Chem. 275: 12848-12856 [Abstract] [Full Text]
Delahaye, L., Rocchi, S., Van Obberghen, E. (2000). Potential Involvement of FRS2 in Insulin Signaling. Endocrinology 141: 621-628 [Abstract] [Full Text]
Schmitz, J., Dahmen, H., Grimm, C., Gendo, C., Muller-Newen, G., Heinrich, P. C., Schaper, F. (2000). The Cytoplasmic Tyrosine Motifs in Full-Length Glycoprotein 130 Have Different Roles in IL-6 Signal Transduction. J. Immunol. 164: 848-854 [Abstract] [Full Text]
Paradis, H, Gendron, R. (2000). LIF transduces contradictory signals on capillary outgrowth through induction of stat3 and (P41/43)MAP kinase. J. Cell Sci. 113: 4331-4339 [Abstract]
Bode, J. G., Gatsios, P., Ludwig, S., Rapp, U. R., Haussinger, D., Heinrich, P. C., Graeve, L. (1999). The Mitogen-activated Protein (MAP) Kinase p38 and Its Upstream Activator MAP Kinase Kinase 6 Are Involved in the Activation of Signal Transducer and Activator of Transcription by Hyperosmolarity. J. Biol. Chem. 274: 30222-30227 [Abstract] [Full Text]
Kim, H., Baumann, H. (1999). Dual Signaling Role of the Protein Tyrosine Phosphatase SHP-2 in Regulating Expression of Acute-Phase Plasma Proteins by Interleukin-6 Cytokine Receptors in Hepatic Cells. Mol. Cell. Biol. 19: 5326-5338 [Abstract] [Full Text]
Lai, C.-f., Ripperger, J., Wang, Y., Kim, H., Hawley, R. B., Baumann, H. (1999). The STAT3-independent Signaling Pathway by Glycoprotein 130 in Hepatic Cells. J. Biol. Chem. 274: 7793-7802 [Abstract] [Full Text]
Kiuchi, N., Nakajima, K., Ichiba, M., Fukada, T., Narimatsu, M., Mizuno, K., Hibi, M., Hirano, T. (1999). STAT3 Is Required for the gp130-mediated Full Activation of the c-myc Gene. J. Exp. Med. 189: 63-73 [Abstract] [Full Text]
Myers Jr., M. G., Mendez, R., Shi, P., Pierce, J. H., Rhoads, R., White, M. F. (1998). The COOH-terminal Tyrosine Phosphorylation Sites on IRS-1 Bind SHP-2 and Negatively Regulate Insulin Signaling. J. Biol. Chem. 273: 26908-26914 [Abstract] [Full Text]
Sengupta, T. K., Talbot, E. S., Scherle, P. A., Ivashkiv, L. B. (1998). Rapid inhibition of interleukin-6 signaling and Stat3 activation mediated by mitogen

1.	Adachi, M., M. Ishino, T. Torigoe, Y. Minami, T. Matozaki, T. Miyazaki, T. Taniguchi, Y. Hinoda, and K. Imai. 1997. Interleukin-2 induces tyrosine phosphorylation of SHP-2 through IL-2 receptor beta chain. Oncogene 14:1629-1633[Medline].
2.	Baumann, H., R. E. Hill, D. M. Sauder, and G. P. Jahreis. 1986. Regulation of major acute-phase plasma proteins by hepatocyte-stimulating factors of human squamous carcinoma cells. J. Cell. Biol. 102:370-383[Abstract/Free Full Text].
3.	Baumann, H., C. Richards, and J. Gauldie. 1987. Interaction among hepatocyte-stimulating factors, interleukin 1 and glucocorticoid for regulation of acute phase plasma proteins in human hepatoma (HepG2) cells. J. Immunol. 139:1422-1428.
4.	Baumann, H., K. R. Prowse, S. Marinkovic, K.-A. Won, and G. P. Jahreis. 1989. Stimulation of hepatic acute phase response by cytokines and glucocorticoids. Ann. N.Y. Acad. Sci. 557:280-295[Medline].
5.	Baumann, H., A. J. Symes, M. R. Comeau, K. K. Morella, Y. Wang, D. Friend, S. F. Ziegler, J. S. Fink, and D. P. Gearing. 1994. Multiple regions within the cytoplasmic domains of the leukemia inhibitory factor receptor and gp130 cooperate in signal transduction in hepatic and neuronal cells. Mol. Cell. Biol. 14:138-146[Abstract/Free Full Text].
6.	Behrmann, I., C. Janzen, C. Gerhartz, de L. H. Schmitz-Van, H. Hermanns, B. Heesel, L. Graeve, F. Horn, J. Tavernier, and P. C. Heinrich. 1997. A single STAT recruitment module in a chimeric cytokine receptor complex is sufficient for STAT activation. J. Biol. Chem. 272:5269-5274[Abstract/Free Full Text].
7.	Bennett, A. M., S. F. Hausdorff, A. M. O'Reilly, R. M. Freeman, Jr., and B. G. Nell. 1996. Multiple requirements for SHPTP2 in epidermal growth factor-mediated cell cycle progression. Mol. Cell. Biol. 16:1189-1202[Abstract].
8.	Berger, L. C., and R. G. Hawley. 1997. Interferon- $beta$ interrupts interleukin-6 dependent signaling events in myeloma cells. Blood 89:261-271[Abstract/Free Full Text].
9.	Bone, H., U. Dechert, F. Jirik, J. W. Schrader, and M. J. Welham. 1997. SHP1 and SHP2 protein-tyrosine phosphatases associate with betac after interleukin-3-induced receptor tyrosine phosphorylation. J. Biol. Chem. 272:14470-14476[Abstract/Free Full Text].
10.	Campos, S. P., Y. Wang, and H. Baumann. 1996. Insulin modulates STAT3 protein activation and gene in hepatic cells. J. Biol. Chem. 271:24418-24424[Abstract/Free Full Text].
11.	Carlberg, K., and L. R. Rohrschneider. 1997. Characterization of a novel tyrosine phosphorylated 100-kDa protein that binds to SHP-2 and phosphatidylinositol 3'-kinase in myeloid cells. J. Biol. Chem. 272:15943-15950[Abstract/Free Full Text].
12.	Case, R. D., E. Piccione, G. Wolf, A. M. Benett, R. J. Lechleider, B. G. Neel, and S. E. Shoelson. 1994. SH-PTP2/Syp SH2 domain binding specificity is defined by direct interactions with platelet-derived growth factor beta-receptor, epidermal growth factor receptor, and insulin receptor substrate-1-derived phosphopeptides. J. Biol. Chem. 269:10467-10474[Abstract/Free Full Text].
13.	Endo, T. A., M. Masuhara, M. Yokouchi, R. Suzuki, H. Sakamoto, K. Mitsui, A. Matsumoto, S. Tanimura, M. Ohtsubo, H. Misawa, T. Miyazaki, N. Leonor, T. Taniguchi, T. Fujita, Y. Kanakura, S. Komiya, and A. Yoshimura. 1997. A new protein containing an SH2 domain that inhibits JAK kinases. Nature 387:921-924[Medline].
14.	Fukada, T., M. Hibi, Y. Yamanaka, M. Takahashi-Tezuka, Y. Fujitani, T. Yamaguchi, K. Nakajima, and T. Hirano. 1996. Two signals are necessary for cell proliferation induced by a cytokine receptor gp130: involvement of STAT3 in antiapoptosis. Immunity 5:449-460[Medline].
15.	Gauldie, J., C. Richards, D. Harnish, P. Lansdorp, and H. Baumann. 1987. Interferon- $beta$ ₂/BSF-2 shares identity with monocytoe derived hepatocyte stimulating factor (HSF) and regualtes the major acute phase protein response in liver cells. Proc. Natl. Acad. Sci. USA 84:7251-7255[Abstract/Free Full Text].
16.	Giordano, V., G. De Falco, R. Chiari, I. Quinto, P. G. Pelicci, L. Bartholomew, P. Delmastro, M. Gadina, and G. Scala. 1997. Shc mediates IL-6 signaling by interacting with gp130 and Jak2 kinase. J. Immunol. 158:4097-4103[Abstract].
17.	Hawley, R. G., F. H. Lieu, A. Z. Fong, S. J. Goldman, J. P. Leonard, and T. S. Hawley. 1996. Retroviral vectors for production of interleukin-12 in the bone marrow to induce a graft-versus-leukemia effect. Ann. N.Y. Acad. Sci. 795:341-345[Medline].
18.	Immenschuh, S., Y. Nagae, H. Satoh, H. Baumann, and U. Muller-Eberhard. 1994. The rat and human hemopexin genes contain an identical interleukin-6 response element that is not a target of CAT enhancer-binding protein isoforms. J. Biol. Chem. 269:12654-12661[Abstract/Free Full Text].
19.	Jackson, D. E., C. M. Ward, R. Wang, and P. J. Newman. 1997. The protein-tyrosine phosphatase SHP-2 binds platelet/endothelial cell adhesion molecule-1 (PECAM-1) and forms a distinct signaling complex during platelet aggregation. J. Biol. Chem. 272:6986-6993[Abstract/Free Full Text].
20.	Kazlauskas, A., G.-S. Feng, T. Pawson, and M. Valius. 1993. The 64-kDa protein that associates with the platelet-derived growth factor receptor $beta$ subunit via Tyr-1009 is the SH-2 containing phosphotyrosine phosphatase Syp. Proc. Natl. Acad. Sci. USA 90:6939-6942[Abstract/Free Full Text].
21.	Kharitonenkov, A., Z. Chen, I. Sures, H. Wang, J. Schilling, and A. Ullrich. 1997. A family of proteins that inhibit signalling through tyrosine kinase receptors. Nature 386:181-186[Medline].
22.	Kim, H., and H. Baumann. 1997. The carboxyl-terminal region of STAT3 controls gene induction by the mouse haptoglobin promoter. J. Biol. Chem. 272:14571-14579[Abstract/Free Full Text].
22a.	Kim, H., and H. Baumann. Unpublished data.
23.	Klingmuller, U., U. Lorenz, L. C. Cantley, B. G. Neel, and H. F. Lodish. 1995. Specific recruitment of SH-PTP1 to the erythropoietin receptor causes inactivation of JAK2 and termination of proliferative signals. Cell 80:729-738[Medline].
24.	Kuhne, M. R., T. Pawson, G. E. Lienhard, and G.-S. Feng. 1993. The insulin receptor substrate 1 associates with the SH-2 containing phophotyrosine phosphatase Syp. J. Biol. Chem. 268:11479-11481[Abstract/Free Full Text].
25.	Kumar, G., S. Gupta, S. Wang, and E. Nel. 1994. Involvement of Janus kinases, p52^shc, Raf-1, and MEK-1 in the IL-6 induced mitogen-activated protein kinase cascade of growth responsive B cell line. J. Immunol. 152:4436-4447.
26.	Lai, C.-F., J. Ripperger, K. K. Morella, Y. Wang, D. P. Gearing, G. H. Fey, and H. Baumann. 1995. Separate signaling mechanisms are involved in the control of STAT protein activation and gene regulation via the interleukin 6 response element by the box 3 motif of gp130. J. Biol. Chem. 270:14847-14850[Abstract/Free Full Text].
27.	Lai, C.-F., J. Ripperger, K. K. Morella, Y. Wang, D. P. Gearing, N. D. Horseman, S. P. Campos, G. H. Fey, and H. Baumann. 1995. STAT3 and STAT5B are targets of two different signal pathways activated by hematopoietin receptors and control transcription via separate cytokine response elements. J. Biol. Chem. 270:23254-23257[Abstract/Free Full Text].
28.	Li, W., R. Nishimura, A. Kashishian, A. G. Batzer, W. J. Kim, J. A. Cooper, and J. Schlessinger. 1994. A new function for a phosphotyrosine phosphatase: linking GRB2-Sos to a receptor tyrosine kinase. Mol. Cell. Biol. 14:509-517[Abstract/Free Full Text].
29.	Liu, L., J. E. Damen, M. D. Ware, and G. Krystal. 1997. Interleukin-3 induces the association of the inositol 5-phosphatase SHIP with SHP2. J. Biol. Chem. 272:10998-11001[Abstract/Free Full Text].
30.	Lutticken, C., U. M. Wegenka, J. Yuan, J. Buschmann, C. Schindle, A. Ziemiecki, A. G. Harpur, A. F. Wilks, K. Yasukawa, T. Taga, and T. Kishimoto. 1994. Association of transcription factor APRF and protein kinase Jak1 with the interleukin-6 signal transducer gp130. Science 263:89-92[Abstract/Free Full Text].
31.	Matsuda, T., T. Fukada, M. Takahashi-Tezuka, Y. Okuyama, Y. Fujitani, Y. Hanazono, H. Hirai, and T. Hirano. 1995. Activation of Fes tyrosine kinase by gp130, an interleukin-6 family cytokine signal transducer, and their association. J. Biol. Chem. 270:11037-11039[Abstract/Free Full Text].
32.	Matsuda, T., M. Takahashi-Tezuka, T. Fukada, Y. Okuyama, Y. Fujitani, S. Tsukada, H. Mano, H. Hirai, O. N. Witte, and T. Hirano. 1995. Association and activation of Btk and Tec tyrosine kinases by gp130, a signal transducer of the interleukin-6 family of cytokines. Blood 85:627-633[Abstract/Free Full Text].
33.	Miller, A. D., and C. Buttimore. 1986. Redesign of retrovirus packaging cell lines to avoid recombination leading to helper virus production. Mol. Cell. Biol. 6:2895-2902[Abstract/Free Full Text].
34.	Morella, K. K., C.-F. Lai, S. Kumaki, N. Kumaki, Y. Wang, E. M. Bluman, B. A. Witthuhn, J. N. Ihle, J. Giri, D. P. Gearing, D. Cosman, S. F. Ziegler, D. J. Tweardy, S. P. Campos, and H. Baumann. 1995. The action of interleukin-2 receptor subunits defines a new type of signaling mechanism for hematopoietic receptors in hepatic cells and fibroblasts. J. Biol. Chem. 270:8298-8310[Abstract/Free Full Text].
35.	Mosley, B., M. P. Beckmann, C. J. March, R. L. Idzerda, S. D. Gimpel, T. Vanden Bos, D. Friend, D. Anderson, J. Jackson, J. M. Wignall, C. Smith, B. Gallis, J. E. Sims, D. Urdal, M. B. Widmer, and D. Cosman. 1989. The murine interleukin-4 receptor: molecular cloning and characterization of secreted and membrane bound forms. Cell 59:335-348[Medline].
36.	Murakami, M., M. Narazaki, M. Hibi, H. Yawata, K. Yasukawa, M. Hamaguchi, T. Taga, and T. Kishimoto. 1991. Critical cytoplasmic region of the interleukin 6 signal transducer gp130 is conserved in the cytokine receptor family. Proc. Natl. Acad. Sci. USA 88:11349-11353[Abstract/Free Full Text].
37.	Naka, T., M. Narazaki, M. Hirata, T. Matsumoto, S. Minamoto, A. Aono, N. Nishimoto, T. Kajita, T. Taga, K. Yoshizaki, S. Akira, and T. Kishimoto. 1997. Structure and function of a new STAT-induced STAT inhibitor. Nature 387:924-929[Medline].
38.	O'Mahoney, J. V., and T. E. Adams. 1994. Optimization of experimental variables influencing reporter gene expression in hepatoma cells following calcium phosphate transfection. DNA Cell Biol. 13:1227-1232[Medline].
39.	Prowse, K. R., and H. Baumann. 1988. Hepatocyte-stimulating factor, beta-2 interferon, and interleukin-1 enhance expression of the rat alpha 1-acid glycoprotein gene via a distal upstream regulatory element. Mol. Cell. Biol. 8:42-51[Abstract/Free Full Text].
40.	Sadowski, H. B., K. Shuai, J. E. Darnell, Jr., and M. Z. Gilman. 1993. A common nuclear signal transduction pathway activated by growth factor and cytokine receptors. Science 261:1739-1744[Abstract/Free Full Text].
41.	Schiemann, W. P., J. L. Bartoe, and N. M. Nathanson. 1997. Box 3-independent signaling mechanisms are involved in leukemia inhibitory factor receptor alpha- and gp130-mediated stimulation of mitogen-activated protein kinase. J. Biol. Chem. 272:16631-16636[Abstract/Free Full Text].
42.	Stahl, N., T. J. Farruggella, T. G. Boulton, Z. Zhong, J. E. Darnell, Jr., and G. D. Yancopoulos. 1995. Choice of STATs and other substrates specified by modular tyrosine-based motifs in cytokine receptors. Science 267:1349-1353[Abstract/Free Full Text].
43.	Stahl, N., T. G. Boulton, T. Farruggella, N. Y. Ip, S. Davis, B. A. Witthuhn, F. W. Quelle, O. Silvennoinen, G. Barbieri, S. Pellegrini, et al. 1994. Association and activation of Jak-Tyk kinases by CNTF-LIF-OSM-IL-6 beta receptor components. Science 263:92-95[Abstract/Free Full Text].
44.	Starr, R., T. A. Willson, E. M. Viney, L. J. Murray, J. R. Rayner, B. J. Jenkins, T. J. Gonda, W. S. Alexander, D. Metcalf, N. A. Nicola, and D. J. Hilton. 1997. A family of cytokine-inducible inhibitors of signalling. Nature 387:917-921[Medline].
45.	Sturgill, T. W., L. B. Ray, E. Erikson, and J. L. Maller. 1988. Insulin-stimulated MAP-2 kinase phosphorylates and activates ribosomal protein S6 kinase II. Nature 334:715-718[Medline].
46.	Symes, A., N. Stahl, S. A. Reeves, T. Farruggella, T. Servidei, T. Gearan, G. Yancopoulos, and J. S. Fink. 1997. The protein tyrosine phosphatase SHP-2 negatively regulates ciliary neurotrophic factor induction of gene expression. Curr. Biol. 7:697-700[Medline].
47.	Takahashi-Tezuka, M., M. Hibi, Y. Fujitani, T. Fukada, T. Yamaguchi, and T. Hirano. 1997. Tec tyrosine kinase links the cytokine receptors to PI-3 kinase probably through JAK. Oncogene 14:2273-2282[Medline].
48.	Tauchi, T., J. E. Damen, K. Toyama, G. S. Feng, H. E. Broxmeyer, and G. Krystal. 1996. Tyrosine 425 within the activated erythropoietin receptor binds Syp, reduces the erythropoietin required for Syp tyrosine phosphorylation, and promotes mitogenesis. Blood 87:4495-4501[Abstract/Free Full Text].
49.	Wang, X. Y., D. K. Fuhrer, M. S. Marshall, and Y. C. Yang. 1995. Interleukin-11 induces complex formation of Grb2, Fyn, and Jak2 in 3T3L1 cells. J. Biol. Chem. 270:27999-28002[Abstract/Free Full Text].
50.	Wang, Y., K. K. Kuropatwinski, D. W. White, T. S. Hawley, R. G. Hawley, L. A. Tartaglia, and H. Baumann. 1997. Leptin receptor action in hepatic cells. J. Biol. Chem. 272:16216-16223[Abstract/Free Full Text].
51.	Xia, S., D. W. Rose, T. Sasuoka, H. Maegawa, T. R. Burke, P. P. Roller, S. E. Shoelson, and J. M. Olefsky. 1994. SYP(SH-PTP2) is a positive mediator of growth factor-stimulated signal transduction. J. Biol. Chem. 269:21244-21248[Abstract/Free Full Text].
52.	Yin, T., R. Shen, G.-S. Feng, and Y.-C. Yang. 1997. Molecular characterization of specific interactions between SHP-2 phosphatase and JAK tyrosine kinases. J. Biol. Chem. 272:1032-1037[Abstract/Free Full Text].