Association of Insulin Receptor Substrate 1 (IRS-1) Y895 with Grb-2 Mediates the Insulin Signaling Involved in IRS-1-Deficient Brown Adipocyte Mitogenesis

doi:10.1128/MCB.21.7.2269-2280.2001

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Molecular and Cellular Biology, April 2001, p. 2269-2280, Vol. 21, No. 7
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.7.2269-2280.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Association of Insulin Receptor Substrate 1 (IRS-1) Y895 with Grb-2 Mediates the Insulin Signaling Involved in IRS-1-Deficient Brown Adipocyte Mitogenesis

Angela M. Valverde,¹ Cecilia Mur,¹ Sebastián Pons,²^, Alberto M. Alvarez,³ Morris F. White,² C. Ronald Kahn,² and Manuel Benito¹^,^*

Departamento de Bioquímica y Biología Molecular, Centro Mixto CSIC/UCM, Facultad de Farmacia,¹ and Centro de Citometría de Flujo y Microscopía Confocal,³ Universidad Complutense, 28040 Madrid, Spain, and Joslin Diabetes Center, Harvard Medical School, Boston, Massachusetts²

Received 13 April 2000/Returned for modification 18 October 2000/Accepted 3 January 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

We have recently generated immortalized fetal brown adipocyte cell lines from insulin receptor substrate 1 (IRS-1) knockoutmice and demonstrated an impairment in insulin-induced lipid synthesisas compared to wild-type cell lines. In this study, we investigatedthe consequences of IRS-1 deficiency on mitogenesis in responseto insulin. The lack of IRS-1 resulted in the inability of insulin-stimulatedIRS-1-deficient brown adipocytes to increase DNA synthesis andenter into S/G₂/M phases of the cell cycle. These cells showeda severe impairment in activating mitogen-activated protein kinasekinase (MEK1/2) and p42-p44 mitogen-activated protein kinase (MAPK)upon insulin stimulation. IRS-1-deficient cells also lacked tyrosinephosphorylation of SHC and showed no SHC-Grb-2 association inresponse to insulin. The mitogenic response to insulin could bepartially restored by enhancing IRS-2 tyrosine phosphorylationand its association with Grb-2 by inhibition of phosphatidylinositol3-kinase activity through a feedback mechanism. Reconstitutionof IRS-1-deficient brown adipocytes with wild-type IRS-1 restoredinsulin-induced IRS-1 and SHC tyrosine phosphorylation and IRS-1-Grb-2,IRS-1-SHC, and SHC-Grb-2 associations, leading to the activationof MAPK and enhancement of DNA synthesis. Reconstitution of IRS-1-deficientbrown adipocytes with the IRS-1 mutant Tyr895Phe, which lacksIRS-1-Grb-2 binding, restored SHC-IRS-1 association and SHC-Grb-2association. However, the lack of IRS-1-Grb-2 association impairedMAPK activation and DNA synthesis in insulin-stimulated mutantcells. These data provide strong evidence for an essential roleof IRS-1 and its direct association with Grb-2 in the insulinsignaling pathway leading to MAPK activation and mitogenesis inbrownadipocytes.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

A complete understanding of insulin actions on cell growth and metabolism requires the identification of a complex networkof signaling pathways. Insulin initiates its biological effectsby binding to and activating its endogenous tyrosine kinase receptors(9, 28). These receptors are believed to transduce signalsby phosphorylation on tyrosine residues of several cellular substrates,including insulin receptor substrate (IRS) proteins (IRS-1, -2,-3, and -4) (14, 15, 33, 34). These phosphorylated substratesthen bind proteins containing Src homology 2 (SH2) domains, includingthe p85 regulatory subunit of phosphatidylinositol 3-kinase (PI3-kinase) (2), growth factor receptor binding protein 2 (Grb-2),which links signaling via SOS to activation of the Ras complex(23), and protein tyrosine phosphatase SHP2 (12), that leadto activation of various downstream signaling pathways. However,IRS proteins display important differential sensitivities forbinding these SH2 proteins (27). Another substrate for activatedinsulin receptors is SHC, which exists in three isoforms: p66,p52, and p46 (20). Like IRS proteins, SHC proteins are tyrosinephosphorylated upon insulin receptor activation but can only associatewith Grb-2 (22, 23).

Recent studies performed in animal models by homologous recombinant gene targeting suggest that IRS proteins play importantand distinctive roles in insulin and insulin-like growth factorI (IGF-I) signaling. Whereas IRS-1 has been shown to be the mayorplayer in IGF-I-induced mitogenesis (5), IRS-2 is more tightlylinked to glucose homeostasis. In fact, in mice made deficientfor IRS-1, glucose metabolism and growth are reduced by 50 to60%, despite the fact that IRS-2 and other proteins can act asalternative substrates of the insulin receptor kinase (1, 19,24). In contrast, IRS-2-deficient mice have a phenotype of type2 diabetes due to insulin resistance and $beta$ -cell failure (35,36). These phenotypes suggest that IRS-2 may play a greaterrole in glucose homeostasis, while IRS-1 is more important forsomatic cell growth. More recently, deletion of IRS-3 did notshow a discernible phenotype from that of wild-type mice (16),whereas mice lacking IRS-4 exhibited mild defects in growth, reproduction,and glucose homeostasis (6). However, the relative role ofthe different IRS proteins in mediating insulin action in theindividual tissues is stillunclear.

Several reports from our laboratories have demonstrated that fetal brown adipocytes are an excellent cell model for studyinginsulin action since these cells bear a high number of high-affinityinsulin receptors as well as both IRS-1, IRS-2, and other insulinsignaling molecules (26, 30-32). More recently, in order to dissectthe insulin signaling pathways leading to the different insulinbiological effects, we have developed immortalized fetal brownadipocyte cell lines from IRS-1-deficient mice (IRS-1^/), heterozygous mice (IRS-1^+/), and wild-type mice (IRS-1^+/+). IRS-1 has been shown to be an essential molecule to maintainthe adipogenic phenotype, despite the fact that IRS-2 is overexpressedin IRS-1-deficient brown adipocytes (29). In the present study,we investigated the molecular mechanisms by which the lack ofIRS-1 results in the inability of brown adipocytes to activatethe Ras/mitogen-activated protein kinase (MAPK) pathway, DNA synthesis,and the entry of the cells in the S/G₂/M phases of the cell cycle.We have been able to partly restore MAPK activation and DNA synthesisin IRS-1-deficient cells by pretreatment with PI 3-kinase inhibitors,which presumably act through a feedback mechanism. In addition,we have found that adding back IRS-1, but not the mutant Y895F,which lacks Grb-2 binding, to the IRS-1-deficient brown adipocytescan restore signaling and mitogenicfunction.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Materials. Fetal calf serum (FCS) and culture media were obtained from Gibco Inc. (Gaithersburg, Md.). Insulin, wortmannin, and anti-mouseimmunoglobulin G (IgG)-agarose were from Sigma Chemical Co. (St.Louis, Mo.). Protein A-agarose was from Roche Molecular Biochemicals(Mannheim, Germany). LY294002 was from Calbiochem (Calbiochem-NovabiochemIntl, La Jolla, Calif.). The antibodies against the insulin receptor $beta$ -chain (sc-09) and Grb-2 (sc-255) were purchased from Santa Cruz(Santa Cruz Biotechnology, Palo Alto, Calif.). The polyclonalanti-IRS-1, monoclonal antiphosphotyrosine (clone 4G10), and polyclonalanti-SHC antibodies were purchased from Upstate Biotechnology(Lake Placid, N.Y.). For SHC immunoprecipitations, a polyclonalanti-SHC antibody was purchased from Transduction LaboratoriesInc. (Lexington, Ky.). The anti-phospho MAPK (Thr202/Tyr204),anti-phospho MEK1/2 (Ser217/221), anti-MEK1/2, and anti-MAPK antibodieswere purchased from New England Biolabs (Beverly, Mass.). [ $gamma$ -³²P]ATP (3,000 Ci/mmol) and [³H]thymidine (0.2 µCi/ml;1 µM) were from Amersham (Aylesbury, UnitedKingdom). All other reagents used were of the purest gradeavailable.

Cell culture. Brown adipocytes were obtained from interscapular brown adipose tissue of 17.5 to 18.5 fetuses from 2 to 3 pregnant mice ofnormal genotype or from a pool of tissue of fetuses obtained from2 to 3 pregnant IRS-1^+/ mice mated with IRS-1^/ males and were further submitted to collagenase dispersion aspreviously described (17). Then cells were infected with thepuromycin-resistance retroviral vector pBabe, which encodes simianvirus 40 large T antigen as described previously (29). Followinginfection, fetal brown adipocytes were maintained in culture mediumfor 72 h before selection with puromycin (1 µg/ml) for 1 week.Several IRS-1^+/+, IRS-1^+/, and IRS-1^/ cell lines were cloned and expanded, and the expression of IRS-1was assessed by Western blotting (29). Three wild-type and IRS-1^/ clones were cultured in Dulbecco modified Eagle medium (DMEM)supplemented with 10% FCS and puromycin (1 µg/ml).

Immunoprecipitations. Quiescent cells were treated without or with several doses of insulin as indicated and lysed at 4°C in 1 ml of a solutioncontaining 10 mM Tris-HCl, 5 mM EDTA, 50 mM NaCl, 30 mM sodiumpyrophosphate, 50 mM NaF, 100 µM Na₃VO₄, 1% Triton X-100, and1 mM phenylmethylsulfonyl fluoride, pH 7.6 (lysis buffer). Lysateswere clarified by centrifugation at 15,000 × g for 10 min. Afterprotein content determination, equal amounts of protein (500 to600 µg) were immunoprecipitated at 4°C with the correspondingantibodies. The immune complexes were collected on protein A-agaroseor anti-mouse IgG-agarose beads. Immunoprecipitates were washedwith lysis buffer and extracted for 5 min at 95°C in 2× sodiumdodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE)sample buffer (200 mM Tris-HCl, 6% SDS, 2 mM EDTA, 4% 2-mercaptoethanol,10% glycerol, pH 6.8) and analyzed by SDS-PAGE.

Western blotting. After SDS-PAGE, proteins were transferred to Immobilon membranes and were blocked using 5% nonfat dried milk or 3% bovineserum albumin (BSA) in 10 mM Tris-HCl, 150 mM NaCl, pH 7.5, andincubated overnight with several antibodies as indicated in 0.05%Tween 20, 10 mM Tris-HCl, 150 mM NaCl, pH 7.5. Immunoreactivebands were visualized using the ECL Western blotting protocol(Amersham).

Protein determination. Protein determination was performed by the Bradford dye method (4) using Bio-Rad reagent and BSA as thestandard.

DNA constructs and expression vectors. The green fluorescent protein-wild-type IRS-1 (GFP-IRS-1^wt) and green fluorescent protein-IRS-1 mutant F895 (GFP-IRS-1^F895) plasmids were created by subcloning wild-type IRS-1 cDNA andIRS-1 mutant Y895F cDNA constructs in frame into the HindIII sitewithin the pGFPC2 vector (CLONTECH, Palo Alto, Calif.). The pCMVhisIRS-1^wt and pCMVhis IRS-1^F895 cDNA constructs were prepared as described previously (18).

Transfections. IRS-1-deficient brown adipocytes (clone 4) were cultured for 24 h in the presence of 10% FCS, and when 60 to 70% confluencewas reached cells were transfected according to the calcium phosphate-mediatedprotocol with the plasmid constructs indicated for each case.For pCMVhis IRS-1^wt and pCMVhis IRS-1^F895 constructs, 10 µg of DNA was added to each dish. After 4 to 6h of incubation, cells were shocked with 3 ml of 15% glycerolfor 2 min, washed, and then fed with DMEM-10% FCS. Twenty-fourhours after transfection, histidinol (10 mM) was added to selectstable transfectants. Several histidinol-resistant cell lineswere obtained, and the expression of IRS-1^wt and the mutant IRS-1^F895 was assessed by Westernblotting.

GFP-IRS-1^wt and GFP-IRS-1^F895 constructs were used for transient transfection experiments. Fifteen micrograms of DNA was added toeach dish, and after 4 to 6 h of incubation cells were shockedwith 3 ml of 15% glycerol for 2 min, washed, and then fed withDMEM-10% FCS. After 48 h of culture under these conditions, cellswere detached from the monolayer, and green fluorescent cellswere purified by cell sorting in a FACStar PLUS (Becton-Dickinson,San Jose, Calif.) flow cytometer. Fluorescent cells were collectedin DMEM supplemented with 20% FCS and subsequently plated backand immediately used for further experiments. GFP-positive cellswere visualized using an MRC-1024 confocal microscope (Bio-Rad,Hempestead, UnitedKingdom).

[³H]Thymidine incorporation into DNA. Cells were plated at 0.5 × 10⁶/dish in 6-cm dishes in DMEM with 10% FCS. After 24 h, the medium was changed to DMEM with 0.05%insulin-free BSA, and cells were further cultured for 24 h inthe absence or presence of various doses of insulin. DNA synthesiswas determined by [³H]thymidine incorporation (0.2 µCi/ml) over the last 4 h of culture(17). After two washes with ice-cold phosphate-buffered saline(PBS), cells were lysed in 0.1% SDS. Trichloroacetate-precipitableDNA was then counted for incorporated radioactivity. All assayswere performed in triplicate and expressed in counts per minute/dish.

Analysis of cell cycle by flow cytometry. Cells were plated at 0.5 × 10⁶/dish in 6-cm dishes in DMEM with 10% FCS. After 24 h, the medium was changed to DMEM with 0.05%insulin-free BSA and cells were further cultured for another 24h in the absence or presence of various doses of insulin. Cellswere stained with the Kinesis test from Bio-Rad. The percentageof cells in G₀/G₁ and S plus G₂/M phases of the cell cycle weredetermined in a FACScan flow cytometer (Becton-Dickinson) usingModfit software (Verity Software) and a doublet discriminatorto analyze singlecells.

	RESULTS

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Brown adipocytes from IRS-1-deficient mice do not respond to insulin by increasing DNA synthesis. The immortalized brown adipocyte cell lines derived from the IRS-1^/ mice completely lacked IRS-1 protein expression (29), whereasthe IRS-1^+/+ cell lines expressed high levels of endogenous IRS-1 similarto those of primary brown fat cells (31). To analyze the effectof the IRS-1 null mutation on brown adipocyte insulin-inducedcell growth, quiescent (24-h serum-starved) IRS-1^/ and control (IRS-1^+/+) cells were cultured in a serum-free medium in the absence orpresence of various doses of insulin (1, 10, and 100 nM) for 24h. DNA synthesis was measured in both cell lines by [³H]thymidine incorporation during the last 4 h of culture. Althoughimmortalized fetal brown adipocytes showed an intrinsic mitogeniccompetence in the absence of insulin as described previously forprimary cells (17), IRS-1^+/+ cells showed markedly increased (threefold) DNA synthesis inthe presence of insulin, the maximal effect being elicited at100 nM (Fig. 1A). The basal rate of DNA synthesis in the IRS-1^/ brown adipocytes was similar to that in the wild type. However,these cells did not respond to insulin by increasing DNA synthesis.The lack of effect of insulin-induced mitogenesis in IRS-1-deficientbrown adipocytes was also assessed by measuring the percentageof cells in S plus G₂/M phases of the cell cycle, either in theabsence or in the presence of insulin. As shown in Fig. 1B, thepresence of insulin (10 to 100 nM) for 24 h significantly increasedthe percentage of IRS-1^+/+ cells in S plus G₂/M phases of the cell cycle compared to nontreatedcells. However, no insulin effect in the distribution of the cellsalong the phases of the cell cycle was observed in IRS-1^/ brown adipocytes.

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FIG. 1. Mitogenic response to insulin in wild-type and IRS-1-deficient brown adipocytes. (A) Three clones of wild-type (+/+) and IRS-1-deficient ( $-$ / $-$ ) immortalized brown adipocytes were cultured for 24 h in serum-free medium either in the absence or presence of insulin (1, 10, and 100 nM). DNA synthesis was determined by [³H]thymidine incorporation (0.2 µCi/ml) over the last 4 h of culture. After two washes with ice-cold PBS, cells were lysed and trichloroacetate-precipitable DNA was then counted for incorporated radioactivity. Results are expressed as disintegrations per minute (dpm) per dish and are means ± standard errors from six independent experiments, each one performed in triplicate. (B) Cells were cultured for 24 h either in the absence or presence of various doses of insulin as described for panel A. At the end of the culture time, the percentage of cells in S plus G₂/M phases of the cell cycle was determined as described in Materials and Methods. Results are means ± standard errors from six independent experiments.

IRS-1^/ brown adipocytes failed to activate MEK1/2 and p42-p44 MAPK in response to insulin. Activation of the Ras-MAPK signaling cascade has been shown to be an essential requirement for insulin-IGF-I-induced brownadipocyte mitogenic responses (21). To assess the impact ofthe lack of IRS-1 expression on this pathway, we determined insulin-inducedMEK1/2 and p42-p44 MAPK activation in IRS-1^+/+ and IRS-1^/ brown adipocytes. Quiescent (20-h serum-starved) IRS-1^+/+ and IRS-1^/ cell lines were stimulated with insulin (1 to 100 nM) for 5 min.Then cells were lysed and equals amount of protein were submittedto SDS-PAGE followed by Western blotting with anti-phospho MEK1/2and anti-phospho p42-p44 MAPK antibodies. Insulin induced bothMEK1/2 and MAPK phosphorylation in a dose-dependent manner inwild-type brown adipocytes (Fig. 2). In contrast, no insulin effectwas observed in IRS-1^/ brown adipocytes, although basal phosphorylation of both kinaseswas higher than that observed in wild-type cells. Furthermore,total MEK1/2 and MAPK content remained unchanged in all the celllines, indicating that IRS-1 mediates insulin-induced MAPK activationin brown adipocytes.

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FIG. 2. Insulin did not activate MAPK cascade in IRS-1-deficient brown adipocytes. Quiescent (20-h serum-starved) wild-type (+/+) and IRS-1-deficient ( $-$ / $-$ ) brown adipocytes were stimulated with insulin (1 to 100 nM) for 5 min. Control cells were cultured in the absence of the hormone. Cells were then lysed and equal amounts of protein (50 µg) were submitted to SDS-PAGE followed by Western blot analysis with the anti-phospho MEK1/2, anti-MEK1/2, anti-phospho MAPK, and anti-MAPK antibodies. The positions of phosphorylated MEK1/2 and p42-p44 MAPK are indicated by arrowheads. Results from a representative experiment are shown. The autoradiograms corresponding to five independent experiments, using two clones of each cell type, were quantitated by scanning densitometry. Results are expressed as arbitrary units of phosphorylated MEK1/2 and phosphorylated p42-p44 MAPK and are means ± standard errors.

Insulin-induced tyrosine phosphorylation of SHC and its association with Grb-2 is severely impaired in IRS-1-deficient brown adipocytes. SHC is another insulin receptor substrate implicated in the activation of the Ras-MAPK signaling pathway via association withthe adapter protein Grb-2 (22, 23). The fact that insulin-inducedMAPK activation is abolished in IRS-1-deficient brown adipocytesprompted us to investigate the role of SHC signaling in thesecells. When quiescent IRS-1^+/+ brown adipocytes were cultured in serum-free medium for 20 h,there was a significant tyrosine phosphorylation of p52 and p46SHC proteins in the basal state (Fig. 3). In these cells, insulin(1 to 100 nM) stimulation for 5 min resulted in a marked increasein SHC tyrosine phosphorylation as compared to the controls. IRS-1-deficientcells showed basal tyrosine phosphorylation of SHC higher thanthat observed in wild-type brown adipocytes, but these cells didnot further increase SHC phosphorylation in response to insulin.However, the total amount of SHC proteins remained unchanged inall cell lines. We also observed a lack of effect of insulin inIRS-1^/ cells when the anti-insulin receptor $beta$ -chain immunoprecipitateswere analyzed by Western blotting with anti-SHC antibody, theamount of insulin receptor $beta$ -chain being unchanged in all celllines. Immunoprecipitation with anti-SHC antibody followed byanti-Grb-2 Western blotting revealed a marked increase in SHC-Grb-2association upon insulin stimulation of wild-type brown adipocytes;maximal effect was elicited at a 10 nM insulin concentration.However, IRS-1-deficient brown adipocytes lacked SHC-Grb-2 associationin response to insulin. These data suggest that in IRS-1-deficientbrown adipocytes SHC cannot compensate for the loss of IRS-1-mediatedsignaling through Grb-2.

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FIG. 3. Insulin effect on SHC tyrosine phosphorylation and its association with an insulin receptor and Grb-2 in wild-type and IRS-1-deficient brown adipocytes. Quiescent (20-h serum-starved) wild-type (+/+) and IRS-1-deficient ( $-$ / $-$ ) brown adipocytes were stimulated with insulin (1 to 100 nM) for 5 min. Control cells were cultured in the absence of the hormone. At the end of the culture time, cells were lysed and 600 µg of total protein was immunoprecipitated (IP) with anti-SHC or anti-insulin receptor (IR) antibodies. The resulting immune complexes were analyzed by Western blotting (WB) with anti-Tyr(P), anti-SHC, anti-IR, and anti-Grb-2 antibodies as indicated in each panel. The positions of p66, p52, and p46 SHC proteins and IR $beta$ -chain and Grb-2 are indicated by arrows. The results shown are representative of three experiments, which used two clones of each cell type. The corresponding autoradiograms were quantitated by scanning densitometry. Results are expressed as arbitrary units of SHC tyrosine phosphorylation, IR-associated SHC, or SHC-associated Grb-2 and are means ± standard errors.

IRS-1 coimmunoprecipitates with SHC in wild-type brown adipocytes. The loss of insulin-induced SHC tyrosine phosphorylation and its subsequent association with Grb-2 in brown adipocytes lackingIRS-1 suggested the possibility of the formation of a signalingcomplex including SHC and IRS-1 in wild-type brown adipocytes.Western blot analysis of cell lysates from wild-type cells followinginsulin (1 to 100 nM) stimulation revealed the presence of IRS-1in anti-SHC immunoprecipitates (Fig. 4). Indeed, IRS-1-SHC coimmunoprecipitationwas not observed when the cell lysates were incubated with anti-mouseIgGs as a nonimmune control (Fig. 4, upper right panel). Interestingly,phosphorylated IRS-2 does not coimmunoprecipitate with SHC eitherin wild-type or IRS-1-deficient brown adipocytes (results notshown).

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FIG. 4. IRS-1 coimmunoprecipitates with SHC in wild-type brown adipocytes. Quiescent (20-h serum-starved) wild-type (+/+) and IRS-1-deficient ( $-$ / $-$ ) brown adipocytes were stimulated with insulin (1 to 100 nM) for 5 min. Control cells were cultured in the absence of the hormone. At the end of the culture time, cells were lysed and 600 µg of total protein was immunoprecipitated (IP) with the anti-SHC monoclonal antibody. The resulting immune complexes were analyzed by Western blotting (WB) with polyclonal anti-IRS-1 and anti-SHC antibodies. The positions of IRS-1 and p66, p52, and p46 SHC proteins are indicated by arrowheads. The results shown are representative of three experiments, which used two different clones of IRS-1^+/+ cells. The corresponding autoradiograms were quantitated by scanning densitometry. Results are expressed as arbitrary units of SHC-associated IRS-1 and are means ± standard errors (bottom right panel). As a nonimmune control, cell lysates from untreated and insulin-stimulated wild-type brown adipocytes were incubated with anti-SHC antibody or anti-mouse IgGs and were analyzed by Western blotting with the anti-IRS-1 antibody (upper right panel).

PI 3-kinase inhibitors enhanced IRS-2-Grb-2 association and partially restored insulin-induced mitogenesis in IRS-1-deficient cells. Previous studies in our laboratory have demonstrated that, despite the fact that brown adipocytes express IRS-2, its associationwith Grb-2 is virtually absent in primary brown adipocytes (31).In addition, insulin-induced IRS-1 and IRS-2 tyrosine phosphorylationcan be enhanced by pretreatment of these cells with PI 3-kinaseinhibitors as a result of a reduction of the serine/threoninephosphorylation state of both IRS-1 and IRS-2 (30). Since IRS-1^/ brown adipocytes overexpress IRS-2, we addressed the possibilityof restoring insulin-induced mitogenesis in these cells by enhancingIRS-2 tyrosine phosphorylation and subsequently its associationwith Grb-2. To test this, quiescent IRS-1^+/+ and IRS-1^/ cells were pretreated for 45 min with either 40 nM wortmanninor 5 µM LY294002 and were stimulated with 10 nM insulin for afurther 5 min. Cells were then lysed, and equal amounts of proteinwere immunoprecipitated with the anti-Grb-2 antibody and submittedto Western blot analysis with anti-IRS-2 antibody. As shown inFig. 5A, the presence of IRS-2 in anti-Grb-2 immunoprecipitatesupon insulin stimulation was very low in both wild-type and IRS-1^/ cell lines. However, pretreatment with PI 3-kinase inhibitorsincreased IRS-2-Grb-2 association twofold in wild-type brown adipocytesand threefold in IRS-1-deficient cells, the expression of Grb-2being unchanged in both cell lines.

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FIG. 5. PI 3-kinase inhibitors increased insulin-induced Grb-2-associated IRS-2 and the mitogenic response in IRS-1-deficient brown adipocytes. (A) Quiescent IRS-1^+/+ (+/+) and IRS-1^/ ( $-$ / $-$ ) brown adipocytes were pretreated for 45 min with either 40 nM wortmannin (W) or 5 µM LY294002 (Ly) and then stimulated with 10 nM insulin (ins; also designated i) for a further 5 min. Cells were lysed and immunoprecipitated (IP) with the anti-Grb-2 antibody and analyzed by Western blotting (WB) with anti-IRS-2 or anti-Grb-2 antibodies. Results from a representative experiment are shown. The autoradiograms corresponding to three independent experiments, which used two different clones of each cell type, were quantitated by scanning densitometry. Results are expressed as arbitrary units of Grb-2-associated IRS-2 and are means ± standard errors. (B) Cells were preincubated with 40 nM wortmannin (W) or 5 µM LY294002 (Ly) as described for panel A. Then cells were further stimulated for 5 min with various doses of insulin and were lysed. Equal amounts of protein (30 to 50 µg) were submitted to Western blot analysis with anti-phospho p42-p44 MAPK and anti-MAPK antibodies. Results from a representative experiment of three experiments are shown. (C) Quiescent wild-type and IRS-1^/ brown adipocytes were cultured for 24 h with 100 nM insulin in both the absence and presence of either 40 nM wortmannin or 5 µM LY294002. [³H]thymidine incorporation into acid-insoluble material was determined during the last 4 h of culture. Results are expressed as disintegrations per minute (dpm) per dish and are means ± standard errors from six independent experiments, which used three different clones of each cell type.

We further analyzed whether the enhanced IRS-2-Grb-2 association in IRS-1-deficient cells by PI 3-kinase inhibitors had apositive effect on insulin-induced MAPK activation and subsequentproliferation of these cells. Fig. 5B shows an anti-phospho p42-p44MAPK Western blot of wild-type and IRS-1^/ brown adipocytes which had been pretreated with 5 µM LY294002or 40 nM wortmannin for 45 min and stimulated with various dosesof insulin (1 to 100 nM) for a further 5 min. Whereas no insulineffect on MAPK activation was observed in IRS-1-deficient brownadipocytes, these cells recovered MAPK activation in responseto insulin after pretreatment with PI 3-kinase inhibitors, theactivation of p42-p44 MAPK being substantially recovered underthese experimental conditions (Fig. 5B). The effect of PI 3-kinaseinhibitors on insulin-induced DNA synthesis in wild-type and IRS-1-deficientbrown adipocytes is shown in Fig. 5C. Treatment of IRS-1^/ cells with 40 nM wortmannin or 5 µM LY294002 together with 100nM insulin for 24 h also resulted in a marked increase in [³H]thymidine incorporation as compared with control cells culturedin the absence of the hormone. As shown in Fig. 1 and 5C, in theabsence of pretreatment with wortmannin or the LY compound IRS-1^/ cells did not respond to insulin in increasing DNAsynthesis.

Reconstitution of IRS-1 expression in IRS-1-deficient cells. To investigate whether the loss of IRS-1 expression is responsible for the lack of insulin-stimulated cell growth, we reconstitutedIRS-1 expression in IRS-1-deficient brown adipocytes. These cellswere transfected with the pCMVhis vector containing the cDNA forIRS-1^wt, and stable transfected cell lines were selected in 10 mM histidinol-containingmedium. In parallel, we transfected a pCMVhis IRS-1^F895 mutant, in which the tyrosine in position 895 (which has beenshown to be responsible for Grb-2 association) was replaced byphenylalanine (18), and histidinol-resistant cell lines wereselected for further experiments. Figure 6A shows that IRS-1^wt and IRS-1^F895 expression in the reconstituted cell lines represents about 50to 60% and 40%, respectively, of that seen in wild-type cells.Next, we tested if exogenously expressed IRS-1^wt and IRS-1^F895 were functional by their tyrosine phosphorylation response toinsulin stimulation. Quiescent cells were serum-starved for 20h and then stimulated with 10 nM insulin for a further 5 min.Cell lysates were immunoprecipitated with the anti-IRS-1 antibodyand analyzed by Western blotting with the anti-Tyr(P) antibody.Both overexpressed IRS-1^wt and IRS-1^F895 underwent tyrosine phosphorylation in response to insulin. Inthese cells, the levels of tyrosine phosphorylation of both IRS-1^wt and IRS-1^F895 in response to insulin paralleled those seen in protein expression(Fig. 6B). In addition, anti-IRS-1 Western blotting of anti-Grb-2immunoprecipitates revealed that, whereas reconstituted IRS-1^wt associated with Grb-2 after insulin stimulation, no associationwith Grb-2 was found in the insulin-stimulated IRS-1^F895 cell line. By contrast, both IRS-1^wt and IRS-1^F895 could be detected in anti-SHC immunoprecipitates, indicatingthat the mutation Y895F in IRS-1 did not impair its coimmunoprecipitationwith SHC upon insulin stimulation (Fig. 7). However, IRS-1-SHCcoimmunoprecipitation was not observed when the cell lysates wereincubated with anti-mouse IgGs as a nonimmune control (upper rightpanel, Fig. 7). Furthermore, tyrosine phosphorylation of SHC andits association with Grb-2 in response to insulin stimulation,which were absent in IRS-1^/ cells, were recovered up to levels parallel to those seen inprotein expression after adding back either IRS-1^wt or IRS-1^F895.

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FIG. 6. Reconstitution of IRS-1 expression in IRS-1-deficient brown adipocytes. (A) IRS-1-deficient brown adipocytes (clone 4) were cultured in the presence of 10% FCS until 60 to 70% confluence was reached. Then cells were transfected with pCMVhis IRS-1^wt and pCMVhis IRS-1^F895 cDNA constructs according to the calcium phosphate-mediated protocol. Twenty-four hours after transfection, histidinol (10 mM) was added to select stable transfectants. Several histidinol-resistant cell lines were obtained, and the expression of IRS-1^wt and the mutant IRS-1^F895 was assessed by Western blot analysis with anti-IRS-1 antibody. (B) Quiescent cells were stimulated with 10 nM insulin for 5 min, and total cell lysates were immunoprecipitated (IP) with anti-IRS-1 or anti-Grb-2 antibodies. The resulting immune complexes were analyzed by Western blotting (WB) with anti-Tyr(P), anti-IRS-1, and anti-Grb-2 antibodies as indicated for each panel. The positions of IRS-1 and Grb-2 are indicated. A representative experiment is shown. The autoradiograms corresponding to three independent experiments, which used two clones of reconstituted cells, were quantitated by scanning densitometry. Results are expressed as arbitrary units of tyrosine phosphorylated IRS-1 and are means ± standard errors.

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FIG. 7. Reconstitution of IRS-1^wt or IRS-1^F895 restored IRS-1-SHC coimmunoprecipitation and SHC signaling. Quiescent cells (IRS-1^+/+, IRS-1^/, and pCMVhis IRS-1^wt and pCMVhis IRS-1^F895 transfectants) were stimulated with insulin (10 to 100 nM) for 5 min. Control cells were cultured in the absence of hormone. Total cell lysates were immunoprecipitated (IP) with anti-SHC antibody and were subsequently analyzed by Western blotting with anti-IRS-1, anti-Tyr(P), anti-Grb-2, and anti-SHC antibodies as indicated on each panel. The results shown are representative of 4 to 5 experiments, which used two clones of reconstituted cells. As a nonimmune control, cell lysates from untreated and insulin (100 nM)-stimulated wild-type, pCMVhis IRS-1^wt, and pCMVhis IRS-1^F895 brown adipocytes were incubated with anti-SHC antibody or anti-mouse IgGs and analyzed by Western blotting with the anti-IRS-1 antibody (right panel).

Reconstitution of IRS-1-Ras-MAPK signaling cascade and mitogenesis in IRS-1-deficient cells. Finally, we determined whether the IRS-1-Ras-MAPK signaling cascade and the mitogenesis induced by insulin in brown adipocyteswere recovered in these stable transfectants. As shown in Fig.8, insulin induced MAPK phosphorylation in a dose-dependent mannerin IRS-1^+/+ brown adipocytes and IRS-1^wt-reconstituted brown adipocytes. In contrast, no insulin effectwas observed in cells transfected with the mutant IRS-1^F895. These results suggest that in brown adipocytes the IRS-1-Grb2association mediates insulin-induced MAPK activation rather thanhaving some compensatory effect via the SHC signaling pathway.In parallel, the mitogenic effect of insulin as determined by[³H]thymidine incorporation was recovered when IRS-1^wt, but not IRS-1^F895, was expressed in IRS-1-deficient cells.

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FIG. 8. Reconstitution of IRS-1^wt, but not IRS-1^F895, restores MAPK activation and mitogenesis in brown adipocytes. (A) Quiescent cells (IRS-1^+/+ and pCMVhis IRS-1^wt and pCMVhis IRS-1^F895 stable transfectants) were stimulated with various doses of insulin for 5 min, and total protein was submitted to Western blot analysis with anti-phospho MAPK and anti-MAPK antibodies. Results from a representative experiment out of three, which used two clones of reconstituted cells, are shown. (B) Cells were cultured for 24 h in a serum-free medium either in the absence or presence of insulin (10 to 100 nM). DNA synthesis was determined by [³H]thymidine incorporation (0.2 µCi/ml) over the last 4 h of culture. Results are expressed as disintegrations per minute (dpm) per dish and are means ± standard errors from six independent experiments, each one performed in triplicate. +/+, IRS-1^+/+.

The role of IRS-1 in insulin-induced MAPK activation and mitogenesis was confirmed by transient transfection of IRS-1-deficientbrown adipocytes with IRS-1^wt and IRS-1^F895 subcloned in the pGFPC2 vector. After transfection, positivecells could be visualized by confocal microscopy due to theirgreen fluorescence (Fig. 9A) and could be separated by cell sortingto be used for further experiments. These transfectants showedsignificant tyrosine phosphorylation levels of both IRS-1^wt and IRS-1^F895 upon insulin stimulation, as shown in the anti-Tyr(P) Westernblot analysis of anti-IRS-1 immunoprecipitates (Fig. 9B). In addition,MAPK phosphorylation in response to insulin was recovered whenIRS-1^wt, but not IRS-1^F895, was transiently added back to IRS-1-deficient cells (Fig. 9C).Likewise, the mitogenic effect of insulin was recovered in IRS-1^wt-transfected cells but not in IRS-1^F895 transfectants (Fig. 9D).

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FIG. 9. Reconstitution of insulin-induced mitogenesis by transient transfection with GFP-IRS-1^wt, but not with GFP-IRS-1^F895, construct. (A) IRS-1-deficient brown adipocytes were transfected with the GFP-IRS-1^wt and GFP-IRS-1^F895 cDNA constructs as described in Materials and Methods. A representative image of fluorescent cells is shown. (B) Quiescent cells were stimulated with 10 nM insulin for 5 min, and total cell lysates were immunoprecipitated (IP) with anti-IRS-1 antibody. The resulting immune complexes were analyzed by Western blotting (WB) with the anti-Tyr(P) antibody. The position of IRS-1 is indicated. A representative experiment is shown. (C) Quiescent cells (IRS-1^+/+ and pGFPIRS-1^wt and pGFPIRS-1^F895 transfectants) were stimulated with insulin (10 and 100 nM) for 5 min, and total cell lysates were submitted to Western blot analysis with the anti-phospho MAPK and anti-MAPK antibodies. A representative autoradiogram is shown. (D) Cells were cultured for 24 h in a serum-free medium either in the absence or presence of insulin (10 to 100 nM). DNA synthesis was determined by [³H]thymidine incorporation (0.2 µCi/ml) over the last 4 h of culture. After two washes with ice-cold PBS, cells were lysed and trichloroacetate-precipitable DNA was then counted for incorporated radioactivity. Results are expressed as disintegrations per minute (dpm) per dish and are means ± standard errors from six independent experiments, each one performed in triplicate. +/+, IRS-1^+/+.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

A complete understanding of insulin action requires the identification of the intracellular pathways that regulate insulin-stimulatedgrowth, development, and metabolism. In this regard, during thelast years several laboratories have provided considerable characterizationof the role of docking proteins, such as IRS proteins and SHC,that interact with the insulin receptor and mediate intracellularsignals in the insulin action cascade. Moreover, a variety ofrecent studies have demonstrated that animal models lacking IRS-1or IRS-2 produced by targeted gene mutation can be very usefulto study the specific role of each docking protein in the complexinsulin signaling network. Accordingly, our laboratory addressedthis issue by generating immortalized fetal brown adipocyte celllines from IRS-1 knockout mice. Although these cells maintainedthe phenotypic features of brown adipocytes under growing conditions(10% FCS) and also overexpressed IRS-2, they lack the insulineffect on increasing cytosolic lipid content (29) and fail toundergo normal adipocyte differentiation (M. Fasshauer and C.R. Kahn, personal communication). In addition, insulin-stimulatedIRS-1-deficient cells failed to activate protein kinase B (Aktor PKB), indicating that the IRS-1-PI 3-kinase-Akt signaling pathwayis a requirement for insulin-induced lipid synthesis in brownadipocytes (29).

The facts that IRS-1-deficient mice display intrauterine growth retardation (1, 24) and that IGF-I-insulin is a completemitogen in primary cultures of rat brown adipocytes (17, 21)prompted us to investigate whether IRS-1 is the major dockingprotein leading the mitogenic signaling cascade in fetal brownadipocytes. Accordingly, in this study we found that whereas brownadipocytes from wild-type mice respond to physiological dosesof insulin by increasing DNA synthesis, the growth response ofIRS-1-deficient cells to this hormone is severely impaired asa result of a failure to enter S/G₂/M phases of the cell cycle,indicating that the lack of IRS-1 impairs the mitogenic effectof insulin in brownadipocytes.

Activation of p42-p44 MAPK by the upstream kinase MEK1/2 has been shown to be an essential requirement in the molecular mechanismsby which insulin induces the proliferation of brown adipocytes(21). However, the role of IRS-1 in MAPK activation may differfrom tissue to tissue. Thus, muscles from IRS-1-deficient miceshowed an impairment in insulin-induced MAPK activation, whilein the liver this response was unaltered (37). Furthermore,3T3 fibroblasts lacking IRS-1 lost their mitogenic response toIGF-I. However, those cells increased MAPK activity in responseto IGF-I but not to PI 3-kinase activity, suggesting that signalingthrough PI 3-kinase rather than through MAPK is required for proliferationin fibroblasts (5). The results presented here indicate thatin brown adipocytes, insulin stimulates MAPK in an IRS-1-dependentmanner and that the overexpression of IRS-2 fails to rescue insulin-stimulatedentry into S, G₂, and M phases of the cell cycle. Importantly,in our model of IRS-1-deficient cells, insulin-induced SHC tyrosinephosphorylation is also impaired, while SHC expression remainsunchanged. Indeed, a direct interaction between phosphorylatedIRS-1 and SHC using the yeast two-hybrid system has been describedpreviously (10). In intact cells, however, we cannot excludethe possibility that another protein, such as the insulin receptorand/or a different insulin receptor substrate, could mediate theinteraction between IRS-1 and SHC. In addition, reconstituted32D-insulin receptor cells show insulin-induced SHC phosphorylationand MAPK activation (7). However, those cells constitutivelylack the expression of essential players in the insulin action,such as IRS-1 and IRS-2, missing the complexity of the insulinsignaling machinery observed in physiological insulin target cells,such as brown adipocytes. Taken together, our results indicatethat phosphorylation of IRS-1 upon insulin stimulation is a crucialevent for MAPK activation and proliferation in brownadipocytes.

One mechanism by which IRS tyrosine phosphorylation is regulated involves serine/threonine phosphorylation. Previous studieshave reported that serine/threonine phosphorylation of IRS-1 inducedby okadaic acid or tumor necrosis factor alpha results in decreasedtyrosine phosphorylation of IRS-1 and insulin resistance (8,25). Likewise, PI 3-kinase appears to be a key regulator ofIRS-1 and IRS-2 phosphorylation and signaling by promoting serine/threoninephosphorylation in a negative feedback loop (11, 13), thiseffect being abolished by inhibitors of this enzyme. Furthermore,although IRS-2 is highly expressed in primary brown adipocytesand brown adipocyte cell lines (29, 31), its binding withGrb-2 is virtually undetectable, as has also been reported for32D reconstituted cells (27). Thus, we attempted to restorethe mitogenic response in IRS-1-deficient cells by enhancing IRS-2tyrosine phosphorylation and its signaling through the Ras-MAPKpathway. Pretreatment of IRS-1-deficient brown adipocytes witheither wortmannin or LY294002 before insulin stimulation significantlyenhanced IRS-2-Grb-2 association and partly restored the activationof p42-p44 MAPK in response to insulin. As it has been previouslydemonstrated that MAPK activation is required for insulin-inducedbrown adipocyte proliferation (21), the recovery of phosphorylatedMAPK upon insulin stimulation in the presence of two unrelatedPI 3-kinase inhibitors also increased DNA synthesis in IRS-1-deficientcells. Consequently, despite the fact that IRS-2 is endogenouslyoverexpressed in IRS-1-deficient cells, this protein does notcompensate for the lack of IRS-1 in inducing mitogenesis, unlessits tyrosine phosphorylation is enhanced through a feedback mechanismvia inhibition of PI 3-kinase.

Finally, if the loss of IRS-1 expression is responsible for the observed reduction in insulin-stimulated growth, then reconstitutionof IRS-1 expression would be predicted to correct most, if notall, of these signaling effects. For this goal, we transfectedIRS-1^/ cells with the pCMVhis IRS-1^wt construct and generated stable cell lines. This method allowedus to recover 40 to 60% of the IRS-1 expression seen in wild-typecells. In parallel, we generated stable transfectants expressingpCMVhis IRS-1^F895, a mutant lacking Grb-2 binding (18). The fact that both transfectantsexhibited tyrosine phosphorylation of IRS-1 but only IRS-1^wt associated Grb-2 in response to insulin allowed us to comparethe IRS-1-Ras-MAPK signaling cascades in both IRS-1 reconstitutedbrown adipocyte celllines.

The reintroduction of both IRS-1^wt and IRS-1^F895 restored both SHC tyrosine phosphorylation and IRS-1-SHC association upon insulinstimulation, virtually lost in IRS-1-deficient brown adipocytes.Interestingly, a downstream event, such as SHC-Grb-2 association,was also recovered accordingly in both transfectants with theamount of IRS-1 protein content found in reconstituted cells.More importantly, insulin induced MAPK phosphorylation and DNAsynthesis in IRS-1^wt-reconstituted cells. However, none of these events could be recoveredwhen the mutant IRS-1^F895 was added back to the cells, indicating that the contributionof SHC signaling to the Grb-2-Ras-MAPK pathway in these cellsis not sufficient to induce mitogenesis in the absence of IRS-1-Grb-2signaling. These results were confirmed in cells transiently expressingthese proteins and selected by fluorescence-activating cell sorting.A possible explanation to account for these data may arise fromthe possible location of SHC and IRS-1 in different cell compartmentsrecruiting distinct Grb-2-SOS pools, the IRS-1-Grb-2-SOS one beingindispensable to achieve Ras-MAPK activation andmitogenesis.

In conclusion, our data demonstrate that the lack of IRS-1 causes an impairment of insulin to stimulate MAPK and mitogenesisin brown adipocytes. This impairment is partly overcome by inhibitionof PI 3-kinase and is concurrent with an enhancement of IRS-2-Grb-2association. The reconstitution of IRS-1-deficient brown adipocytesby wild-type IRS-1 but not by the Y895F IRS-1 mutant completelyrestores MAPK activation and mitogenesis in response to insulin,indicating that IRS-1-Grb-2 association but not SHC-Grb-2 associationis an essential requirement in mediating insulin signaling leadingto MAPK activation and mitogenesis in brownadipocytes.

	ACKNOWLEDGMENTS

This work was supported by grant PM97-0050 from the Ministerio de Educación y Cultura,Spain.

We also recognize the valuable technical skill of M. López.

	FOOTNOTES

^* Corresponding author. Mailing address: Departamento de Bioquímica y Biología Molecular, Centro Mixto CSIC/UCM, Facultadde Farmacia, Ciudad Universitaria, 28040 Madrid, Spain. Phone:34-91-3941777. Fax: 34-91-3941779. E-mail: benito{at}eucmax.sim.ucm.es.

Present address: Instituto de Neurobiología Cajal, Consejo Superior de Investigaciones Científicas, 28002 Madrid,Spain.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Araki, E., M. A. Lipes, M. E. Patti, J. C. Brüning, B. L. Haag III, R. S. Johnson, and C. R. Kahn. 1994. Alternative pathway of insulin signalling in mice made with targeted disruption of the IRS-1 gene. Nature 372:186-190[CrossRef][Medline].
2.	Backer, J. M., M. G. Myers, Jr., S. E. Schoelson, D. J. Chin, X. J. Sun, M. Miralpeix, P. Hu, B. Margolis, E. Y. Skolnik, J. Schlessinger, and M. F. White. 1992. The phosphatidylinositol 3-kinase is activated by association with IRS-1 during insulin stimulation. EMBO J. 11:3469-3479[Medline].
3.	Baserga, R. 1991. Growth regulation of the PCNA gene. J. Cell. Sci. 98:433-436[Free Full Text].
4.	Bradford, M. 1976. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal. Biochem. 72:248-254[CrossRef][Medline].
5.	Brüning, J. C., J. Winnay, B. Cheatham, and C. R. Kahn. 1997. Differential signaling by insulin receptor substrate 1 (IRS-1) and IRS-2 in IRS-1-deficient cells. Mol. Cell. Biol. 17:1513-1521[Abstract].
6.	Fantin, V. R., Q. Wang, G. E. Lienhard, and S. R. Keller. 2000. Mice lacking insulin receptor substrate 4 exhibit mild defects in growth, reproduction, and glucose homeostasis. Am. J. Physiol. Endocrinol. Metab. 278:E127-E133[Abstract/Free Full Text].
7.	Harada, S., R. M. Smith, M. F. White, and L. Jarret. 1996. Insulin-induced egr-1 and c-fos expression requires insulin receptor, Shc, and mitogen-activated protein kinase, but not insulin receptor substrate-1 and phosphatidylinositol 3-kinase activation. J. Biol. Chem. 271:30222-30226[Abstract/Free Full Text].
8.	Hotamisligil, G. S., P. Peraldi, A. Budavari, R. Ellis, M. F. White, and B. M. Spiegelman. 1996. IRS-1-mediated inhibition of insulin receptor tyrosine kinase activity in TNF- $alpha$ and obesity-induced insulin resistance. Science 271:665-668[Abstract].
9.	Kasuga, M., F. A. Karlsson, and C. R. Kahn. 1982. Insulin stimulates the phosphorylation of the 95,000-dalton subunit of its own receptor. Science 215:185-187[Abstract/Free Full Text].
10.	Kasus-Jacobi, A., D. Perdereau, S. Tartare-Deckert, E. Van Obberghen, J. Girard, and A. F. Burnol. 1997. Evidence for a direct interaction between insulin receptor substrate-1 and Shc. J. Biol. Chem. 272:17166-17170[Abstract/Free Full Text].
11.	Kim, B., P. S. Leventhal, M. F. White, and E. L. Feldman. 1998. Differential regulation of insulin receptor substrate-2 and mitogen-activated protein kinase tyrosine phosphorylation by phosphatidylinositol 3-kinase inhibitors in SH-SY5Y human neuroblastoma cells. Endocrinology 139:4881-4889[Abstract/Free Full Text].
12.	Kuhne, M. R., T. Pawson, G. E. Lienhard, and G.-S. Feng. 1993. The insulin receptor substrate 1 associates with the SH2-containing phosphotyrosine phosphatase Syp. J. Biol. Chem. 268:11479-11481[Abstract/Free Full Text].
13.	Lam, K., C. L. Carpenter, N. B. Ruderman, J. C. Friel, and K. L. Kelly. 1994. The phosphatidylinositol 3-kinase serine phosphorylates IRS-1: stimulation by insulin and inhibition by wortmannin. J. Biol. Chem. 269:20648-20652[Abstract/Free Full Text].
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