The T-Cell Receptor Regulates Akt (Protein Kinase B) via a Pathway Involving Rac1 and Phosphatidylinositide 3-Kinase

doi:10.1128/MCB.20.15.5469-5478.2000

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Molecular and Cellular Biology, August 2000, p. 5469-5478, Vol. 20, No. 15
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

The T-Cell Receptor Regulates Akt (Protein Kinase B) via a Pathway Involving Rac1 and Phosphatidylinositide 3-Kinase

Elisabeth M. Genot,¹^,²^,^* Cecile Arrieumerlou,³ Gregory Ku,⁴ Boudewijn M. T. Burgering,⁵ Arthur Weiss,⁴ and Ijsbrand M. Kramer²

Department of Immunology, Imperial College, London W12 0NN, United Kingdom¹; Growth Factors and Differentiation Laboratory, University of Bordeaux I, 33 405 Talence Cedex,² and Laboratoire d'Immunologie Cellulaire, CERVI, UMR 7627 CNRS, 75013 Paris,³ France; Department of Medicine, Microbiology and Immunology, Howard Hughes Medical Institute, University of California at San Francisco, San Francisco, California 94143-0795⁴; and Laboratory for Physiological Chemistry, Utrecht University, 3584 CG Utrecht, The Netherlands⁵

Received 3 February 2000/Returned for modification 7 March 2000/Accepted 8 May 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The serine/threonine kinase Akt (also known as protein kinase B) (Akt/PKB) is activated upon T-cell antigen receptor (TCR)engagement or upon expression of an active form of phosphatidylinositide(PI) 3-kinase in T lymphocytes. Here we report that the smallGTPase Rac1 is implicated in this pathway, connecting the receptorwith the lipid kinase. We show that in Jurkat cells, activatedforms of Rac1 or Cdc42, but not Rho, stimulate an increase inAkt/PKB activity. TCR-induced Akt/PKB activation is inhibitedeither by PI 3-kinase inhibitors (LY294002 and wortmannin) orby overexpression of a dominant negative mutant of Rac1 but notCdc42. Accordingly, triggering of the TCR rapidly stimulates atransient increase in GTP-Rac content in these cells. Similarto TCR stimulation, L61Rac-induced Akt/PKB kinase activity isalso LY294002 and wortmannin sensitive. However, induction ofAkt/PKB activity by constitutive active PI 3-kinase is unaffectedwhen dominant negative Rac1 is coexpressed, placing Rac1 upstreamof PI 3-kinase in the signaling pathway. When analyzing the signalinghierarchy in the pathway leading to cytoskeleton rearrangements,we found that Rac1 acts downstream of PI 3-kinase, a finding thatis in accordance with numerous studies in fibroblasts. Our resultsreveal a previously unrecognized role of the GTPase Rac1, actingupstream of PI 3-kinase in linking the TCR to Akt/PKB. This isthe first report of a membrane receptor employing Rac1 as a downstreamtransducer for Akt/PKBactivation.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Engagement of the T-cell antigen receptor (TCR) by antigen in a major histocompatibility complex context or by antibodiesthat cross-link this receptor triggers a complex series of signalingevents that lead to reorganization of the cytoskeleton as wellas transcriptional activation of multiple genes and culminatein T-lymphocyte activation and proliferation (9). One of theearliest events triggered by TCR engagement is the activationof protein tyrosine kinases (PTKs). Activation of the Src tyrosinekinase Lck is necessary to phosphorylate the cytoplasmic tailsof the CD3 complex on tyrosine residues within the immunoreceptortyrosine-based activation motifs (ITAMs). Phosphorylation of theITAMs provides docking sites for the Src homology domains (SH2)of the Syk family PTKs which, once recruited, become activatedand cause subsequent tyrosine phosphorylation of multiple substrates.One such substrate is the integral membrane protein LAT (linkerfor activation of T cells), whose phosphorylation allows recruitmentof a whole range of signaling molecules, including Grb2, PLC- $gamma$ ,GADs, SLP-76, Cbl, Vav, and the regulatory subunit p85 of phosphatidylinositide(PI) 3-kinase, through either direct or indirect interactions(46). With respect to PI 3-kinase, the TCR is endowed with atleast two other putative modes of activation: via a direct mechanism,by binding of the p85 regulatory subunit of PI 3-kinase to thetyrosine phosphorylated ITAM (11, 25), or in an indirect way,through activation of Ras (12), which in turn could interactwith and activate the p110 catalytic subunit of PI 3-kinase (31,32). PI 3-kinase catalyzes the phosphorylation of phosphoinositidesat the D3 hydroxyl of the myoinositol ring, generating polyphosphoinositidesPtdIns(3)P, PtdIns(3,4)P2, and PtdIns(3,4,5)P3, which act as secondmessengers to recruit and activate downstreameffectors.

One well-characterized PI 3-kinase effector is Rac1 (27), a GTPase which controls cytoskeletal organization and cell morphology(24). In various cell types, activation of Rac1 in responseto growth factors elicits actin polymerization at the plasma membraneto produce lamellipodia and membrane ruffles (30). In T cells,membrane ruffling is induced in response to the T-cell growthfactor interleukin 2 (IL-2) via a pathway also involving PI 3-kinaseand Rac1 (3). Another major target of PI 3-kinase signalingis the serine/threonine kinase Akt (also known as protein kinaseB) (Akt/PKB). This kinase regulates critical functions, such asinsulin signaling, cell survival, and cell cycle progression (reviewedin reference 10). Akt/PKB is activated by a number of receptorsthat activate PI 3-kinase in various cell types and by variousligands, such as growth factors including insulin, epidermal growthfactor (EGF), platelet-derived growth factor (PDGF), basic fibroblastgrowth factor (bFGF), or cytokines, such as IL-2, IL-3, IL-4,granulocyte-macrophage colony-stimulating factor, or the B-cellantigen receptor (17). In these systems, it has been shown thatactivation of PI 3-kinase is necessary for the induction of activationof Akt/PKB. In mature T cells, Akt/PKB has also been shown toprotect against cell death and to control cell cycle progression,two events essential for proper clonal expansion (1, 7).In these cells, stimulation of Akt/PKB by the TCR is also strictlydependent on the activity of PI 3-kinase since it is blocked bythe PI 3-kinase inhibitors wortmannin and LY294002 (15). Moreover,ectopic expression of constitutively active forms of PI 3-kinasestimulates Akt/PKB (15, 26).

Considerable progress has been made toward understanding how PI 3-kinase activates Akt/PKB (5). The generation of the polyphosphoinositidesby PI 3-kinase serves to localize Akt/PKB at the plasma membrane,through binding of its PH domain. This event is thought to exposeAkt/PKB to phosphoinositide-dependent kinases (PDKs). Akt/PKBis then phosphorylated on threonine 308 in the activation loopof the kinase domain by PDK1 and on serine 473 at the carboxyterminus by an as-yet-unidentified kinase often referred to asPDK2. In COS-1 cells, it was shown that phosphorylation of eitherthreonine 308 or serine 473 leads to partial activation of theenzyme in vitro and that phosphorylation of both residues resultsin a synergistic activation of Akt/PKB catalytic function (2).Activated Akt/PKB next detaches from the membrane and phosphorylatessubstrates in the cytosol andnucleus.

In order to delineate the roles of small GTPases in effector pathways downstream of the TCR (16, 44), we screened fora possible involvement of members of the Ras and Rho family ofGTPases in the activation of Akt/PKB. Our previous studies haverevealed that in Jurkat T cells, TCR-induced Akt/PKB activationis indeed mediated by PI 3-kinase but occurs independently ofRas (15). We now report that Rac1 is a key player in the activationof Akt/PKB. Akt/PKB activity is induced by a constitutively activemutant of Rac1 in a PI 3-kinase-dependent manner, positioningthis GTPase between the receptor and the lipid kinase. Furthermore,we provide evidence that, within the same cell, PI 3-kinase andRac1 are placed in opposite positions in the pathways resultingin Akt/PKB activation versus cytoskeletalrearrangement.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Cells and reagents. JHM1, a subline of the human T-acute lymphocytic lymphoma cell line Jurkat (15), was maintained in RPMI medium supplementedwith 5% heat-inactivated fetal calf serum and 2 mg of geneticin(Gibco BRL) per ml at 37°C under 5% CO₂. Cells were transferredto geneticin-free medium 48 h prior to the experiments. Reagentswere from Sigma. Antibodies UCHT1 (reactive with human CD3), 12CA5(antihemagglutinin [anti-HA] tag), and 9E10 (anti-myc tag) wereaffinity purified from hybridoma supernatants at the ImperialCancer Research Fund (ICRF) by standard protocols. Antibodiesagainst Akt/PKB were from U.B.I. or New England Biolabs, and anti-Rac1and anti-Cdc42 antibodies were obtained from Santa Cruz Biotechnology.Peroxidase-labeled antibodies used in the Western blotting protocolwere from Amersham International (Amersham, Buckinghamshire, UnitedKingdom), and LY294002 and wortmannin were from Calbiochem. Histone2B (H2B) was from BoehringerMannheim.

Plasmids and reporter constructs. Plasmids directing expression of wild-type or mutated N-terminal-HA-tagged Akt/PKB were used in kinase assays. pSG5 HA-wtAkt/PKB,pcDNA3 EE-T308A Akt/PKB, pSG5 HA-S473A-Akt/PKB, and pSG5 HA- $Delta$ PH-Akt/PKBhave been described previously (8, 34, 38). Constitutivelyactive, myc-tagged L61Rac and its mutants and L61Cdc42 were subclonedfrom PRK5 into pEFBOS vector (22). The chimera construct ofPI 3-kinase, pEFrCD2p110, and the pSG5p110K227E mutant have alsobeen described previously (27, 33). All plasmids were purifiedby equilibrium centrifugation in CsCl-ethidium bromide gradientsby using standardprocedures.

Cells and transfections. Cells were transfected via electroporation (Gene pulser; Bio-Rad, Hemel Hempstead, United Kingdom) as previously described(16). Briefly, cells were pulsed (at 1.5 × 10⁷ cells/0.5 ml) in complete medium at 960 µF and 310 V. Cells transfectedwith similar plasmid mixtures were pooled and realiquoted beforetreatment with stimulating antibodies. The amounts of DNA transfectedin each experiment were kept constant by adding emptyvector.

Rac1 activation assay. The assay was performed essentially as described previously (21). The GST-PAK70-106 (GST-CRIB) was a generous gift fromE. Manser (23). For each point, 4.5 million cells were treatedwith phosphate-buffered saline (PBS), in the absence or presenceof 10 µg of UCHT1 antibody per ml or 0.5 mM carbachol for thetime periods indicated. Cells were lysed by incubation for 15min at 4°C in a buffer containing 25 mM HEPES (pH 7.3), 0.15 MNaCl, 5 mM MgCl₂, 0.5 mM EGTA (pH 8), 20 mM beta-glycerophosphate(pH 7.5), 0.5% Triton X-100, 4% glycerol, 10 mM NaF, 2 mM sodiumorthovanadate, 5 mM dithiothreitol, 0.5 mM phenylmethylsulfonylfluoride, 5 µg of leupeptin per ml, and 5 µg of pepstatin perml. The lysate was centrifuged at 14,000 × g for 10 min at 4°C.The supernatant was next incubated with 40 µg of bacterially expressedglutathione S-transferase (GST)-CRIB prebound to 20 µl of gluthathioneagarose and was tumbled for 15 min at 4°C. The beads were collectedin a spin column and washed with 500 µl of lysis buffer. Fortymicroliters of 1× reducing sample buffer was added, followed byan incubation at 100°C for 5 min. Eluted proteins were resolvedby sodium dodecyl sulfate-15% polyacrylamide gel electrophoresis(SDS-15% PAGE) and Western blotting with an anti-Rac1 antiserum(TransductionLabs).

Kinase assays and Western blot analysis. For Akt/PKB kinase assays, cells were transfected with an HA-tagged version of wtAkt/PKB together with various expressionplasmids. At 18 to 24 h after transfection, cells were harvestedand equivalent numbers of living cells were subjected to immunoprecipitationusing 12CA5 antibodies as previously described (15). The kinasereaction was performed using H2B as a substrate in the presenceof [ $gamma$ -³²P]ATP. After incubation at room temperature for 30 min, the reactionwas stopped with Laemmli sample buffer and kinase reaction productswere analyzed by SDS-15% PAGE. The lower half of the gel was drieddown, and ³²P incorporation into H2B was quantitated using a PhosphorImager(Molecular Dynamics). The upper part of the gel containing immunoprecipitatedtagged protein kinase was transferred onto polyvinyldifluoridinemembrane membranes (Immobilon; Millipore). Membranes were blockedin PBS-0.05% Tween 20 (PBST) plus 5% milk (5% bovine serum albuminfor phosphospecific antibodies) for 2 h. Appropriate dilutionsof the relevant antibodies were incubated with the membrane overnightat 4°C. After extensive washes, membranes were incubated withthe second antibody in PBST for 1 h at room temperature. Membrane-boundantibodies were visualized by autoradiography using ECL Westernblotting detection reagents (Amersham) and Kodak XS1 films. Theamount of Akt/PKB detected by Western blotting was determinedby scanning the autoradiography followed by processing of thedata with the Adobe Photoshop program. H2B phosphorylation wasnormalized for the amount of HA-Akt/PKB in each sample and thusexpressed as fold increase of the control activity. To assessprotein expression from the transfected plasmid, proteins wereacetone precipitated from supernatants of immunoprecipitates for1 h at $-$ 20°C, pelleted, and resuspended in reducing Laemmli samplebuffer. After separation by SDS-PAGE, proteins were transferredto polyvinylidene difluoridine membranes (Immobilon; Millipore)followed by Western blotting as describedabove.

Analysis of morphological changes. Cells were cotransfected with 5 µg of pEF.BOS.GFP and either 45 µg of the empty vector or N17Rac, V12Rac, L61Rac, L61RacF37A,L61RacY40C, or rCD2p110 construct. After 48 h, living cells werepurified on Ficoll-Hypaque gradients and analyzed for morphologicalchanges as previously described (3). Experiments were performedwith cells kept in suspension at 37°C in a saline solution (140mM NaCl, 5 mM KCl, 10 mM HEPES [pH 7.4], 1 mM MgCl₂) containing1 million cells/ml. Fetal calf serum was added at 0.3% to reduceadhesion of cells to the glass coverslips. When the effect ofwortmannin (100 nM) or LY294002 (10 µM) was being tested, thecompound was added 20 min prior to morphologicalanalysis.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Activated Rac1 is a strong activator of Akt/PKB in T cells. Because engagement of the TCR stimulates Akt/PKB activity in a PI 3-kinase-dependent (LY294002-sensitive) yet Ras-independentmanner (15), we investigated if other monomeric GTPases, inparticular members of the Rho family, could stimulate this proteinkinase. For this purpose, constitutively active forms of Rho,Rac, or Cdc42 GTPases were transiently expressed in cells fromthe Jurkat J.HM1 T-cell line and Akt/PKB activity was measuredin an in vitro kinase assay using H2B as a substrate. Constitutivelyactivated Rac1 or Cdc42 (mutation at position 12 or 61) raisedbasal levels of Akt/PKB activity 4.5- and 4-fold, respectively,whereas constitutively active RhoA showed no induction (Fig. 1A).This effect was specific for the GTP-bound form, since wild-typeRac1, which in its resting state binds GDP in vivo, was unableto activate Akt/PKB. To further characterize the Rac1 effectorpathway that regulates Akt/PKB activity, we tested the effector-loopmutants L61RacF37A and L61RacY40C. These mutants still displayconstitutive activity but have selectively lost interaction withsome downstream effectors (22, 40). The L61RacY40C mutantretains the ability to efficiently induce Akt/PKB activity, whereasthe L61RacF37A mutant was less effective (Fig. 1B). Expressionof the Rac mutants was verified by Western blotting (data notshown). To attest that these Rac1 mutants discriminate betweenRac1 effector pathways in T cells, we measured their ability toinduce Jun-N-terminal kinase 2 activity in Jurkat T cells andobtained data consistent with those found in other cell types(data not shown and references 22 and 40). To compare Akt/PKBinduction by activated forms of Rac1 (L61Rac) with PI 3-kinase-mediatedstimulation, we expressed a chimeric construct of PI 3-kinase,rCD2p110, in which p110 has been fused to the extracellular domainof the CD2 cell surface marker (rat CD2) (27). The chimera warrantsrecruitment of the catalytic subunit to the plasma membrane andsomehow mimics the role of p85. Similar levels of Akt/PKB activitywere obtained when using either L61Rac or rCD2p110 (Fig. 1C).These results establish that GTP-bound Rac1 and Cdc42 are strongactivators of Akt/PKB in T cells. Rac1 employs a downstream effectorthat retains the ability to bind the L61RacY40C mutant.

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FIG. 1. Activated Rac1 stimulates Akt/PKB in T cells. (A) Jurkat cells (15 million per condition) were transfected with plasmids encoding HA-Akt/PKB (10 µg), together with the empty vector (20 µg), the plasmid encoding wild-type Rac1 (wtRac1, 20 µg), or constitutively active forms of either Rac1 or one of the other small GTPases (each 20 µg). Eighteen hours later, cells were harvested and equal numbers of living cells were lysed and subjected to an immunokinase assay as described in Materials and Methods. Results from one representative experiment are shown in the top panel, whereas the histogram presents the mean ± standard deviation of at least three experiments. (B) Conditions were the same as those for panel A except that Rac1 and Rac1-effector-loop mutants were compared for their induction of Akt/PKB kinase activity (mean ± standard deviation of three experiments). (C) Conditions were the same as those for panel A except that 20 µg of the empty vector or the plasmid encoding constitutively activated forms of either Rac1 (L61Rac) or PI 3-kinase chimera (rCD2p110) was cotransfected with HA-Akt/PKB (mean ± standard deviation of seven experiments).

Akt/PKB activation by L61Rac1 is not mediated through an autocrine loop. Because transient-transfection experiments were carried out over a relatively long time period (24 h), we could not rule outthe possibility that Akt/PKB activation might be a consequenceof the induction of autocrine growth factors, subsequently activatingPI 3-kinase in L61-Rac1-transfected cells. To investigate if thestimulatory potential of activated Rac1 involved a factor thatwas released in the medium, we employed a cell mixing protocolas follows. Either activated Rac1 (L61Rac) was cotransfected withepitope-tagged Akt/PKB (added in the same cuvette) or Rac1 andtagged Akt/PKB were transfected into separate populations of cells(two separate cuvettes), which were mixed after electroporationand cultured together until the cells were harvested and subjectedto the kinase assay. In parallel, the experiment was also performedwith the constitutively activated PI 3-kinase chimera (rCD2p110)as a positive control. Elevated Akt/PKB activity was observedonly when both constructs, L61Rac and tagged-Akt/PKB, were expressedin the same cell, and not when they were expressed in neighboringcells kept in the same culture (Fig. 2). Similar results wereobtained with the activated V12 or L61Cdc42 constructs (data notshown). It is therefore unlikely that Rac1 activates Akt/PKB throughan autocrine mechanism.

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FIG. 2. Rac1-induced PKB activation is not mediated by an autocrine factor. Jurkat cells were transfected with plasmids encoding HA-Akt/PKB (10 µg) together with either an empty vector or with the plasmid encoding L61Rac or rCD2p110 (first set); in parallel, HA-Akt/PKB, L61Rac, and rCD2p110 were transfected into separate cuvettes which were subsequently mixed in combination (second set) as indicated. Akt/PKB kinase activity was assessed 24 h posttransfection. TCR stimulation was for 10 min. Kinase activity was determined as described for Fig. 1.

UCHT1-mediated TCR triggering stimulates Rac1 activation. To assess the physiological implication of Rac1 in T-cell signaling following TCR stimulation with the UCHT1 antibody (reactivewith the $varepsilon$ -chain of the TCR), we investigated the activation ofendogenous Rac1. Relative GTP-Rac levels were estimated usingan in vitro binding assay that measures a GTP-dependent absorptionof Rac to the GTPase-binding amino terminus of the p21-activatedkinase (PAK1) (23). We treated Jurkat cells with UCHT1 for 2,5, or 10 min and performed the GTP-Rac1 pull-down experiment (21).A transient increase was observed in the amount of precipitatedRac1, with a maximal fourfold increase at 2 min of incubation(Fig. 3). Because the clone of Jurkat cells used in these experimentsstably expresses the muscarinic acetylcholine receptor, we testedcarbachol-mediated Rac1 stimulation as a positive control andfound a response with similar magnitude. These results show thatTCR triggering elicits a rapid and transient increase in the GTP-Raccontent in Jurkat cells.

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FIG. 3. UCHT1 stimulates an increase in GTP-Rac. Jurkat cells (4.5 million per condition) were incubated in PBS in the absence or presence of UCHT1 (10 µg/ml) or carbachol (0.5 mM). At the times indicated, cells were lysed, and after partial purification, Rac1 binding to the CRIB domain was assessed as described in Materials and Methods. Western blot detection of Rac1 with anti-tag antibodies is shown. The top gel represents GTP-loaded Rac eluted from the beads; the bottom gel quantitates Rac1 from the total lysate to verify equivalent levels of myc-tagged Rac1 expression.

TCR-induced Akt/PKB activation is sensitive to PI 3-kinase inhibitors as well as N17Rac. We next investigated whether Rac1 or Cdc42 could be components of the signaling pathway that couples the TCR to Akt/PKB. Forthis purpose, we ectopically expressed the inhibitory mutant forRac1, N17Rac, or N17Cdc42 together with a tagged Akt/PKB construct.As a control, the consequences of pharmacological inhibition ofPI 3-kinase on TCR-induced Akt/PKB activation were assessed. After24 h of culture of transfected cells, the activity of Akt/PKBwas measured in an in vitro kinase assay at various time pointsafter TCR engagement. Triggering of the TCR induced a rapid increasein Akt/PKB activity that was sustained for at least 30 min (Fig.4A and B). The presence of N17Rac, or the treatment with the LY249002inhibitor, suppressed protein kinase activity at all time pointstested. In contrast, N17Cdc42 showed no effect (Fig. 4C and D).Taken together, these results indicate that a functional Rac1molecule is required for TCR-mediated Akt/PKB activation.

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FIG. 4. TCR-induced Akt/PKB activation is inhibited by LY294002 or N17Rac. (A) Jurkat cells were transfected with tagged Akt/PKB (10 µg) together with either an empty vector or the dominant negative N17Rac construct (20 µg). On the next day, cells were harvested and split into three sets. The first set, transfected with control vector, was incubated in control medium. The second set, transfected with control vector, was incubated in medium containing the PI 3-kinase inhibitor LY294002 (10 µM, for 30 min at 37°C). The third set, transfected with N17Rac, was grown in control medium. Aliquots containing equal cell numbers were incubated for the time indicated with 10 µg of UCHT1 antibody per ml, and kinase activity (shown in panel B) was determined as described for Fig. 1. The figure represents one experiment out of three. (C) Jurkat cells were transfected with tagged Akt/PKB (10 µg) together with either an empty vector, the dominant negative N17Rac construct (20 µg), or the dominant negative N17Cdc42 construct (20 µg). On the next day, each set of cells was harvested, aliquots containing equal cell numbers were made, and kinase activity was determined as described for Fig. 1. (D) Expression of the inhibitory mutants was assessed by Western blotting using either anti-myc tag, or anti-Rac1 or anti-Cdc42 antibodies. The figure represents one experiment out of three.

L61Rac activates Akt/PKB upstream of PI 3-kinase. Although the major pathway for Akt/PKB activation involves a functional PI 3-kinase, other mechanisms have been described.In particular, an increase in the intracellular concentrationof calcium (45) or cyclic AMP (14) stimulates Akt/PKB activityin a wortmannin- or LY294002-insensitive manner. It was thereforeimportant to determine whether Rac1-mediated activation of Akt/PKBwas sensitive to PI 3-kinase inhibitors. Results from these experimentsare presented in Fig. 5A and show that the PI 3-kinase inhibitorLY294002 almost completely inhibited L61Rac induction of Akt/PKBactivity. These results strongly suggest that PI 3-kinase is locateddownstream of Rac1 in the signaling pathway leading to activationof Akt/PKB. The fact that both the LY249002 compound and the N17Racmutant block TCR-mediated Akt/PKB induction prompted us to investigatethe possibility that Rac1 and PI 3-kinase are positioned in alinear pathway, downstream of the TCR. We therefore performedthe reverse experiment, for which we used constitutively activePI 3-kinase mutants and studied the effects of dominant negativeRac. Two mutants of PI 3-kinase were used, the rCD2p110 mutantactivated through membrane localization (27) and the p110K227Emutant activated by point mutation (33). N17Rac did not significantlyaffect the induction mediated by either mutant of PI 3-kinase(Fig. 5B and C). H2B phosphorylation was slightly reduced in N17Rac-transfectedcells, but Western blot experiments showed that Akt/PKB expressionwas also diminished, meaning that the specific kinase activitywas unchanged in these cells. We conclude that Rac1 acts upstreamof PI 3-kinase in the TCR-mediated Akt/PKB activation pathway.

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FIG. 5. Rac1-mediated activation of Akt/PKB requires functional PI 3-kinase, but PI 3-kinase-mediated activation of Akt/PKB does not require functional Rac1. (A) Cells were transfected with Akt/PKB together with either the empty vector or the construct encoding constitutively active Rac1 (L61Rac), in the presence or in the absence of LY294002 inhibitor, in triplicate. Eighteen hours later, samples were harvested and assayed for kinase activity. Kinase activity was calculated as fold induction of basal activity (bottom) and presented as the mean ± standard deviation of triplicate samples of one representative experiment out of four. (B) Cells were transfected with Akt/PKB together with either the empty vector or the construct encoding active PI 3-kinase (rCD2p110), in the presence or in the absence of N17Rac, in triplicate. Eighteen hours later, samples were harvested and assayed for kinase activity, which is presented as the mean fold induction ± standard deviation of triplicate samples (bottom). (C) Conditions were the same as those in panel B except that rCD2p110 was replaced by p110K227E to simulate Akt/PKB activity.

Phosphorylation of threonine 308 and integrity of the PH domain are critical for Rac1- and PI 3-kinase-dependent Akt/PKB activation. The mechanism by which Akt/PKB is activated has been investigated extensively but is not yet fully elucidated (5). Translocationto the plasma membrane has not always been found necessary foractivation (14). In addition, phosphorylation of threonine 308appears to be more important for Akt/PKB activation than phosphorylationof serine 473, since replacing threonine 308 by a nonphosphorylableamino acid (alanine) always completely ablates Akt/PKB activity,whereas mutation of serine 473 has a more variable effect (2,5, 39). We next studied the requirement for the PH domainand phosphorylation at sites 308 and 473 in TCR-, L61Rac-, orrCD2p110-mediated activation of Akt/PKB. We employed a varietyof Akt/PKB constructs, either mutated at these phosphorylationsites or with the PH domain deleted, to prevent phosphorylationor translocation, respectively. Western blot experiments showedthat all mutants were expressed at similar levels in Jurkat cells(Fig. 6). When the PH domain of Akt/PKB was lacking, the kinasecould no longer be activated by L61Rac, rCD2p110 (Fig. 6), orTCR stimulation (data not shown). When threonine 308 was replacedby an alanine residue, Akt/PKB induction in response to eitherrCD2p110 or L61Rac was also ablated. In contrast, a mutation atsite 473 had little or no effect on Akt/PKB activation by rCD2p110or L61Rac. Unexpectedly, this mutant had elevated basal activityin comparison to wild-type Akt/PKB. Combined with the resultspresented in Fig. 5, these data indicate that TCR-, rCD2p110-,and L61Rac-mediated activation of Akt/PKB require both an intactPH domain and phosphorylation at residue 308.

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FIG. 6. Activation of Akt/PKB by Rac1 or PI 3-kinase requires phosphorylation at residue 308 and a PH domain. (A) Cells were transfected with wtAkt/PKB or with mutants T308A, S473A, or Akt/PKB lacking the PH domain, together with either the empty vector, the construct encoding constitutively active Rac1 (L61Rac), or the construct encoding constitutively active PI 3-kinase (rCD2p110). Eighteen hours later, samples were harvested and assayed for kinase activity. (B) The histogram presents mean values ± standard deviation obtained from two independent experiments.

TCR, L61Rac, and rCD2p110 regulate Akt/PKB phosphorylation in a similar manner. We next addressed the question whether activation of the TCR, expression of rCD2p110, or L61Rac would induce phosphorylationof Akt/PKB at positions 308 and 473. For this purpose, we usedphosphospecific antibodies directed against Akt/PKB regulatoryphosphorylation sites in the Western blot experiments. We firstinvestigated TCR-mediated phosphorylation of endogenous Akt/PKBin a time course experiment. In the absence of stimulation, basalphosphorylation was observed on both residues, which was substantiallyincreased at both sites, following TCR stimulation by UCHT1 (Fig.7A). Phosphorylation of Akt/PKB at both residues was transient,with a peak at 10 to 20 min and a decline to basal levels at 30min. When rCD2p110 or L61Rac was expressed in these cells, a similarphosphorylation pattern was seen (albeit in a nontransient fashion),with an increase in both threonine 308 and serine 473 phosphorylations(Fig. 7B). We also found that treatment of the cells with thePI 3-kinase inhibitor wortmannin ablates rCD2p110- or L61Rac-inducedphosphorylation at these sites (Fig. 7C). By using the Akt/PKBS473A mutant, we further showed that mutation of this site doesnot impair phosphorylation at threonine 308, as previously describedfor COS-1 cells (2). Lastly, we verified the effect of L61Cdc42and found a phosphorylation pattern similar to that induced byL61Rac1 (Fig. 7D). Taken together, these results indicate thatTCR, L61Rac, or rCD2p110 induce Akt/PKB phosphorylation at bothsites, indicative of a similar way of activation.

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FIG. 7. TCR stimulation, L61Rac, or rCD2p110 induce phosphorylation of Akt/PKB at threonine 308 and serine 473. (A) Jurkat cells were washed three times in serum-free medium and incubated at 37°C for 10 min before stimulation. UCHT1 (10 µg/ml) was then added for the indicated times, and samples were prepared for Western blot analysis. Phosphorylation on threonine 308 and serine 473 was assessed with phosphospecific antibodies in parallel, using two identical sets of samples for the detection. (B) Cells were cotransfected with wtAkt/PKB (10 µg) together with 30 µg of the empty vector, L61Rac, or rCD2p110. On the next day, cells were collected and washed and cell lysates were made for Western blot analysis. Phosphorylation on threonine 308 and serine 473 was assessed with phosphospecific antibodies in parallel, as described for panel A, and a third set of sample was used to assess the total Akt/PKB content in these transfected cells. (C) Cells were transfected with 15 µg of plasmids encoding rCD2p110 or L61Rac together with either 10 µg of wtAkt/PKB or 10 µg of the Akt/PKB S473A mutant, or cells were transfected with wtAkt/PKB and treated with wortmannin (+ WMN) (100 nM) or untreated as indicated. Akt/PKB phosphorylation status on threonine 308 and serine 473 was assessed as described above. (D) Cells were transfected with 30 µg of plasmids encoding L61Rac or L61Cdc42, together with 10 µg of wtAkt/PKB. Akt/PKB phosphorylation was assessed as described above, and expression of the stimulatory mutant was verified by Western blotting using anti-myc, anti-Rac, or anti-Cdc42 antibodies.

Rac1 is positioned downstream of PI 3-kinase in the pathway controlling spike formation in T cells. One of the major biological effects mediated by Rac1 is to control actin polymerization at the leading edge of the plasmamembrane, leading to the extension of lamellipodia and the subsequentformation of membrane ruffles in adherent cells. In this process,Rac1 is a clear downstream effector of PI 3-kinase. Our resultsprompted us to investigate whether a similar positioning appliesfor cytoskeletal changes in T lymphocytes. We therefore examinedthe ability of various dominant negative and constitutively activemutants of PI 3-kinase and Rac1 to alter T-cell morphology incells kept in suspension. In these experiments, green fluorescentprotein (GFP) was cotransfected with the various constructs toallow selection of transfected cells for microscopic analysisas already described (3). Cells transfected with constitutivelyactive Rac1 mutants (either V12Rac or L61Rac) or PI 3-kinase (rCD2p110)exhibited profound morphological changes, defined as membranespikes (Fig. 8A). The changes in cell morphology triggered byboth constructs were qualitatively the same. Constitutively activeRac1-mediated changes were, however, not sensitive to LY294002or wortmannin, whereas rCD2p110-induced changes were completelyinhibited. We also tested Rac1-effector loop mutants and foundthat L61RacY40C was as effective as L61Rac, whereas L61RacF37Awas inactive (Fig. 8B). These results are identical to those foundin fibroblasts (22) and confirm that with respect to the formationof membrane spikes in T cells, a similar cascade is employed asdescribed for adherent cells, a cascade in which Rac1 is positioneddownstream of PI 3-kinase.

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FIG. 8. Alteration in cell shape mediated by ectopic expression of activated Rac1 is insensitive to the PI 3-kinase inhibitor wortmannin. (A) Jurkat cells were cotransfected with the plasmid encoding GFP together with either the empty vector or plasmids encoding V12Rac or rCD2p110. Forty-eight hours later, living cells were isolated and analyzed for morphological changes under nonadherent conditions. Each set of cells was incubated with (bottom) or without (top) LY294002 for 20 min prior to analysis. (B) Jurkat cells were cotransfected with GFP as in panel A and with either the empty vector, plasmids encoding mutated forms of Rac1, or the plasmid encoding active PI 3-kinase. Forty-eight hours later, living cells were isolated and analyzed for morphological changes in the presence of wortmannin (100 nM) or LY294002 (10 µM). Data are presented as percentages of deformed cells among cells expressing GFP (mean ± standard error of the mean of three experiments).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We demonstrate that Akt/PKB is activated by the TCR in a PI 3-kinase- and Rac1-dependent manner. Constitutively active Rac1alone is sufficient to fully activate Akt/PKB in T cells, andmoreover, L61Rac-mediated stimulation of Akt/PKB activity is indistinguishablefrom that mediated by the active form of PI 3-kinase, rCD2p110,or engagement of the TCR. Phosphorylation at threonine 308 andintegrity of the PH domains were found essential for activationof Akt/PKB by the three stimuli mentioned above, whereas phosphorylationof serine 473 appeared not essential. These results position Rac1as an upstream regulator of PI 3-kinase in the activation of Akt/PKBin Jurkat lymphoid cells. Although L61Cdc42 could also induceactivation of Akt/PKB, the dominant negative mutant N17Cdc42 didnot prevent TCR-mediated Akt/PKB activation. This finding suggeststhat although L61Cdc42 can activate Akt/PKB, such a pathway isnot operative downstream of the TCR for Akt/PKBstimulation.

Our findings apparently contrast with the current idea that Rac1 and Akt/PKB are activated in parallel, downstream of a PI3-kinase-controlled signaling pathway, as demonstrated in endothelialcells (39), in COS cells (20), or in neuronal cells (38).It is reasonable to assume that differences in PI 3-kinase effectorpathways in distinct cell lineages may, at least in part, accountfor these discrepancies. In particular, differences between regulatorypathways controlling Akt/PKB can be expected in nonadherent andadherent cells, taking into account the important role of focaladhesion complexes in the regulation of the PI 3-kinase-Akt/PKBpathway. In nonadherent cells, a different type of regulationis certain to be put in place to warrant Akt/PKB-controlled cellsurvival in the absence of these complexes. Moreover, evidencehas been provided that PI 3-kinase can be either upstream or downstreamof the Rho family of GTPases, depending on which event is analyzed(29, 36). For instance, Rac1 is an effector of PI 3-kinasefor membrane ruffling (27), but Rac1 has been positioned upstreamof PI 3-kinase in the regulation of integrin-mediated cell motilityand invasiveness (19). The involvement of a lipid kinase differentfrom PI 3-kinase, downstream of Rac1, is also described for T-cellspreading on fibronectin (13). The existence of different poolsof GTPases that are spatially restricted, already suggested byother studies, provides a plausible explanation for these results(27). The coexistence of functionally distinct pools of a GTPasewithin the same cell could regulate disparate effector targetsin response to a similar upstream signal. Alternatively, distinctPI 3-kinase isoforms may be involved in these pathways, respondingto distinct upstream signaling (differential interactions). Thispossibility has been clearly illustrated in studies with macrophages,where it was shown that distinct isotypes modulate discrete cellularresponses: colony-stimulating factor 1 (CSF1)-induced DNA synthesisis under the control of p110 $alpha$ , whereas actin organization andmigration depend on a functional p110 $beta$ or p110 $delta$ (37). Sincethe lipid kinase activities of most of the PI 3-kinase enzymes,including p110 $alpha$ , p110 $beta$ , and p110 $delta$ , exhibit comparable sensitivitiesto inhibition by wortmannin or the LY294002 compound, these inhibitorswould not discriminate between different p110 isoforms in ourstudy.

Although PI 3-kinase can be recruited to the phosphorylated ITAMs upon TCR stimulation (11, 25) and in theory could beactivated by Ras through direct interaction with the p110 catalyticsubunit, these pathways appear not to be operational with respectto Akt/PKB activation. These direct links do not explain the inhibitoryeffect of dominant negative Rac1 on TCR responses, nor do theyexplain how Rac1 can activate Akt/PKB. Our data therefore favoran indirect pathway, in which an intermediate component is requiredto activate Rac1 prior to activation of PI 3-kinase. Recent studieshave given proof of such a mechanism, where the TCR activatesthe guanine nucleotide exchange factor Vav, which in turn bringsRac1 in a GTP-bound state, thus allowing for downstream signaling(21). It is through such a mode of action that we envision Racto be involved in the activation of PI 3-kinase. The followingquestion remains: why could these direct pathways not bypass therequirement for Rac1 in activation of Akt/PKB? A possible explanationcomes from studies of Akt/PKB regulation in adipocytes for whichit has been shown that the site of activation of PI 3-kinase isessential in determining activation of downstream effectors (41).In these cells, PDGF activates PI 3-kinase through direct bindingto its receptor, but PDGF is not very effective in activatingAkt/PKB and is totally ineffective in stimulating glycogen synthesis(which involves PI 3-kinase and Akt/PKB). Insulin, on the contrary,which activates PI 3-kinase through insulin receptor substrate1 (IRS-1), is very effective in stimulating Akt/PKB and in inducingglycogen synthesis. Apparently, the localization of the PI 3-kinaseis different between the two stimuli, with PDGF PI 3-kinase activityresiding mainly in the membrane, whereas with insulin, the lipidkinase activity is found in a high-speed pellet associated witha cytoskeleton-like protein complex. In T lymphocytes, LAT couldrepresent the equivalent of IRS-1, and with respect to TCR stimulation,ITAM-mediated activation of PI 3-kinase might have different cellulareffects from the LAT-mediated activation of PI 3-kinase. Becausethere are several different isoforms of both the regulatory andcatalytic subunits of PI 3-kinase, different isoforms of PI 3-kinasemay couple uniquely to different effectors in distinctmicrodomains.

We have shown that activation of Akt/PKB in Jurkat cells requires membrane localization and subsequent phosphorylation atresidue Thr-308 in the catalytic domain (activation loop). Thefollowing question remains: how is Rac1 involved in Akt/PKB regulation?Rac1 could interfere at the level of membrane recruitment, throughregulation of PI 3-kinase, or at the level of phosphorylationat threonine 308, through regulation of PDK1. Evidence for interferenceat the level of generation of PI-3,4,5-triphosphate is providedby several reports that describe a direct interaction of Rac1or Cdc42 with the p85 regulatory subunit of PI 3-kinase in a GTP-dependentmanner (6, 43). In particular, it was shown that the bcrdomain (breakpoint cluster) of p85 is instrumental in this interaction(35), which results in activation of PI 3-kinase (47). Theresults of our study would favor the model in which Rac1, in itsGTP-bound state, binds to p85, an interaction that is requiredfor the activation of the p110 catalytic subunit. It has beendemonstrated that p85 $beta$ preferentially binds to members of theRho family of GTPases (C. M. Yballe, D. A. Fruman, and L. C. Cantley,Abstr. Kestone Meet. Specificity Signal Transduction, abstr. p62,1999). Interestingly, this isoform is selectively regulated inresponse to activation of the TCR by UCHT1 (28). LAT, whoseexpression is restricted to T, NK, and mast cells, could serveas a unique scaffold for this complex, bringing together p85 $beta$ ,Rac1, and Vav (46). Interestingly, LAT and Rac1 have been foundto be permanently present in glycosphingolipid-enriched microdomainsin hematopoietic cells (4). Our observation that N17Rac hasno effect on activation of PKB by constitutively active variantsof PI 3-kinase makes it unlikely that Rac1 acts at the level ofregulation of PDK1. However, it remains possible that constitutivelyactive PI 3-kinase recruits or activates a PDK1 that differs fromthe one activated by the TCR. In this case, one can envision thatRac1 is necessary for activation or proper localization of PDK1in response to engagement of the TCR but that this role is notrequired when constitutive active PI 3-kinase comes into play(42). Further analysis is required to elucidate how Rac1, PI3-kinase, and PDK1 are linked with the TCR in the signal transductionpathway that leads to activation of Akt/PKB.

In conclusion, our data reveal that Rac1 and Akt/PKB are not always on separated pathways downstream of PI 3-kinase as previouslythought and that these GTPases can be either upstream or downstreamof PI 3-kinase, depending on the cellular event considered. Rac1is a selective regulator of the serine/threonine kinase Akt/PKBand operates upstream of PI 3-kinase in the signal transductionpathway in Jurkat Tlymphocytes.

	ACKNOWLEDGMENTS

This work was supported by a Wellcome Foundation Grant DMIH 3468. E.M.G. is a member of the INSERM organization. C.A. wassupported from a fellowship from the Fondation pour la RechercheMedicale.

We are grateful to Sarah Beach for initial technical assistance, Ludowijk Dekker for help with radioactive experiments, AlanHall and Julian Downward for various plasmids, Alain Trautmannand Peter Parker for helpful discussions, Bart Vanhaesebroeckand Jacques Nunes for advice, and Doreen Cantrell and Robert Lechlerfor constantsupport.

	FOOTNOTES

^* Corresponding author. Mailing address: Growth Factors and Differentiation Laboratory, Batiment de Biologie Animale, Universityof Bordeaux I, Avenue des facultés, 33 405 Talence Cedex, France.Phone: (33) 5 56 84 89 25. Fax: (33) 5 56 84 87 05. E-mail: e.genot{at}croissance.u-bordeaux.fr.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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