Ig Receptor Binding Protein 1 (alpha 4) Is Associated With a Rapamycin-Sensitive Signal Transduction in Lymphocytes Through Direct Binding to the Catalytic Subunit of Protein Phosphatase 2A

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Blood, Vol. 92 No. 2 (July 15), 1998: pp. 539-546
Ig Receptor Binding Protein 1 ( $alpha$ 4) Is Associated With a Rapamycin-Sensitive Signal Transduction in Lymphocytes Through Direct Binding to the Catalytic Subunit of Protein Phosphatase 2A

By Seiji Inui, Hideki Sanjo, Kazuhiko Maeda, Hideyuki Yamamoto, Eishichi Miyamoto, and Nobuo Sakaguchi
From the Departments of Immunology and of Pharmacology, Kumamoto University School of Medicine, Kumamoto, Japan.

  ABSTRACT

Abstract
Introduction
Methods
References

Rapamycin is an immunosuppressant that effectively controls various immune responses; however, its action in the signal transductionof lymphocytes has remained largely unknown. We show here thata phosphoprotein encoded by mouse $alpha$ 4 (m $alpha$ 4) gene transmitting asignal through B-cell antigen receptor (BCR) is associated withthe catalytic subunit of protein phosphatase 2A (PP2Ac). The middleregion of $alpha$ 4, consisting of 109 amino acids (94-202), associatesdirectly with PP2Ac, irrespective of any other accessory molecule.Rapamycin treatment disrupts the association of PP2Ac/ $alpha$ 4 in parallelwith the inhibitory effect of lymphoid cell proliferation. Theeffect of rapamycin was inhibited with an excess amount of FK506that potentially completes the binding to FKBP. Rapamycin treatmentalso suppresses the phosphatase activity of cells measured byin vitro phosphatase assay. Introduction of the m $alpha$ 4 cDNA intoJurkat cells or the increased association of PP2Ac/ $alpha$ 4 by the culturewith low serum concentration confers cells with rapamycin resistance.Moreover, glutathione S-transferase (GST)- $alpha$ 4 augments the PP2Aactivity upon myelin basic protein (MBP) and histone in the invitro assay. These results suggest that $alpha$ 4 acts as a positiveregulator of PP2A and as a new target of rapamycin in the activationof lymphocytes.

  INTRODUCTION

Abstract
Introduction
Methods
References

CROSS-LINKING OF B-cell antigen receptor (BCR) induces activation of multiple signal transduction pathways associated withthe BCR-complex.^1-6 However, the signal affected by the Immunosuppressantrapamycin has largely remained unsolved. Two analogous immunosuppressants,cyclosporin A (CsA) and FK506, bind to cyclophilin and FKBP12,respectively,⁷ both of which inhibit the activity of calcineurin(protein phosphatase 2B),⁸ a phosphatase that regulates NF-ATactivity involved in T-cell receptor signal transduction.⁹Rapamycin of a similar structure to FK506 associates with thesame FKBP, but the action thereafter is likely to be different.¹⁰^,¹¹Rapamycin is shown to inhibit the growth signal mediated throughthe interleukin-2 receptor (IL-2R) and the downstream moleculeinvolved in the rapamycin-sensitive pathway is named TOR (targetof rapamycin) in yeast and mammalian cells.^12-16 The rapamycin/FKBPcomplex interacts with TOR, subsequently inhibiting the activityof S6 kinase (S6K) that promotes cell cycle progression at G1to S phase.¹⁷ Interaction of rapamycin/FKBP also inhibits thedownregulation of p27 kip, which negatively regulates cell cycleprogression.¹⁸ Despite this evidence, it has not been determinedwhether the molecules are interacting directly in the downstreamsignals through rapamycin/FKBP/TOR-sensitive pathways.

In a search of molecules involved in the BCR-mediated signal transduction, we identified a component associated with Ig- $alpha$ (CD79a, MB-1) and isolated a candidate cDNA clone ( $alpha$ 4) using amonoclonal antibody (Ab).^{19, 20} The $alpha$ 4 is phosphorylated in vivo by phorbol 12-myristate 13-acetate,and BCR cross-linking induces a transient association of $alpha$ 4 witha tyrosine-phosphorylated molecule, indicating the involvementof the $alpha$ 4 in the BCR-mediated signal transduction.²⁰ The molecule,now designated as Ig receptor binding protein 1 ( $alpha$ 4), has severalphosphorylatable sites by protein kinase C and casein kinase 2(CK2) and a proline-rich sequence that is a possible interactionsite with SH3 motif. Recently, a yeast homologue of $alpha$ 4 named Tap42was cloned, and it was shown that nutrient growth signal inducesassociation of Tap42 with protein phosphatase 2A (PP2A) and therelated phosphatase SIT4.²¹ It was also shown that rapamycininhibits the growth of yeast by dissociating Tap42 from PP2A/SIT4.

PP2A is a major intracellular serine/threonine phosphatase and plays pivotal roles in the control of cell cycle, proliferation,viral transformation, and metabolic pathways.^22-24 PP2A representscomplex structures in various cells as a family of holoenzymesconsisting of a common core dimer of a 39-kD catalytic C subunitand a 65-kD A subunit associated with various regulatory B subunits.A and C subunits are expressed ubiquitously, but B subunits areexpressed in a tissue-specific and developmentally regulated manner.^25-27These regulatory subunits can modify PP2A enzyme activity, substratespecificity, or subcellular localization of the enzyme.²³^,²⁴^,²⁶^,²⁷Recent studies further reported different types of binding moleculesto the catalytic subunit of PP2A (PP2Ac). These types includeeRF1,²⁸ Hox11,²⁹ and CK2,³⁰ which showed binding to PP2Acin cells in addition to their unique functions such as the proteinsynthesis, the nuclear transcription factor activity, or the kinaseactivity of several cellular protein molecules. These moleculespresumably participate in cell proliferation: eRF1 targets thePP2A to polysome without affecting enzyme activity, Hox11 inhibitsthe enzyme activity of PP2A and induces M phase of the cell cycle,and, conversely, CK2 augments PP2Ac activity by phosphorylatingPP2Ac.

We show here that human Igbp1/ $alpha$ 4 (h $alpha$ 4) is directly associated with PP2Ac in human lymphoid cell lines through the middle portionof $alpha$ 4 protein. Rapamycin disrupts the PP2Ac/ $alpha$ 4 interaction inrapamycin-sensitive Jurkat cells but not in rapamycin-resistantRaji cells. We demonstrate that the introduction of mouse $alpha$ 4 (m $alpha$ 4)into Jurkat cells conferred rapamycin resistance, indicating thatPP2A/ $alpha$ 4 acts as a new target of rapamycin. Furthermore, $alpha$ 4 augmentsthe enzyme activity of PP2A both in vitro and in vivo and rapamycininhibits the PP2A activity in Jurkat cells by disrupting the PP2A/ $alpha$ 4association.

  MATERIALS AND METHODS

Abstract
Introduction
Methods
References

Reagents and Abs. Rapamycin was purchased from Wako Chemicals (Osaka, Japan). FK506 was purchased from Fujisawa Pharmaceutical Co (Osaka, Japan).Anti-PP2Ac Ab was purchased from Upstate Biotechnology Inc (LakePlacid, NY). Anti-m $alpha$ 4 Ab was prepared and characterized previously.²⁰Anti-h $alpha$ 4 serum was prepared by immunizing rabbits with the GST-h $alpha$ 4.The serum purified by the GST-h $alpha$ 4 affinity column was used asanti-h $alpha$ 4.

cDNA construct and fusion proteins. Human PP2Ac and h $alpha$ 4 cDNAs were prepared by reverse transcriptase with oligo dT primer from mRNA of human B-lymphoid cell lineRPMI8866 and the subsequent polymerase chain reaction (PCR) reaction.The primers for the amplification were 5 $'$ -GGATCCTCATGGACGAGAAGGTGTTC-3 $'$ and 5 $'$ -GGATCCCAGGAAGTAGTCTGGGGTAC-3 $'$ for PP2Ac³¹ and 5 $'$ -GGATCCAGATGGCTGCTGAGGACGAG-3 $'$ and 5 $'$ -GGATCCGCCCATGTTCTGTCGGTTCC-3 $'$ for $alpha$ 4, according to thesequence reported previously (Gene Bank accession no. Y08915).Both cDNAs were subcloned into the BamHI site of pGEX3X vector.The constructs with truncated h $alpha$ 4 cDNAs were prepared as follows.H $alpha$ 4 (1-93), (94-293), and (94-202) cDNA fragments were preparedby digestion with BamHI-HincII, HincII-EcoRI, and HincII-EcoRVof human $alpha$ 4 cDNA and were subcloned into BamHI/Sma I, Sma I/EcoRI,and Sma I sites of pGEX3X vector, respectively. H $alpha$ 4 (1-293) and(210-293) were prepared from the EcoRI fragments of h $alpha$ 4 cDNAsisolated independently from RPMI8866 and IM9 cDNA libraries, respectively,and were subcloned into the EcoRI site of pGEX2T vector. The orientationsand the reading frames of the cDNA inserts were verified by nucleotidesequencing of the final constructs. GST fusion proteins were preparedby affinity chromatography, as described.²⁰

Cell lysis, immunoprecipitation, and Western blotting. Cells were lysed in lysis buffer containing 1% Nonidet P-40, 150 mmol/L NaCl, 10 mmol/L Tris-Cl (pH 7.8), 1 mmol/L EDTA, 0.05%NaN₃, 100 mmol/L NaVO₄, 1 mmol/L phenylmethylsulfonylfluoride(PMSF), and 10 µg/mL aprotinin. The lysates were centrifuged for5 minutes at 12,000g at 4°C to remove nuclei and insoluble materialsand were used for immunoprecipitation as previously described¹⁹or for the in vitro phosphatase assay. The lysates of 1 × 10⁷ cells were incubated with specific Abs for 2 hours at 4°C. Immunecomplexes were collected with 30 µL of protein A-Sepharose beads(Pharmacia Biotech, Uppsala, Sweden), washed 4 times with thelysis buffer, and then resuspended with sodium dodecyl sulfate(SDS) sample buffer. For the pull-down assay, the lysate of 5× 10⁷ cells was incubated with 10 µg of each fusion protein and theprecipitated molecules were collected with Glutathione-Sepharosebeads (Pharmacia). After SDS-polyacrylamide gel electrophoresis(SDS-PAGE), separated proteins were transferred onto nitrocellulosefilters by electroblotting. PP2Ac or $alpha$ 4 was detected by anti-PP2AcAb or anti-h $alpha$ 4 Ab at the dilution of 1/1,000 or 1/400, respectively.The blots were developed using an enhanced chemiluminescence kit(Amersham Life Science, Tokyo, Japan) according to the manufacturer'sprotocol.

Proliferation assay. Cells were cultured at 1 × 10⁴ cells/well in 96-well microtiter plates containing 200 µL of RPMI-1640 culture medium with variousconcentrations of rapamycin for 48 hours. Relative cell numberswere analyzed by WST-1 assay.³² Cells were pulsed with 50 µLof WST-1 solution (1 mmol/L WST-1 and 20 mmol/L of 1-methoxy PMS),a compound of soluble tetrazolium (Dojindo, Kumamoto, Japan),for the last 4 hours. The absorbance was then measured with anenzyme-linked immunosorbent assay (ELISA) plate reader at a wavelengthof 405 nm.

Transfection. H $alpha$ 4 cDNA was subcloned into pCDM8 expression vector. Cells were transfected with 20 µg of $alpha$ 4 cDNA and 2 µg of pSV2neo, whichwere linearized by Sac II and BamHI, respectively. These DNAswere transfected into Jurkat cells by the electroporation method,as previously described.³³ After 2 days in the culture medium,transfected cells were selected in the presence of 1.0 mg/mL G418(GIBCO, Grand Island, NY).

Phosphatase assay. The holoenzyme of PP2A from rat brain was purified according to the protocol described previously,³⁴ and the preparationof PP2A did not contain any activities of protein phosphatase1, calcineurin, and protein phosphatase 2C. MBP or histone H1was phosphorylated by cyclic AMP-kinase with 0.2 mmol/L [ $gamma$ -³²P]-ATP (3,000 to 5,000 cpm/pmol) for 60 minutes under standardassay conditions. Phosphorylated MBP or histone H1 were heat-treatedat 65°C for 15 minutes to remove cyclic AMP kinase activity andcollected by ammonium sulfate fractionation (0% to 80%) in thepresence of 1 mg/mL bovine serum albumin (BSA). The proteins werewashed 3 times with 80% ammonium sulfate and dialyzed againsta buffer containing 10 mmol/L Tris-HCl (pH 7.5), 10 mmol/L 2-mercaptoethanol,and 10% (vol/vol) glycerol overnight. The standard assay systemfor dephosphorylation of MBP or histone H1 contained, in a finalvolume of 25 µL, 50 mmol/L imidazole-HCl (pH 7.0), 0.1% 2-mercaptoethanol(vol/vol), 1 mmol/L EDTA, 52 µg/mL of phosphorylated MBP or histoneH1, and each sample of protein phosphatase 2A. The okadaic acid(OA)-sensitive phosphatase activity was calculated after measuringthe phosphatase activities in vitro in the presence and absenceof 50 nmol/L of okadaic acid (Sigma Chemicals Co, St Louis, MO),respectively. After 10 minutes of incubation at 30°C, 100 µL of15% trichloroacetic acid was added, and the protein phosphataseactivities were measured by the release of free ³²P from ³²P-labeled substrates. All assays were performed in triplicate.

  RESULTS AND DISCUSSION

Direct association of Igbp1 ( $alpha$ 4) with PP2Ac. Because the direct association of $alpha$ 4 with PP2Ac was expected, we examined the coprecipitation of $alpha$ 4 and PP2A in lymphoid cellsby anti-PP2Ac Western blot analysis. Cell lysate of Jurkat T-cellswas first immunoprecipitated with the anti-h $alpha$ 4 Ab. Anti-PP2AcAb clearly detected a 39-kD PP2Ac in the $alpha$ 4 immunoprecipitatewith rabbit anti-h $alpha$ 4 Ab as well as in whole cell lysates, indicatingthat PP2Ac was coprecipitated with $alpha$ 4 in Jurkat (Fig 1A). To confirmthe association of PP2Ac/ $alpha$ 4, it was necessary to detect an associationof $alpha$ 4 in the anti-PP2Ac immunoprecipitate. This reciprocal experimentfailed due to the close migration of $alpha$ 4 to nonspecific bands fromrabbit anti-h $alpha$ 4 Ab (data not shown). Therefore, we used a pull-downassay using a recombinant protein of GST-PP2Ac to precipitatethe associated molecules from Jurkat. Cell lysates were mixedwith affinity-purified GST-PP2Ac and precipitated with Glutathione-Sepharosebeads. Western blot analysis of the precipitate with anti-h $alpha$ 4Ab clearly detected a 45-kD band identical to the $alpha$ 4 recognizeddirectly with the anti-h $alpha$ 4 Ab (Fig 1B). It was detected only withthe GST-PP2Ac but not with the control GST. We confirmed similarresults using WEHI 231 B cells (data not shown). These resultsdemonstrate that $alpha$ 4 is associated with PP2Ac in lymphoid cells.PP2Ac associates with a regulatory subunit PR65, and this coredimer can further interact with various cellular regulatory components.²³^,²⁴To understand the molecular interaction directly, we studied theassociation of $alpha$ 4 and PP2Ac using a recombinant $alpha$ 4. Radiolabeled $alpha$ 4 synthesized in vitro by reticulocyte lysate from murine $alpha$ 4cDNA in pGEM3Z vector by T7 polymerase in the presence of ³⁵S-methionine was mixed with GST-PP2Ac. A 45-kD $alpha$ 4 protein wascoprecipitated specifically with GST-PP2Ac but not with GST alone(Fig 1C), indicating that the association of $alpha$ 4 and PP2Ac didnot require other cellular components from lymphocytes. Althoughthe $alpha$ 4 protein contained the reticulocyte lysate, it suggestedthat the association of $alpha$ 4 protein with PP2Ac does not requireconventional regulatory components for PP2Ac existing in lymphoidcells. In the same binding assay, we examined the involvementof rapamycin. Rapamycin did not directly induce the dissociationof $alpha$ 4 and PP2Ac (data not shown).

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Fig 1. Association of $alpha$ 4 with PP2Ac. (A) Cell lysates of Jurkat were immunoprecipitated for 2 hours at 4°C with either anti-h $alpha$ 4 Ab,anti-PP2Ac Ab, or preimmune serum. The immunoprecipitates wereseparated by SDS/10% PAGE and transferred to a nitrocellulosefilter. The filter was then probed with anti-PP2Ac Ab. The migrationof human PP2Ac is indicated. (B) Cell lysates of Jurkat (50 ×10⁶ cells) were mixed with 10 µg of GST-PP2Ac fusion protein or thecontrol GST alone. The precipitates (15 × 10⁶ cell equivalents per lane) were captured by Glutathione-Sepharosebeads, separated by SDS/10% PAGE, and transferred to nitrocellulosefilter. The filter was immunodetected with anti-h $alpha$ 4 Ab. Jurkatcell lysate (1 × 10⁶/lane) was used as a positive control for $alpha$ 4 immunoblotting. Themigration of $alpha$ 4 is indicated. (C) m $alpha$ 4 was synthesized in vitroin the presence of ³⁵S-methionine using an in vitro translation kit (Amersham). GST-PP2Acor GST alone was mixed with radiolabeled $alpha$ 4 and precipitated byGlutathione-Sepharose. Recovered proteins were separated by SDS-PAGEand subsequently developed by autoradiography. (D) Schematic diagramof GST- $alpha$ 4 fusion proteins used to localize the region that isnecessary for binding to PP2Ac. Numbers on the left side indicatethe positions of amino acid residues of $alpha$ 4. Restriction enzymesites used for construction of mutants are shown. Ba, BamHI; EI,EcoRI; EV, EcoRV; HII, HincII. Hatched regions indicate the bindingsite. The intensities of the PP2Ac bands in the pull-down assayperformed in (E) are indicated by ++, +, and $-$ . (E) Various mutantsof GST- $alpha$ 4 fusion proteins were tested for their binding activitiesto PP2Ac.

Next, we studied the specific binding site of $alpha$ 4 to PP2Ac. Deletion mutants of $alpha$ 4 prepared as GST-fusion proteins were usedto determine the binding region for PP2Ac. Western blot analysiswith anti-PP2Ac Ab showed that the middle region of $alpha$ 4 encompassing109 amino acids was necessary and sufficient for the binding toPP2Ac but that the amino- or carboxyl-terminal portion did notbind to PP2Ac in this assay (Fig 1D and E). The amino acid sequence,required for binding to PP2Ac, did not show any unique motif.The SH3-binding consensus motif (PEKPPMKP) present in $alpha$ 4²⁰ was not involved in this interaction. A similar association ofPP2A was recently shown for Hox11 and eRF1. Hox11 is capable ofbinding to PP2Ac directly, inhibiting cell cycle arrest at thetransition from G2 to M phase. The interaction site was narroweddown to amino acids 149 to 199 of Hox11.²⁹ The carboxyl-terminalside 43 amino acids of human eRF1 (amino acids 338-381) are responsiblefor the binding to PP2Ac.²⁸ In a homology comparison of theamino acid sequences, no obvious similarity was found to the bindingsite on $alpha$ 4 (data not shown).

Involvement of PP2Ac/ $alpha$ 4 in rapamycin-sensitive signal transduction pathway. To determine the functional contribution of the PP2Ac/ $alpha$ 4 complex in lymphocytes, we tested whether rapamycin affects the associationof $alpha$ 4 with PP2Ac. Rapamycin sensitivity varies among cell lines.³⁵The growth of a T-cell line Jurkat was sensitive to rapamycintreatment, but that of a B-cell line Raji was resistant (Fig 2A).Jurkat cells were treated with various concentrations of rapamycin,and the association was monitored by immunoprecipitation withanti-h $alpha$ 4 Ab followed by immunoblot with anti-PP2Ac Ab. Rapamycintreatment induced the dissociation of PP2Ac from $alpha$ 4 in a dose-dependentmanner (Fig 2B). The concentration of rapamycin that induced thedissociation of PP2Ac/ $alpha$ 4 was comparable to that required for growthinhibition. Dissociation of PP2Ac from $alpha$ 4 was discernible after12 hours and almost no PP2Ac remained in association with $alpha$ 4 after48 to 72 hours of treatment (Fig 2C). The amount of $alpha$ 4 proteinwas quite similar in each lane, as confirmed on the same filterby reprobing with anti- $alpha$ 4 antibody (Fig 2B). Existence of PP2Acand h $alpha$ 4 proteins was also confirmed by Western blot with the wholecell lysates (Fig 2B). Interestingly, rapamycin could not dissociate $alpha$ 4 from PP2Ac in rapamycin-resistant Raji cells (Fig 2B and C).Furthermore, we examined whether the dissociation of the $alpha$ 4/PP2Acby the treatment of rapamycin was inhibited in the presence ofFK506, which binds to the same binding molecule FKBP (Fig 2D).Increasing concentrations of FK506 recovered the association of $alpha$ 4 and PP2Ac. PP2A is obviously associated with a number of signalingmolecules in a variety of cell types,²³^,²⁴ but none of themolecules was shown to be affected by rapamycin treatment. Thisresult is, to our knowledge, the first report in which rapamycintreatment dissociates the complex structure composed of PP2Ac.

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Fig 2. Rapamycin-sensitive dissociation of PP2Ac and $alpha$ 4. (A) Rapamycin sensitivity was measured on the proliferation of Jurkat andRaji. Jurkat is sensitive to rapamycin treatment, but Raji isrelatively insensitive. Relative cell proliferation was comparedafter measuring by WST-1 assay.³¹ (B) Rapamycin induces thedose-dependent dissociation of PP2Ac/ $alpha$ 4 complex in rapamycin-sensitiveJurkat but not in rapamycin-resistant Raji. Cell lysates wereprepared after the culture and the PP2Ac coprecipitated with $alpha$ 4is detected by Western blot analysis. After detecting signals,the probe on the filter was stripped off according to the company'sprotocol (Amersham). The filter was then reprobed with anti-h $alpha$ 4Ab to see the amount of h $alpha$ 4 protein in each lane. To further confirmthe existence of similar amounts of PP2Ac and h $alpha$ 4 proteins, Westernblot analysis was performed with the whole cell lysates (WCL).(C) Both Jurkat and Raji cells were treated with rapamycin (330nmol/L) and the PP2Ac associated with $alpha$ 4 was detected by Westernblot analysis. Cells were harvested at the time points indicatedand the immunoblot was developed with anti-PP2Ac Ab. The migrationof PP2Ac is as indicated. (D) Effect of FK506 was examined duringthe treatment of rapamycin. Varying concentrations of FK506 wereadded in the culture of Jurkat with rapamycin (10 nmol/L). Thecells were harvested after 48 hours and lysed as described above.The $alpha$ 4-associated PP2Ac was detected on Western blot analysis.The PP2Ac signals were measured by the densitometric analysisand are shown as the relative intensities (%) of control culturein the absence of rapamycin. The amounts of h $alpha$ 4 immunoprecipitatedwith anti-h $alpha$ 4 Ab were controlled by reprobing the same filter(data not shown).

The effect of the increased $alpha$ 4 expression was examined by DNA transfection of m $alpha$ 4 into human cells. The introduced m $alpha$ 4 wasclearly identified as a larger band on Western blot analysis bythe anti-m $alpha$ 4 Ab. Jurkat-m $alpha$ 4 transfectant expressed m $alpha$ 4 in additionto h $alpha$ 4 detected by the anti-h $alpha$ 4 Ab, but parental Jurkat cellsand Jurkat transfectants with neomycin-resistant gene alone (Jurkat-neo)expressed h $alpha$ 4 only (Fig 3A). Rapamycin inhibited the proliferationof Jurkat cells, as shown in Fig 3B. Jurkat transfected with m $alpha$ 4,expressing the double amounts of $alpha$ 4 protein, became less susceptibleto rapamycin in comparison to parental Jurkat cells (Fig 3B).The control transfectant expressing neomycin alone was as sensitiveto rapamycin as parental Jurkat cells. M $alpha$ 4 is 93% homologous toh $alpha$ 4 at amino acid level (data not shown), and we assumed thatthis highly conserved structure of m $alpha$ 4 allowed it to functionadditively with h $alpha$ 4 in Jurkat cells. Because conditions of cellculture affect the rapamycin sensitivity,³⁶ we tested whethera reduced concentration of serum in culture medium influencesthe expression of $alpha$ 4 and its association with PP2Ac. Jurkat cellscultured in medium containing less than 2% fetal calf serum (FCS)became more resistant to rapamycin than those cultured with 10%FCS (Fig 3C). Low concentration of serum did not change the expressionlevel of $alpha$ 4 (data not shown) and PP2A (Fig 3D; WCL) themselves;however, the association of $alpha$ 4 and PP2A was augmented in Jurkatwhen cultured in the medium with less than 2% FCS (Fig 3D; Ippt).These results indicate that the PP2A/ $alpha$ 4 association functionsas a new target of rapamycin in lymphoid cells.

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Fig 3. The correlation of $alpha$ 4 expression and rapamycin sensitivity. (A) Expression of $alpha$ 4 in transfectants was shown by Western blotanalysis. Jurkat transfectants expressing m $alpha$ 4 or neomycin-resistantgene, parental Jurkat, and mouse B-cell line WEHI 231 were lysedin lysis buffer containing 1% NP-40. The immunoblot was developedwith anti-m $alpha$ 4 Ab (left side) or anti-h $alpha$ 4 Ab (right side). Anti-h $alpha$ 4Ab recognizes both h $alpha$ 4 and m $alpha$ 4 proteins. The migrations of mouseand h $alpha$ 4 are as indicated. (B) Cells were cultured at 1 × 10⁴/well in 200 µL of medium with various concentrations of rapamycinfor 48 hours. Relative cell numbers were analyzed by WTS-1 assay.Results are shown as the percentage of the control culture withoutrapamycin. Data are representative of 4 independent experimentsand are shown as the mean of duplicate samples ± standard deviations.(C) Jurkat cells were cultured at 1 × 10⁵/mL with various concentrations of serum as 10%, 2%, or 0.4% for72 hours. Rapamycin sensitivity was measured by the WTS-1 assayas described above. (D) Jurkat cells were cultured in the mediumthat contained either 10%, 2%, or 0.4% of FCS for 72 hours. Theamounts of PP2Ac bound to $alpha$ 4 were detected after immunoprecipitationwith anti-h $alpha$ 4 Ab, followed by anti-PP2Ac Western blot analysis.Total amounts of PP2Ac were detected using whole cell lysate (WCL).Columns below the bands show the arbitrary units to indicate therelative intensity of the bands as determined by a densitometer.

Regulation of PP2A activity by $alpha$ 4 molecule. To evaluate the catalytic activity of PP2Ac bound to $alpha$ 4, an in vitro phosphatase assay was performed using OA, the specificinhibitor for PP2A activity. All results are shown as the OA-sensitivephosphatase activity. PP2Ac coimmunoprecipitated with $alpha$ 4 showedphosphatase activity upon [³²P]-radiolabeled substrate MBP in a similar way as PP2Ac immunoprecipitatedwith anti-PP2Ac antibody (Fig 4A). This result clearly indicatesthat PP2Ac is associated with $alpha$ 4 in lymphocytes and suggests thatrapamycin treatment may alter the activity of PP2A. Because manyPP2Ac-associated molecules have negative regulatory functionson phosphatase activity,²³^,²⁴ we tested whether phosphataseactivity might change in the cells by the dissociation of PP2Ac/ $alpha$ 4complex. Therefore, the amount of PP2Ac on Western blot analysisand the phosphatase activities in total cell lysates were examinedafter rapamycin treatment. Interestingly, rapamycin treatmentinduced a downregulation of phosphatase activity in rapamycin-sensitiveJurkat, but the activity did not change in rapamycin-resistantRaji (Fig 4B). The decrease of phosphatase activity in Jurkatcells after rapamycin treatment is not as marked as the dissociationstate of the $alpha$ 4/PP2Ac complex. Repeated experiments showed similarresults (data not shown), suggesting that the PP2Ac activity mightbe regulated by various regulatory molecules in lymphoid cells.Rapamycin treatment of various concentrations did not alter thelevel of PP2Ac expression in both Jurkat and Raji (Fig 4C). Theseresults suggest that association with $alpha$ 4 maintains higher phosphataseactivity of PP2Ac in lymphoid cells. To further study a regulatoryfunction of $alpha$ 4 on PP2A activity, enzymatic activity was comparedbefore and after $alpha$ 4 cDNA transfection into COS-7 cells. The $alpha$ 4-transfectedCOS-7 showed the increased PP2A activity when compared with mock-transfectedCOS-7 cells (Fig 4D). The change of phosphatase activity was alsoaffected in the presence of rapamycin in the $alpha$ 4-COS transfectant,which was again recovered by the addition of FK506 (Fig 4D). Theseresults further support the idea that $alpha$ 4 is involved as a targetof rapamycin and is functionally composed in the rapamycin/FKBPcomplex. The rapamycin resistance of lymphocytes is probably controlledby the association with PP2Ac.

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Fig 4. Binding of phosphatase activity to $alpha$ 4 in cells. (A) Cell lysates of Jurkat were immunoprecipitated by either anti-h $alpha$ 4 Ab,anti-PP2Ac Ab, or normal rabbit serum (NRS). Phosphatase activitiesin the complex were assayed using ³²P-labeled MBP as a substrate. Results are shown as the percentageof input ³²P dephosphorylated from MBP. Optimal enzyme and substrate ratioand the incubation time were determined with the rat PP2A purifiedas described previously.³³ Data are the mean of duplicate samples+ standard deviations. (B) Jurkat ( $black-square$ ) or Raji ( $square$ ) cells were treatedwith various concentrations of rapamycin for 48 hours. The cellswere lysed and assayed for their phosphatase activity using ³²P-labeled MBP as a substrate. The activity was measured in thepresence or absence of 50 nmol/L of OA and the value without OAsubtracted from that with OA was calculated. For comparison, thevalue of lysate without rapamycin was set as 100%. Protein concentrationsof samples were adjusted and the amounts of PP2Ac protein wereshown in (C). (C) Western blot analysis to demonstrate the amountsof PP2Ac in all samples. Results indicate that proteins are equallyadjusted before measuring the phosphatase activities. (D) COS-7cells were transfected with the m $alpha$ 4 cDNA in pCDM8 or control vector.Cells were lysed after 72 hours of culture and the phosphataseassay was performed as in (B). The effect of rapamycin (10 nmol/L)was measured on m $alpha$ 4-COS transfectant (R+/F $-$ ) in comparison tothe culture without rapamycin (R $-$ /F $-$ ). Recovery of phosphataseactivity was measured by the addition of FK506 (100 nmol/L) (R+/F+).(E) Upregulation of phosphatase activity by $alpha$ 4. Effect of GST- $alpha$ 4() or GST alone ( $square$ ) was measured in the in vitro phosphataseassay using the phosphorylated MBP or histone H1 with purifiedPP2A. Regulatory activity on the PP2A was shown as the percentageof control measured only with substrate and enzyme.

Next, we attempted to directly demonstrate a positive regulation of PP2Ac activity with $alpha$ 4 protein. Affinity-purified GST- $alpha$ 4protein was mixed with purified PP2A in the in vitro phosphataseassay using phosphorylated MBP as a substrate. The phosphataseactivity was augmented in the presence of $alpha$ 4 protein (Fig 4E).The effect was obvious on phosphorylated-histone (right panel),but less on phosphorylated-MBP (left panel) and -casein (datanot shown) as substrates. The augmentation of phosphatase activitywas not observed with other GST-fusion proteins such as with truncated $alpha$ 4 lacking the amino acids (94-202) (data not shown). Many PP2A-bindingmolecules either negatively regulate phosphatase activity²³^,²⁴or do not exhibit any modulating activity, such as eRF1.²⁸ Recently,Heriche et al³⁰ reported that PP2A is directly associated withCK2 $alpha$ , whose catalytic activity appeared to enhance PP2A activityand is presumably involved in deactivation of the mitogen-activatedprotein kinase pathway.

We have demonstrated that $alpha$ 4 is involved in the rapamycin-sensitive signal transduction pathway through the association withPP2Ac and probably controls phosphorylation states of certainfunctional molecules involved in cell cycle progression. PP2Adephosphorylates and inactivates several of the growth factor-stimulatedprotein kinases in vitro, suggesting that PP2A normally functionsas a suppressor of cell growth.²³^,²⁴ Growth factor-stimulatedprotein kinases (MAPK/ERKs) phosphorylate a number of substratesin addition to 90-kD S6 kinase and several transcription factors.³⁷Treatment of active preparations of MAPK/ERK with the catalyticsubunit of PP2A causes dephosphorylation of phospho-threonineand inhibition of kinase activity.³⁸ Treatment of several differentcell types with OA causes activation of MAPK/ERKs,³⁹ demonstratingthat a constitutive level of serine/threonine phosphatase activityis necessary to maintain MAPK/ERKs in a low-activity state. Inour report, rapamycin inhibits the proliferation of cells by dissociatingPP2Ac from $alpha$ 4. The results suggest that PP2A may function undercertain conditions as a positive regulator of cell proliferation.

Rapamycin/FKBP complex interacts directly with mTOR and inhibits its enzymatic activity. Signals induced by growth factorsactivate mTOR, which then activates S6K⁴⁰ and PHAS1.⁴¹ PHAS1 is a direct substrate of mTOR, but the interactionof S6K with mTOR is indirect and the mechanism of S6K activationby mTOR is not determined yet. The mechanism of inhibiting activityof p27 degradation by rapamycin is not clarified either.⁴²^,⁴³In our report, we demonstrated that rapamycin disrupts the PP2A/ $alpha$ 4association, which is now considered as a target of rapamycinin the growth inhibition of lymphoid cells. Di Como and Arndt²¹suggested that Tap42/SIT4 or Tap42/PP2A might be located downstreamof TOR signaling in yeast. It is important to identify the molecularinteraction between PP2A/ $alpha$ 4 and mTOR. The PP2A/ $alpha$ 4 signaling pathwaymight be also involved in B-cell activation, because rapamycinpotentially suppresses the B-cell activation by BCR⁴⁴ or cytokine stimulation.⁴⁵

During the preparation of this manuscript, Murata et al⁴⁶ reported that $alpha$ 4 binds to PP2Ac. Our results presented here aswell as theirs suggest that the Igbp1 ( $alpha$ 4) is involved in therapamycin-sensitive signal transduction pathway, which might regulatethe PP2Ac activity for the cell cycle progression of lymphocytes.

  FOOTNOTES

   Submitted October 14, 1997; accepted March 10, 1998.
   Supported by the grants from the Ministry of Education, Sports, Science and Culture, Japan.
   Address reprint requests to Nobuo Sakaguchi, MD, Department of Immunology, Kumamoto University School of Medicine, 2-2-1,Honjo, Kumamoto 860, Japan; e-mail: nobusaka{at}kaiju.medic.kumamoto-u.ac.jp
   The publication costs of this article were defrayed in part by page charge payment. This article must therefore be herebymarked "advertisement" is accordance with 18 U.S.C. section 1734solely to indicate this fact.

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Abstract
Introduction
Methods
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Ig Receptor Binding Protein 1 (4) Is Associated With a Rapamycin-Sensitive Signal Transduction in Lymphocytes Through Direct Binding to the Catalytic Subunit of Protein Phosphatase 2A

Ig Receptor Binding Protein 1 ( $alpha$ 4) Is Associated With a Rapamycin-Sensitive Signal Transduction in Lymphocytes Through Direct Binding to the Catalytic Subunit of Protein Phosphatase 2A