Folding of Insulin Receptor Monomers Is Facilitated by the Molecular Chaperones Calnexin and Calreticulin and Impaired by Rapid Dimerization

doi:10.1083/jcb.141.3.637

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© The Rockefeller University Press, 0021-9525/1998//637 $5.00
The Journal of Cell Biology, Volume 141, Number 3, , 1998 637-646

Articles

Folding of Insulin Receptor Monomers Is Facilitated by the Molecular Chaperones Calnexin and Calreticulin and Impaired by Rapid Dimerization

Joseph Bass^*^,, Gavin Chiu, Yair Argon^||^,¶, and Donald F. Steiner^,

^* The Department of Medicine, The Howard Hughes Medical Institute, The Department of Biochemistry and Molecular Biology, ^|| The Committee on Immunology, and ^¶ The Department of Pathology, The University of Chicago, Chicago, Illinois 60637

Many complex membrane proteins undergo subunit folding andassembly in the ER before transport to the cell surface. Receptorsfor insulin and insulin-like growth factor I, both integralmembrane proteins and members of the family of receptor tyrosine kinases (RTKs), are unusual in that they require homodimerizationbefore export from the ER. To better understand chaperone mechanismsin endogenous membrane protein assembly in living cells, wehave examined the folding, assembly, and transport of the humaninsulin receptor (HIR), a dimeric RTK. Using pulse-chase labelingand nonreducing SDS-PAGE analysis, we have explored the molecularbasis of several sequential maturation steps during receptorbiosynthesis. Under normal growth conditions, newly synthesizedreceptor monomers undergo disulfide bond formation while associatedwith the homologous chaperones calnexin (Cnx) and calreticulin(Crt). An inhibitor of glucose trimming, castanospermine (CST),abolished binding to Cnx/Crt but also unexpectedly acceleratedreceptor homodimerization resulting in misfolded oligomericproreceptors whose processing was delayed and cell surfaceexpression was also decreased by $~$ 30%. Prematurely-dimerizedreceptors were retained in the ER and more avidly associated with the heat shock protein of 70 kD homologue binding protein.In CST-treated cells, receptor misfolding followed disorderedoligomerization. Together, these studies demonstrate a chaperonefunction for Cnx/Crt in HIR folding in vivo and also provideevidence that folding efficiency and homodimerization are counterbalanced.

Abbreviations used in this paper: BFA, brefeldin A; BiP, binding protein; Cnx, calnexin; Crt, calreticulin; CST, castanospermine; DSP, dithiobis (succinimidyl propionate); ECL, enhanced chemiluminescence; endo H, endoglycosidase H; HA, hemagglutinin; HIR, human insulin receptor; Hsp70, heat shock protein of 70 kD; PMSF, phenylmethlsulfonyl fluoride.

THE efficient production of membrane proteins is an essentialfunction of the eukaryotic secretory pathway. One puzzling featureof the folding and assembly of nascent proteins studied to dateis the great diversity in their rates of assembly and transport(Lodish and Kong, 1984; Helenius, 1994). Various studies indicatethat a major rate-limiting event in the delivery of proteinsto the distal secretory pathway is the time required for conformationalmaturation in the ER (Lodish, 1986; Aridor and Balch, 1996).

In the ER, the high concentration of nascent hydrophobic proteins,combined with the oxidative environment, increases the potentialfor aggregation and misfolding compared with conditions in thecytosol (Gething and Sambrook, 1992; Helenius et al., 1992;Hartl, 1996). Ultimately, a complex quality control networkdistinguishes functional oligomeric proteins from their misfoldedcounterparts. In both mammalian cells and in yeast, two majorclasses of ER chaperones are central components of the qualitycontrol network: these are (a) the heat shock protein of 70kD (Hsp70)¹ homologue binding protein (BiP) (Munro and Pelham, 1986),and (b) the calcium-binding proteins calnexin (Cnx) and calreticulin(Crt) (Ou et al., 1993; Bergeron et al., 1994; Krause and Michalak, 1997).

The most detailed understanding of chaperone action in theER has emerged from studies of the immunoglobulin heavy chainBiP. BiP participates in multiple steps during protein maturation,including translocation, formation of tertiary structure, andretrieval of misfolded proteins from the cis-Golgi (Munro and Pelham, 1986;Kozutsumi et al., 1988; Gething and Sambrook, 1992; Hammond and Helenius, 1994a,b;Brodsky et al., 1995; Lyman and Schekman, 1997).

Cnx and Crt have more recently emerged as ER resident chaperonesthat interact with newly synthesized glycoproteins in earlystages of maturation (David et al., 1993; Ou et al., 1993;Hammond and Helenius, 1994a,b; Hammond et al., 1994; Jackson et al., 1994;Pind et al., 1994; Hebert et al., 1996). Mutant- or incompletelyassembled subunits remain associated with calnexin for a prolongedperiod and are retained in the ER before degradation (Loo and Clarke, 1994).The basis for calnexin association with nascent proteins hasbeen extensively investigated both in vivo with histocompatibilitycomplexes and in vitro with viral hemagglutinin (HA) and vesicular stomatitis virus glycoprotein (Hebert et al., 1996; Vassilakos et al., 1996).An unusual feature of calnexin–substrate interactionsthat has emerged from these studies is that calnexin bindspreferentially to N-linked oligosaccharides independent ofsubstrate conformation (Zapun et al., 1997). Moreover, by usinga specific inhibitor of glucosidases I and II in microsomes,Hebert and co-workers (1995) have presented evidence that substrateinteractions are restricted to glycoproteins containing a singleterminal glucose residue at N-linked sites, and that the subsequent effects on substrate folding are facilitated through this interaction.Accumulating evidence suggests that analogous effects mediatein vivo interactions between major histocompatability complex(MHC) class I and Cnx (Vassilakos et al., 1996). These observations,in combination with the observed decrease in formation of correctlyfolded HA trimers and MHC class I molecules in the presenceof castanospermine (CST), a glucosidase inhibitor, suggest that Cnx acts as a chaperone in vivo. Nonetheless, it remainsunclear whether a general chaperone function for Cnx/Crt inendogenous oligomeric protein folding exists and whether Cnxand/or Crt participate in quality control for such proteins.

Here we have analyzed the integrated effects of Cnx, Crt, andBiP on the folding, assembly, and trafficking of the insulinreceptor, an endogenous membrane protein, in living cells.Initially, we followed the folding and trafficking of humaninsulin receptor (HIR) in pulse-chase experiments in heterologouscells expressing wild-type and uncleaved mutant HIR (R732A).We examined the role of disulfide bond formation in receptormaturation and found it to correspond with maximal bindingof HIR monomers to Cnx/Crt in a glycan-dependent interaction. Disrupting maturation of N-linked glycans with CST, whichwas previously shown to reduce cell surface expression of HIR,blocked Cnx/Crt binding, accelerated dimerization, and resultedin ER retention (Arakaki et al., 1987). Together, our resultsindicate that the timing of HIR assembly is pivotal in ensuringhigh efficiency folding and that ER chaperones participatein HIR maturation by promoting folding before assembly.

Materials and Methods

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Abstract
Materials and Methods
Results
Discussion
References

Miscellaneous
Restriction enzymes and other reagents were purchased from Amersham Pharmacia Biotech., Inc. (enhanced chemiluminescence [ECL],Amplify; Piscataway, NJ), Epicentre Technologies Corp. (brefeldinA [BFA]; Madison, WI), Perkin-Elmer Corp. (Foster City, CA),New England Biolabs Inc. (Beverly, MA), Boehringer MannheimBiochemicals (endoglycosidase H [endo H], neuraminidase, andprotease inhibitors; Indianapolis, IN), Pierce Chemical Co.(cross-linkers; Rockford, IL), Wako Bioproducts (digitonin;Richmond, VA), Bio-Rad Laboratories (Hercules, CA), and SigmaChemical Co. (CST; St. Louis, MO). mAb 83-14 was a gift from K. Siddle (Addenbrooke's Hospital, University of Cambridge,Cambridge, UK), anti-BiP, recombinant hamster BiP, and anti-Cnxwere from Stressgen Biotechnologies Corp. (Victoria, BritishColumbia, Canada), anti-Crt was from Affinity Bioreagents (Golden,CO), and anti-insulin receptor β subunit and antiphosphotyrosineantibodies were from Upstate Biotechnology Inc. (Lake Placid,NY). [³⁵S]Cysteine and [³⁵S]methionine (sp act of >1000Ci/mmol) were from Amersham Pharmacia Biotech., Inc.

Cell Lines
Stable cell lines expressing the insulin receptor were preparedas described previously using CHO cells (Yoshimasa et al., 1990;Bass et al., 1996). Cells were grown in mininmum essential(MEM) alpha medium containing 10% heat-inactivated dialyzedfetal calf serum, 1 µM methotrexate, 100 U/ml penicillin,and 100 µg/ml streptomycin at 37°C in 5% CO₂.

Metabolic Labeling and Cross-linking
Cell labeling was performed after $~$ 1 h of preincubation in methionine- and cysteine-free DME containing 0.1% bovine serum albumin,100 U/ml penicillin, and 100 µg/ml streptomycin. Labelingwas then performed by the addition of methionine/cysteine-freemedium containing 75–100 µCi/ml of [³⁵S]cysteineand [³⁵S]methionine (Amersham Pharmacia Biotech., Inc.; 1,000Ci/mmol). After labeling for the times indicated in the figurelegends, medium was removed and then cells were washed oncein PBS or 130 mM NaCl, 20 mM bicine, pH 8.0, on ice. Cell monolayerswere lysed in either Triton X-100 lysis buffer (1% Triton X-100,50 mM Tris-HCl, pH 8.0, 500 mM NaCl, 1 mM CaCl₂), or in gentledetergent buffers containing either digitonin (50 mM bicine,pH 8.0, 40 mM NaCl, 5 mM KCl, 10 mM Na₂MoO₄, 0.2% digitonin)or 2% CHAPS, 200 mM NaCl, and 50 mM Hepes. A protease cocktailcontaining 10 µM PMSF, 5 µg/ml pepstatin, 50 µg/mlleupeptin, and 5 µg/ml aprotinin was included with eachlysis buffer. The alkylating agent N-ethylmaleimide was addedto a final concentration of 5 mM to each lysis buffer when sampleswere analyzed for oxidative folding intermediates. Where indicated,cross-linking was conducted during lysis with or without 100µg/ml DSP dithiobis (succinimidyl propionate) (PierceChemical Co.) on ice for 15–30 min. Cross-linker was inactivated with 10 mM glycine for 10 min on ice, nuclei werepelleted at 14,000 rpm in a bench top microfuge (5415C; EppendorfScientific, Inc., Hamburg, Germany), and then the soluble lysatefraction was processed for immunoprecipitation. For pulse-chaseanalysis, cells were labeled for 15– 30 min, washed inPBS, and then chased with 2 mM of L-cysteine and L-methioninefor the indicated times. CST was used at a final concentration of 1 mM (prepared by dissolving 5 mg with 65 µl 1N HClin a final volume of 265 µl to yield 100 mM). TCA precipitationdid not reveal significant differences in the amount of proteinsynthesized between the CST-treated and control groups.

For tryptic destruction of cell surface receptors, at the designatedtime of chase plates were washed once with PBS and then L-1-tosylamido-2-phenylethylchloromethyl ketone Trypsin (Pierce Chemical Co.) was addedto a final concentration of 0.5 mg/ml in PBS. The plates wereagitated at room temperature for 10 min, the trypsin was aspiratedon ice, and then the cells were rinsed twice with 1.5 mg/mlof trypsin inhibitor (Boehringer Mannheim Biochemicals) inPBS. The floating cells were pelleted in a microfuge (5415C;Eppendorf Scientific, Inc.) and then combined with cell extractsprepared by scraping the corresponding plates on ice into Triton lysis buffer containing aprotinin.

Immunoprecipitation, Gel Electrophoresis, and Immunoblotting
When immunoprecipitation was performed for analysis of receptor–chaperonecomplexes, the cell lysates were first precleared by incubationwith 5 µl of nonimmune rabbit serum and $~$ 50 µl ofprotein A for 1 h or more, microfuged, and then transferredto a new tube. Primary immunoprecipitation was performed withan amount of each antibody determined to yield quantitativeprecipitation. The lysate was combined with protein A–agaroseand then adjusted to a final volume of 600 µl with TNNB(50 mM Tris-HCl, pH 8.0, 250 mM NaCl, 0.5% NP-40, 0.5 mM PMSF,0.1% BSA, and 0.02% NaN₃) before mixing overnight at 4°C.Immune complexes were recovered by brief centrifugation in abench top microfuge (MF6A; Eppendorf Scienfic, Inc.) and thenwashed in TNNB, TNNB without BSA (TNN), and finally in PBSbefore elution in 0.2 M glycine-HCl, pH 2.5. The pH of elutedcomplexes was neutralized with Tris-HCl, pH 8, and then dilutedin concentrated Laemmli sample buffer to yield a final 1x concentration(50 mM Tris-HCl, pH 6.8, 2% SDS, 0.1% bromophenol blue, 10%glycerol, and either 100 mM DDT or 5% β-mercaptoethanolwhere indicated). Redissolved samples were warmed at 50°Cor boiled in reducing agents for 5 min before electrophoresisthrough 5% stacking and 8% running (5/8%) or 3–10% lineargradient SDS-PAGE at 50–70 V for 18–20 h. Afterelectrophoresis, gels were fixed in a solution of 10% aceticacid and 25% isopropanol and then treated with Amplify. For determination of relative molecular mass, 3–10% gelswere stained with Coomassie brilliant blue dye (0.025% Coomassiebrilliant blue R-250, 45% methanol, and 9.2% acetic acid) anddestained in 7.5% acetic acid and 5% methanol. Gels were dried,exposed to XOMAT film (Eastman Kodak Co., Rochester, NY), andthen the fluorograms were analyzed by phosphorimaging the driedgels (model 425E scanner and ImageQuant software, MolecularDynamics, Inc., Sunnyvale, CA).

Immunoblotting was performed after electrophoresis by transferring the proteins from SDS-PAGE to Immobilon P (membrane presoakedfor $~$ 1 min in methanol; Millipore Corp., Waters Chromatography,Milford, MA), in buffer containing 25 mM Tris-HCl, pH 7.4,192 mM glycine, and 20% methanol at 4°C and 14 V for 12–48h. The membranes were soaked in blocking buffer (5% wt/volnonfat dry milk and 0.2% Tween 20 vol/vol in PBS), rinsed in0.2% Tween 20/PBS three times for 10 min each, and then incubatedovernight at 4°C with the primary antibody (or at room temperature for 1 h) while mixing (Scopsi et al., 1995). Themembranes were rinsed again in 0.2% Tween 20/PBS, incubatedwith HRP-linked protein A for 2 h, and then rinsed and developedusing ECL reagents (Amersham Pharmacia Biotech. Inc.).

Glycosidase Digestion
After immunoprecipitation, samples were eluted in 50 mM sodiumcitrate, pH 3.5, and then the pH of the eluates was adjustedto 5.5 (by adding 8 µl of 1.5 M unbuffered sodium citrateto each 150 µl of eluate). Samples digested with endoH (Boehringer Mannheim Biochemicals) were first diluted 1:2with water, adjusted to $~$ 0.1% SDS, and then heated at 95°Cfor 5 min. After cooling, PMSF was added to a final concentrationof 1 mM, endo H was added to give 30 mU/ml, and then the reactionwas incubated at 37°C overnight. The digestion was terminatedby boiling in Laemmli sample buffer. Samples digested withneuraminidase were adjusted, pH 5, with 1.5 M sodium acetate,pH 5.5, and then diluted in H₂O to give a final concentrationof 50 mM sodium acetate. Calcium chloride was added to a finalconcentration of 9 mM and Vibrio cholera neuraminidase (Calbiochem-NovabiochemCorp., La Jolla, CA) was added to a final concentration of 20mU/100 µl; because PMSF inhibits neuraminidase, we didnot add it to these reaction mixtures. Neuraminidase incubationwas at 37°C for 2 h.

Biotinylation
To compare receptor expression levels in control and CST-treatedcells, confluent monolayers of CHO cells overexpressing thewild-type receptor were incubated at 37°C for 72 h withCST, washed in Hank's balanced salt solution, and then incubatedwith 1 mg/ml of sulfo-N-hydroxysulfosuccinimide ester-biotin(#21217; Pierce Chemical Co.) for 30 min on ice. Monolayerswere washed in PBS containing 15 mM glycine and then lysed in Triton X-100 lysis buffer. Receptors were immunoprecipitated,electrophoresed through 5/8% SDS-PAGE, and then transferredto Immobilon membranes (Millipore Corp.) for blotting withstreptavidin-HRP (1:750 dilution; Amersham Pharmacia Biotech.Inc.). ECL was used to visualize the biotinylated receptorsand then bands were quantitated by densitometry (Molecular Dynamics,Inc.). Blots were subsequently stripped and reprobed with anti-HIRβ subunit antibodies (Upstate Biotechnology Inc., LakePlacid, NY).

Tyrosine Phosphorylation
CHO cells were incubated with cysteine/methionine-free DME containing 75–100 µCi/ml of [³⁵S]methionine and [³⁵S]cysteinefor 3–6 h. Cells were then stimulated with the indicatedconcentrations of insulin at 37°C for 5 min, placed onice, and then lysed in Triton X-100 lysis buffer containing phosphatase inhibitors (100 mM NaF, 2 mM sodium orthovanadate,4 mM sodium pyrophosphate). The phosphorylated receptors wererecovered by immunoprecipitation with antiphosphotyrosine antibody(6G9) and processed for SDS-PAGE, fluorography, and phosphorimaging.The Student's t test was used to determine the significanceof differences in receptor autophosphorylation in control andCST-treated cells (Runyon, 1985).

Results

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Abstract
Materials and Methods
Results
Discussion
References

Insulin Receptor Structure and the Identification of the Molecular Basis for Conversion between Four Maturation Intermediates
Fig. 1 shows a linear representation of the extended insulin receptor polypeptide and the structure of the receptor in the cell membrane. The receptor is initially synthesized as a single chain proreceptor that undergoes N-linked glycosylationat 17 consensus sites (Ebina et al., 1985; Ullrich et al., 1985).Before export from the ER, two proreceptor monomers dimerizeand form two symmetric interchain covalent disulfide bonds (cysteines524–524 and 682–682) (Lu and Guidotti, 1996). Aftermaturation of N-linked oligosaccharides and proreceptor proteolyticcleavage by furin or related convertases, as shown by Fullerand Moehring and co-workers (Robertson et al., 1993; Bravo et al., 1994),the receptor is transferred to the plasma membrane as a heterotetramercomposed of two ${alpha}$ and two β subunits with a molecular massof 350–400 kD (Olson et al., 1988).

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Figure 1 Schematic of insulin receptor structure. (A) A linear representation of the insulin receptor precursor protein is shown with functionally important regions highlighted. The proreceptor undergoes N-linked glycosylation at 17 sites and cleavage at the indicated tetrabasic site. (B) The mature cell surface insulin receptor is composed of two ${alpha}$ and two β subunits that are organized into two separate modules: an extracellular domain consisting of the entire ${alpha}$ and part of the β subunits, and an intracellular domain that contains the tyrosine kinase region of the β subunit. The two ${alpha}$ subunits are joined by two symmetric interchain disulfide bonds, indicated with dark lines (cysteines 524–524 and 682– 682). The plasma membrane heterotetramer has a molecular mass of 350–400 kD.

To monitor insulin receptor folding and transport we performedpulse-chase experiments in CHO cell lines transfected withfull-length wild-type receptors (Figs. 1 and 2). Gel electrophoresiswas performed under both reducing and nonreducing conditionsto follow HIR maturation. After a 30-min pulse, two specieswere seen, migrating at $~$ 200 and $~$ 220 kD, respectively. With shorterpulse times, the faster migrating band (Fig. 2, early monomer, EM) appeared first, with radioactivity progressively chasinginto the second slower migrating band (Fig. 2, late monomer,LM).

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Figure 2 Biosynthesis of the wild-type insulin receptor. (A) Stable CHO cells expressing the wild-type insulin receptor were pulse labeled for 30 min with [³⁵S]methionine and [³⁵S]cysteine (50 µCi/ml), washed with PBS, and then chased in medium containing 2 mM each of methionine and cysteine. Cell extracts were prepared at the indicated times, immunoprecipitated, redissolved in Laemmli sample buffer containing DTT, and then electrophoresed through 5/8% SDS-PAGE. The positions of the receptor subunits are indicated with arrows to the left, and two of the molecular weight markers are indicated with arrows to the right (EM, early monomer; LM, late monomer; D, dimer; T, tetramer). (B) Cells were pulse labeled for 35 min, chased, and then processed under nonreducing conditions by 3–10% linear gradient SDS-PAGE. The position of receptor complexes are indicated with arrows to the left and molecular mass markers are indicated to the right. (C) CHO cells were pulse-labeled with [³⁵S]methionine and [³⁵S]cysteine for 15 min in the presence (lanes 2 and 4) or absence (lanes 1 and 3) of 5 mM DTT. Cell extracts were immunoprecipitated with anti-HIR antibodies, redissolved in Laemmli sample buffer with (lanes 1 and 2) and without 10 mM DTT (lanes 3 and 4) and then analyzed by nonreducing 3–10% SDS-PAGE.

To determine whether these species represented distinct oxidativeintermediates, we followed receptor biosynthesis when the redoxenvironment of the ER was manipulated with the membrane-permeantreducing agent DTT. When the pulse was performed in the presenceof 5 mM DTT, the first monomer band to appear migrated to aposition slightly above that of the early monomer in untreatedcells (Fig. 2 C, lane 4). This intermediate form of the monomericreceptor, which we term "misfolded monomer" (Fig. 2 C, lane4), failed to progress to a second slower-migrating electrophoreticspecies. When receptor monomers from both DTT-treated and untreatedcells were heated in Laemmli gel buffer with reducing agentbefore electrophoresis, both migrated to the same position(Fig. 2 C, compare lanes 1 and 2 with lane 3). The fully reduced monomer (Fig. 2 C, lanes 1 and 2) migrated slightly slower than the nonreduced monomer on the same gel (Fig. 2 C, lane3). Since both the early and late monomers appeared as a singleband after reduction (Fig. 2 C, lane 1), we conclude that theydiffer only in the number and/or arrangement of intramoleculardisulfide bonds. Taken together, this suggests that disulfidebond formation occurs rapidly and that the early and late monomersrepresent two distinct oxidative intermediates of the proreceptor.

After 60 min of chase, a third band of twice the molecular mass( $~$ 380 kD) was observed by nonreducing gel electrophoresis. Shortlythereafter, a fourth species appeared ( $~$ 420 kD), concomitantwith movement of the receptor from ER to trans-Golgi (Olson et al., 1988).The 380-kD band material was sensitive to digestion with endoH, consistent with its localization in a pre–trans-Golgicompartment (data not shown). Acquisition of both endo H resistanceand neuraminidase sensitivity coincided with the appearanceof the 420-kD species (Fig. 3 A), suggesting that this wasthe mature form of the receptor in the most distal compartmentof the secretory pathway.

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Figure 3 Intracellular movement of the receptor based on endoglycosidase sensitivity and gel shifts. (A) CHO cells expressing wild-type receptors were pulse labeled for 30 min and then extracts were prepared after 6 h of chase. Immunoprecipitated receptors were eluted from protein A–agarose in 50 mM sodium citrate, pH 3.5, and incubated with buffer alone (lane 1), neuraminidase (NE, lane 2), or endo H (Endo H, lane 3). The position of receptor complexes are shown with arrows to the left (D, dimer; T, tetramer). (B) Pulse-chase labeling was performed with CHO cells expressing uncleaved mutant proreceptors containing a substitution in the tetrabasic cleavage site (Arg732Ala). Cells were pulse labeled for 30 min, chased, and then analyzed under reducing conditions by 5/8% SDS-PAGE (proHIR I, first proreceptor with high-mannose oligosaccharides; proHIR II, second proreceptor species containing complex oligosaccharides added in the Golgi). (C) CHO cells expressing the R732A mutant receptors were pulse labeled for 15 min, chased, and then analyzed by nonreducing 3–10% linear gradient SDS-PAGE. Folding intermediates and receptor subunits are indicated with arrows to the left and molecular weight markers are indicated to the right (EM, early monomer; LM, late monomer; D, proHIR I dimer; T, dimer species after addition of complex oligosaccharides, for simplicity this is labeled using the same nomenclature as that of the wild-type receptor, i.e., the tetramer).

According to a previous model of insulin receptor biosynthesisproposed by Olson and Lane (1987), the mobility changes describedabove were ascribed to cleavage of the proreceptor dimer into ${alpha}$ and β subunits, possibly reflecting tertiary structuralchanges associated with proteolytic processing (D to T transition;Olson et al., 1988). To examine whether proteolytic cleavagecauses these changes in mobility, we studied the biosynthesisof the R732A mutant proreceptor, which is not cleaved. Sucha mutant insulin receptor gene was previously identified ina patient with insulin-resistant diabetes (Yoshimasa et al., 1988,1990). Surprisingly, despite the lack of proteolytic processingof the R732A proreceptor, the mutant still underwent the samemobility shifts (Fig. 3 C). These results suggest that latechanges in the electrophoretic mobility of the receptor aredue to processing of carbohydrate chains, reflecting movementof the receptor into the trans-Golgi (Kornfeld and Kornfeld, 1985),rather than proteolytic cleavage.

Conversion between Early and Late Monomers Involves Interaction with ER Lectin Chaperones Cnx and Crt
To determine whether subunit maturation is facilitated by ERmolecular chaperones, we next sought to identify chaperonemolecules that associate with newly synthesized receptors. Detergentlysis and chemical cross-linking conditions were optimizedto retain associations between newly synthesized receptorsand ER resident chaperones. After metabolic labeling and immunoprecipitationwith antireceptor antibodies, several coprecipitating proteins were found (Fig. 4 A). In addition to the major bands representingthe proreceptor and the ${alpha}$ and β subunits, two bands wereobserved migrating faster than the position of the 97-kD βsubunit, at $~$ 80 and 90 kD (Fig. 4 A, lanes 3 and 4). These bandswere identified as BiP and Cnx, respectively, using specificantibodies (Fig. 4 A, lanes 2–4). No other major bandswere reproducibly found.

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Figure 4 Isolation of ternary BiP–Cnx–HIR complexes. (A) CHO cells overexpressing wild-type receptors were labeled overnight with [³⁵S]methionine and [³⁵S]cysteine 50 µCi/ml and then lysed in 0.4% digitonin with DSP. Samples in lanes 1–3 were from the same experiment, and the lysate was divided equally, immunoprecipitated, and then processed for 5/8% SDS-PAGE (lane 1, ${alpha}$ NRS [normal rabbit serum]; lane 2, ${alpha}$ BiP; lane 3, ${alpha}$ Cnx; lane 4, ${alpha}$ HIR). The positions of BiP (+), Cnx (**), and the β subunit (*) are indicated to the left in lanes 2–4. A separate analysis from another experiment is shown in lane 4 to more clearly delineate the receptor and chaperone bands; a similar pattern was obtained by immunoprecipitation of the sample shown in lanes 1–3. The positions of receptor subunits, Cnx and BiP are indicated with arrows. (Lanes 5–10) Cells were labeled as in lanes 1–4, and lysis was performed without (lanes 5–7) or with (lanes 8–10) 10 mM ATP. (B) Equivalent amounts of cell lysate protein from CHO cell lines were immunoprecipitated with anti-HIR antibodies, electrophoresed under reducing conditions through 5/8% SDS-PAGE, transferred to immobilon membranes, immunoblotted with anti-BiP antibody, and then developed with ECL reagents (lane 1, recombinant BiP; lanes 2 and 3, cells expressing wild-type receptors) (Bass et al., 1996).

Three criteria were used to establish that the $~$ 80-kD band wasBiP. First, sequential immunoprecipitation with antireceptorantibodies followed by immunoblotting with anti-BiP antibodies,showed BiP immunoreactivity of the $~$ 80-kD band (Fig. 4 B). Second,the $~$ 80-kD band comigrated with recombinant hamster BiP as demonstratedby silver staining the gels (data not shown). Finally, celllysis in the presence of 10 mM ATP dissociated BiP–receptor complexes (Fig. 4 A, compare lane 7 with lane 10). Complexesbetween HIR and BiP were most stable when lysis was performedin the presence of the cross-linking agent DSP (see Fig. 11C, lanes 4 and 5), although ATP-sensitive association withBiP was also detectable by Western blot in the absence of cross-linkingagent (Fig. 4 B, lanes 2 and 3). We found that the anti-BiPantibody reacted only poorly in immunoprecipitation reactionsexplaining the consistently lower amount of HIR recovered inanti-BiP precipitates (Fig. 4). However, this antibody, whichwas raised to a synthetic COOH-terminal peptide, reacted well by immunoblotting (Stressgen anti-Grp 78; Fig. 4 B).

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Figure 11 Maturation model. Temporal sequence of ER folding of the insulin receptor showing synchronization of maturation and chaperone binding. The diagram illustrates that Cnx/Crt bind in complexes to newly synthesized proreceptor monomers (EM, early monomer) and that conversion to a second oxidative intermediate (S–S) occurs during binding to chaperones (LM, late monomer). Post-ER maturation involves proteolytic cleavage and addition of carbohydrate capping sugars to Asn-linked oligosaccharide chains. Addition of carbohydrates results in mobility shifts on nonreducing SDS-PAGE, whereas proteolytic cleavage does not alter the tertiary or quaternary structure of the receptor as detected by nonreducing SDS-PAGE. The dual pathways of maturation involve either Cnx/Crt and BiP (top route) with dimerization occurring at $~$ 75 min posttranslationally, whereas a second pathway occurs when Cnx/Crt are bypassed with rapid dimerization within $~$ 10 min posttranslationally.

The identity of the $~$ 90-kD band was confirmed by coimmunoprecipitationwith anti-Cnx antibodies that coprecipitated both Cnx and theinsulin proreceptor. The observation that anti-Cnx antibodiesselectively coprecipitated the proreceptor and not the cleaved ${alpha}$ or β subunits is consistent with an association betweencalnexin and the receptor in the early secretory pathway beforecleavage into these subunits (Fig. 4 A, compare lanes 3 and4). Furthermore, inhibition of glucose trimming by preincubating cells with CST before lysis, a manipulation that has been shown to disrupt the carbohydrate binding site for Cnx, ledto dissociation of Cnx–proreceptor complexes (Fig. 5 A). Similarly, complexes between the insulin receptor and Crt, a second ER lectin chaperone, were also demonstrated by coimmunoprecipitationwith anti-Crt antibodies (Fig. 5 B). Although it is possiblethat CST effects an intermediate glycoprotein or another ERchaperone required for Cnx/ Crt–HIR binding, it is clearthat Cnx/Crt–HIR complexes were dissociated after CSTtreatment. Proreceptors isolated from cells treated with CSTmigrated more slowly on SDS-PAGE, consistent with the presenceof additional glucose moieties attached to the 17 N-linkedcarbohydrate side chains present in the ectodomain; this alsoprovided an independent confirmation that CST was effectivein blocking glucose trimming (Fig. 5, A and B, ${alpha}$ HIR). Together,the results suggest that the coprecipitation of the proreceptorby anti-Cnx antibodies is due to specific chaperone–receptorinteractions.

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Figure 5 Subunit specificity of Cnx and Crt. CHO cells expressing the wild-type insulin receptor were incubated overnight in the presence or absence of 1 mM CST (A, lanes 1–3, B, lanes 1 and 2). (A) Cells were labeled for 6 h, lysed in digitonin lysis buffer containing DSP, immunoprecipitated with the indicated antibodies, and then processed for 5/8% SDS-PAGE using β-mercaptoethanol as the reducing agent (ME). (B) Cells were labeled for 5 h, lysed in CHAPS lysis buffer without cross-linking, and then processed for 5/8% SDS-PAGE as in A. The positions of the proreceptor, Cnx, and Crt are indicated with arrows to the left. Note that the receptor β subunit has a molecular mass of $~$ 95 kD and migrates close to the position of Cnx, which has a molecular mass of $~$ 90 kD (A, lanes 3 and 6). (C) Cells were pulse labeled for 30 min and then lysed in digitonin buffer after a 30-min chase (lanes 1–4). Equivalent aliquots of lysate were processed for immunoprecipitation with nonimmune serum (lanes 1 and 4), anti-Cnx (lane 3), and anti-Crt (lane 4), and one-third of this amount was processed for immunoprecipitation with anti-HIR (lane 2). Immunoprecipitated protein was analyzed under nonreducing conditions by 3–10% SDS-PAGE. The positions of the early monomer (EM), late monomer (LM), and dimer are indicated with arrows.

To identify whether Cnx and Crt associate with both the monomericand dimeric receptors, or only a subset of receptors, Cnx–HIRcomplexes were analyzed by nonreducing SDS-PAGE. Because ofvariable recovery with different bleeds of the Cnx and Crt immuneserum, and because both antibodies precipitated less proHIRthan antireceptor antibodies, we used more total cell lysatefor immunoprecipitation with Cnx/Crt antibodies than HIR antibodies.Furthermore, we found that the anti-Crt antibody consistentlyrecovered more HIR than comparable amounts of anti-Cnx antibodies(Fig. 5 C, lanes 3 and 4). The relatively greater quantitativeyields with the anti-Crt versus anti-Cnx antibodies have alsobeen observed in fibroblast cultures (Green, W.N., personalcommunication). An additional high molecular weight band thatwas present after precipitation with anti-Crt antibodies appearedto migrate close to the position of the dimeric receptor species;however, this band was not precipitated with antireceptor antibodies(Fig. 5 C, lanes 2 and 4). Additional experiments performedat later chase times failed to show association between dimericreceptors and Cnx/Crt, and recent sucrose gradient analysisconfirms that association of Cnx is restricted to monomericforms of the receptor (data not shown). Since dimeric receptorstypically convert to the tetramer after a brief lag period,it is likely that release from Cnx/Crt occurs before dimerizationand export from the ER (refer to Fig. 2).

Delayed ER Export and Accelerated Dimerization Occur When Binding to Lectin Chaperones Is Blocked
To analyze the effects of Cnx and Crt on receptor maturation,we performed pulse-chase studies after incubation with CST.In CST-treated cells, there was a consistent delay in the processingof the proreceptor into ${alpha}$ and β subunits at late chase timepoints (Fig. 6). However, no significant difference in recoveryof total ³⁵S-labeled receptor was detected at time points upto 7 h of chase, suggesting that the delay in cleavage didnot result in accelerated receptor degradation at these timepoints (data not shown). Since proteolytic cleavage of theproreceptor has been localized to the trans-Golgi apparatus(Molloy et al., 1994), unprocessed proreceptors must have accumulatedin a pre-TGN compartment after CST treatment. The half-life of the total processed ( ${alpha}$ and β subunits) and unprocessed proreceptor in both CST-treated and untreated groups was $~$ 10h (Fig. 6). These values are in agreement with previous measurementsby both Kahn and Lane and co-workers (Kasuga et al., 1981; Ronnett et al., 1983).Although these results suggest that the overall turnover rate of proHIR, ${alpha}$ and β subunits was unchanged after CST treatment,it is possible that unprocessed proreceptors in CST-treatedcells are retained in the ER and degraded rather than transportedto the cell surface.

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Figure 6 Receptor turnover in CST-treated and untreated cells. CHO cells were treated with CST or in labeling medium alone in the presence of [³⁵S]methionine and [³⁵S]cysteine. The plates were then washed and chased in medium containing excess methionine and cysteine. Cell extracts were prepared at the indicated times in Triton X-100 lysis buffer, immunoprecipitated with ${alpha}$ HIR antibodies, redissolved in Laemmli sample buffer containing DTT, and then electrophoresed through 5/8% SDS-PAGE. A fluorogram from a representative experiment is shown. Receptor subunits are indicated with arrows to the left.

The lack of binding to lectin chaperones after CST treatmentsuggested that retention of the dimeric pool of receptors inthe treated group occurred through a calnexin-independent mechanism.To examine whether the retained receptors in CST-treated cellswere associated more avidly with BiP, we performed immunoblottingwith anti-BiP antibodies after immunoprecipitation with anti-HIRantibodies. Fig. 7 shows two- to threefold increases in theamount of BiP associated with the receptor in CST-treated comparedto control cells. This suggests that BiP is involved in retainingproreceptor molecules, which accumulate after blockade of bindingto the lectin chaperones.

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Figure 7 Effect of CST treatment on BiP–HIR association. CST-treated and control CHO cells expressing the wild-type receptor were prepared as described in Fig. 6 except lysis was performed in CHAPS buffer. Cell lysate protein was measured using the Bio-Rad DC protein reagent and equivalent amounts of lysate protein were immunoprecipitated with anti-HIR antibodies, followed by reducing gel electrophoresis and immunoblotting with anti-HIR (top) and anti-BiP (bottom) antibodies. Samples shown in both upper and lower panels are as follows: 5 µg of recombinant BiP (lane 1), anti-HIR immunoprecipitated lysate from control cells (lane 2), and from CST-treated cells (lane 3).

Surprisingly, analysis of receptor biosynthesis after CST treatmenton nonreducing gels showed that conversion from the early monomerto the late monomer and dimerization were all greatly acceleratedafter CST treatment (Fig. 8 A). Accelerated formation of earlyand late monomers is more clearly observed in the fluorogramshown in Fig. 8 B. However, it is possible that the early andlate monomers detected after CST treatment have subtle structuralabnormalities compared to wild-type receptors; such structuraldifferences might not be detected on SDS-PAGE analysis. Theincreased rate of receptor dimerization in CST-treated cellsis clearly noted when the phosphorimaging data from two separatepulse-chase experiments was represented by a histogram (Fig.8 D). Earlier dimerization in CST-treated cells was reproduciblyfound in five additional experiments performed with variedpulse times (data not shown). To test whether dimeric receptorsproduced in the presence of CST progressed more rapidly to the cell surface, we incubated cells at varying time points with trypsin, which specifically releases only the cell surfacereceptors (Shoelson et al., 1988). Transport of these receptorsto the cell surface was demonstrated by the trypsin sensitivityof receptors from treated and untreated cells (Fig. 8 C). Moreover,trypsin-sensitive receptors were found at earlier times inCST-treated cells, and proteolytic cleavage of a subset ofproreceptors into ${alpha}$ and β subunits was similarly detectedat an earlier time point (comparing ${alpha}$ and β subunits visibleat a 1 h time point in CST-treated versus untreated cells,data not shown). Based on insulin cross-linking studies, wefound that all of the receptors present on the cell surfacewere, in fact, processed into ${alpha}$ and β subunits since insulinwas only detected bound to the ${alpha}$ subunit and not to the proreceptor(data not shown). However, despite the rapid dimerization andtransport to the cell surface of a subset of newly synthesizedreceptors, a fraction of the dimeric pool of receptors remaineduncleaved and were retained in a pre-TGN compartment (Fig.6).

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Figure 8 Kinetics of proreceptor folding after CST treatment. (A) Cells were pulse-labeled for 30 min in [³⁵S]methionine and [³⁵S]cysteine (100 µCi/ml) and then chased for the indicated times. The positions of the intermediates are indicated with arrowheads (EM, early monomer; LM, late monomer; D, dimer; T, tetramer). The conversion from dimer to tetramer species in CST-treated cells was obscured due to the higher molecular weight associated with excess untrimmed glucose residues attached to the Asn-linked saccharide chains. Samples were analyzed under nonreducing conditions on 3–10% linear gradient SDS-PAGE. (B) Cst-treated and control cells were pulse labeled for various times and then analyzed as in A. EM and LM, the only species present in untreated cells at these early time points, are indicated with arrows. (C) Cst-treated and control cells were pulse labeled for 20 min, chased for 2 h, and then incubated for 10 min at 25°C in the presence of trypsin (0.5 mg/ml) to release cell-surface receptors before processing as described for Fig. 2. The highest molecular mass species (T) in both Cst-treated and control groups was trypsin sensitive, whereas the lower molecular mass species (D) remained trypsin resistant. (D) Histogram representing the rate of dimerization of receptors in Cst-treated versus control cells. Phosphorimaging data from two experiments with 30-min pulse times was compiled and expressed as the percentage of total radioactivity present at each time point as the dimer.

Functional Receptors Are Delivered to the Cell Surface in CST-treated Cells
To assess levels and function of cell surface receptors in CST-treated and control cells, both biotinylation and insulin-stimulatedtyrosine autophosphorylation were used. Fig. 9 A shows thatcell surface biotinylation of receptors was decreased ( $~$ 30%when three separate experiments were compared) in CST-treatedcells, whereas steady-state levels of the proreceptor wereincreased (Fig. 9 B). Total cellular levels of processed βsubunit were also decreased at steady state (Fig. 9 B). Thedecreased level of the β subunit is consistent with theretention and/or degradation of CST-treated receptors in anunprocessed form in the early secretory pathway.

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Figure 9 Biotinylation of cells treated with Cst. (A) Cell surface receptors were biotinylated after a 72-h incubation with Cst. Cells were solubilized in Triton lysis buffer and then processed for immunoprecipitation with anti-HIR antibodies and analysis by reducing 5/8% SDS-PAGE. Biotinylation was detected after transfer of the proteins to Immobilon P using streptavidin–HRP and ECL (Amersham Pharmacia Biotech. Inc.). (B) Blots were stripped and reprobed with anti-HIR β subunit antibodies. Receptor subunits and the position of molecular weight markers are indicated with arrows.

To measure the ability of the bound hormone to transmit a signalto the intracellular domain of the receptor, we compared insulin-stimulatedtyrosine phosphorylation of the receptor in CST-treated andcontrol groups. Fig. 10 shows that insulin-responsive autophosphorylation,measured by recovery of prelabeled receptor protein after briefincubation with insulin, was equivalent in control and CST-treatedgroups. Together, the results show that steady- state levelsof processed and cell surface receptors were decreased afterCST treatment, although receptors delivered to the cell surfacewere fully responsive to hormone. The correct folding of amajority of receptors in the presence of CST suggests that lectin-basedinteractions are not essential; rather, they enhance or facilitatefolding.

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Figure 10 Insulin-induced receptor autophosphorylation in cells treated with CST. (A) Cells were incubated overnight in 1 mM CST and labeled with [³⁵S]cysteine and [³⁵S]methionine (75 µCi/ml of each) for 5 h. The cells were then stimulated with insulin for 5 min at 37°C (0–100 nM), washed in PBS, lysed in Triton buffer containing phosphatase inhibitors and equivalent amounts of lysate were processed for immunoprecipitation either with anti-HIR or antiphosphotyrosine antibodies. (B) Histogram showing the relative percentage of tyrosine-phosphorylated receptors recovered after stimulation with 100 nM insulin in CST-treated versus control cells. No significant difference was found comparing the two groups (mean ± standard error, n = 3; data from three separate experiments).

	Discussion

Top Abstract Materials and Methods Results Discussion References

Recently, a number of studies have demonstrated that both lectinchaperones and the Hsp70 homologue BiP mediate the folding andassembly of oligomeric membrane proteins (Hammond and Helenius, 1994a,b;Williams and Watts, 1995). In vitro studies have shown thatCST treatment of canine microsomes accelerates the oligomerizationof HA, an exogenous viral protein (Hebert et al., 1996). Thepresent studies establish a new model system to investigatethe role of individual chaperone molecules in endogenous membraneprotein folding in living cells. This model is based on experimentsthat define in more detail the molecular basis for individualmaturation steps in insulin receptor biosynthesis. The resultsfurther provide evidence that N-linked glycosylation, and interactionwith Cnx and Crt, delays dimerization and facilitates foldingto a transport-competent conformation analogous to the effectswith HA (Hebert et al., 1996). Because CST directly affectsglucose trimming from N-linked glycans in HIR, it is possiblethat misfolding is due to disrupted carbohydrate maturationper se. Overall, we found that the integrated effects of N-linkedglycosylation and chaperone binding regulate the productionof functional insulin receptors and influences the rate at whichindividual subunits assemble into homodimers.

The prolonged period that elapses before dimerization exposesthe nascent proreceptor to the aqueous oxidizing environmentof the ER. However, under normal growth conditions, biosynthesisis highly efficient and more than 90% of newly synthesizedreceptors were delivered to the cell surface (refer Fig 2).Interaction with Cnx and Crt might provide protection of exposedhydrophobic domains, preventing their misfolding and aggregation.Association with either Cnx or Crt could create steric hindrance,possibly by interacting with a surface that later becomes inaccessiblein the dimer. This might provide sufficient time for partiallyfolded forms to undergo refolding and attain their native conformation(Hebert et al., 1996; Vassilakos et al., 1996).

The delayed movement of a subset of proreceptors to the trans-Golgiafter treatment of cells with CST suggests that these receptorswere misfolded (refer to Figs. 6 and 7). ER retention of thesedimeric receptors was independent of Cnx and Crt based on coprecipitationassays (refer to Fig. 5). The persistence of BiP–receptorcomplexes after CST treatment could explain the retention ofthese receptor dimers. BiP might additionally protect the retained receptors and promote their eventual resolubilization. Sincegrowth factor receptors have been shown to be important forsurvival of mammalian cells in culture, calnexin- independentproduction of insulin receptors might account for the continuedviability of CST-treated cells (Figs. 9 and 10; Arakaki et al., 1987;Baserga, 1994; Rubini et al., 1997). In addition to BiP, analternative ER retention mechanism for prematurely dimericreceptors might be the presence of free thiols that flag suchmolecules and promote their arrest (Isidoro et al., 1996).

Fig. 11 illustrates a model in which two competing reactionsexist in a hierarchy during receptor biosynthesis. Under normalgrowth conditions, the first reaction, in which monomeric receptorhalves associate with Cnx and Crt, predominates. This leadsto slow but highly efficient production of functional receptors.In the second competing reaction, shown as the lower pathwayin Fig. 11, dimerization is much more rapid (<25 min), afterblockade of N-linked glycosylation. Rapid dimerization leadsto less overall efficient maturation and retention of dimericor aggregated receptors in the ER. In this default pathway, binding to BiP is preserved, perhaps protecting the retainedreceptors until they achieve a transport-competent conformation.

In conclusion, these studies have shown that lectin chaperonesdirectly associate with newly synthesized insulin receptorsduring disulfide bond formation and isomerization, whereas blockadeof glucose trimming dissociates Cnx/Crt–HIR complexesand corresponds with accelerated dimerization and delayed maturation.Experiments with CST suggest that folding to a transport-competent conformation requires a posttranslational delay in homodimerization.Two possible mechanisms could account for the effects of Cnx/Crton receptor folding: (a) Cnx/Crt could either simply facilitatefolding to a dimerization-competent conformation, or (b) theycould directly mediate the dimerization reaction. The developmentof an in vivo system to examine Cnx/Crt and BiP interactionswith a membrane protein provides further opportunity to study how these interactions mediate the ER retention of misfoldedreceptors in cases of diabetes caused by mutations in the receptorgene. Additionally, these interactions might be important duringembryogenesis (e.g., insulin growth factor [IGF]-I receptor)or during differentiation from fibroblast to adipocyte (e.g.,insulin receptor) when rapid increases in receptor synthesisare required. Studies are in progress with mutant forms ofHIR in recombinant cells to further examine the basis of Cnx/Crtassociation with HIR, to determine the mechanisms of HIR retention and degradation, and to search for possible additional ER proteins that might be involved in this process.

Acknowledgments

We thank B. Green for helpful discussions, M. Milewski for technicalassistance, W. Chutkow for graphics, S. Duguay and B. Glickfor comments on the manuscript, and R. Ricks (all six fromUniversity of Chicago, Chicago, IL) for assistance in preparationof the manuscript.

This work was supported by the Howard Hughes Medical Instituteand in part by National Institutes of Health grants (DK 13914and DK20595).

Submitted: 10 November 1997

Revised: 4 March 1998

Address all correspondence to Joe Bass, The University of Chicago, Howard Hughes Medical Institute, 5841 South Maryland Ave.,MC 1028, Chicago, IL 60637. Tel.: (773) 702-1328. Fax: (773)702-4292. E-mail: jbass{at}midway.uchicago.edu

References

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Abstract
Materials and Methods
Results
Discussion
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