ADP-Ribosylation Factor 6 Delineates Separate Pathways Used by Endothelin 1 and Insulin for Stimulating Glucose Uptake in 3T3-L1 Adipocytes

doi:10.1128/MCB.21.15.5276-5285.2001

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Molecular and Cellular Biology, August 2001, p. 5276-5285, Vol. 21, No. 15
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.15.5276-5285.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

ADP-Ribosylation Factor 6 Delineates Separate Pathways Used by Endothelin 1 and Insulin for Stimulating Glucose Uptake in 3T3-L1 Adipocytes

J. Todd R. Lawrence and Morris J. Birnbaum^*

Department of Medicine, Howard Hughes Medical Institute, The Cox Institute, University of Pennsylvania School of Medicine, Philadelphia, Pennsylvania 19104

Received 11 December 2000/Returned for modification 8 February 2001/Accepted 30 April 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

In 3T3-L1 adipocytes, both insulin and endothelin 1 stimulate glucose transport via translocation of the GLUT4 glucose carrierfrom an intracellular compartment to the cell surface. Yet itremains uncertain as to whether both hormones utilize identicalpathways and to what extent each depends on the heterotrimericG protein G $alpha$ q as an intermediary signaling molecule. In this study,we used a novel inducible system to rapidly and synchronouslyactivate expression of a dominant inhibitory form of ADP-ribosylationfactor 6, ARF6(T27N), in 3T3-L1 adipocytes and assessed its effectson insulin- and endothelin-stimulated hexose uptake. Expressionof ARF6(T27N) in 3T3-L1 adipocytes was without effect on the abilityof insulin to stimulate either 2-deoxyglucose uptake or the translocationof GLUT4 or GLUT1 to the plasma membrane. However, the same ARF6inhibitory mutant blocked the stimulation of hexose uptake andGLUT4 translocation in response to either endothelin 1 or an activatedform of G $alpha$ q, G $alpha$ q(Q209L). These results suggest that endothelinstimulates glucose transport through a pathway that is distinctfrom that utilized by insulin but is likely to depend on botha heterotrimeric G protein from the Gq family and the small Gprotein ARF6. These data are consistent with the interpretationthat endothelin and insulin stimulate functionally different poolsof glucose transporters to be redistributed to the plasmamembrane.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

In recent years, it has been appreciated increasingly that a ubiquitous mechanism for controlling cellular transport functionsis by altering the subcellular distribution of highly specificcarrier proteins. A prototype for such processes has been theinsulin-dependent activation of glucose transport, in which asequestered intracellular pool of GLUT4, a specialized hormoneresponse sugar transporter isoform, is rapidly translocated tothe cell surface (4). Despite considerable investigation, theprecise intracellular pathways trafficked by GLUT4 as well asthe key regulatory mechanisms have proven refractory to a detailedunderstanding. Nonetheless, it is clear that exocytosis of GLUT4represents the major insulin-regulated event and that transporterscontinue to recycle in the presence of insulin (31). Moreover,the signaling pathway initiated by insulin appears to depend onthe activity of phosphatidylinositol (PI) 3-kinase to elicit increasesin hexose uptake as well as to modulate other metabolic processes(11). Given this information, much attention has focused ontrafficking events recognized as dependent on or influenced bythe abundance of phosphatidylinositides (9, 11).

ADP-ribosylation factor 6 (ARF6) is a small GTP-binding protein remarkable for its ability to influence both vesicular traffickingand actin cytoskeletal remodeling in mammalian cells. Initiallyimplicated in the regulation of the endocytic pathway, more recentdata have demonstrated a role for ARF6 in regulated secretion;moreover, ARF6 appears to play a role in a recycling pathway inwhich membrane from an endosomal-like compartment is translocatedto the cell surface (7, 8, 14, 15, 18, 32, 34).However, it remains unclear whether the intracellular structureto which ARF6 localizes and which cycles to the plasma membranerepresents a subpopulation of endosomes or a novel compartment(34). As with other members of the Ras superfamily, ARF6 isactivated by a guanine nucleotide exchange factor that releasesthe GDP from the inactive protein, allowing GTP to bind and convertARF6 to its activated form (29). While the relevant in vivoexchange factors for ARF6 remain uncertain, ARF6 activity appearsto be regulated by PI 3-kinase. A class of PI-3,4,5-trisphosphate-dependentexchange proteins demonstrate activity for ARF6 in vitro and,in some cases, colocalize with ARF6 in vivo (reviewed in references10 and 12). Thus, given that both PI 3-kinase and ARF6 havebeen shown to regulate vesicular trafficking at the plasma membrane,it has been proposed that PI 3-kinase regulates vesicular traffickingby controlling the activation state of ARF6 (10). Such a modelhas also proven attractive in regard to insulin-regulated glucoseuptake. Results of peptide inhibition studies using permeabilizedcells have suggested that in 3T3-L1 adipocytes, ARF6 may be involvedin the insulin-stimulated translocation of GLUT4 vesicles to theplasma membrane (27). However, subsequent experiments using3T3-L1 adipocytes expressing a GTP-binding-deficient mutant ofARF6 were unable to establish such a role for the G protein (42).In contrast, ARF6 was found to regulate the insulin-stimulatedsecretion of adipsin from 3T3-L1 adipocytes (42).

It has been reported recently that growth factors acting through the heterotrimeric G protein Gq promote the translocationof an ARF6-containing vesicular compartment to the cell surface(6). In 3T3-L1 adipocytes, stimulation of an analogous pathwayresults in translocation of GLUT4-containing vesicles to the plasmamembrane, thus increasing glucose uptake (22-24, 41). Specifically,endothelin 1 stimulates glucose transport through the type A endothelin,G-protein-coupled receptor via a mechanism that depends on activationof a member of the Gq family of heterotrimeric G proteins. Inthe accompanying article, Bose et al. present evidence that theG $alpha$ 11 isoform may be the physiologically relevant isoform in adipocytes(5). In some studies, the ability of G $alpha$ q/11 to stimulate GLUT4translocation has been dependent on p110 $alpha$ , the catalytic subunitof PI 3-kinase (22). Since insulin-stimulated GLUT4 translocationis also dependent on the activation of p110 $alpha$ , it has been suggestedthat the endothelin and insulin signaling pathways converge atPI 3-kinase and use a common mechanism to accelerate glucose transport(20, 22). However, since others have not been able to demonstratea role for PI 3-kinase in mediating GLUT4 translocation followingendothelin stimulation, the endothelin pathway downstream of aGq family member remains unclear (5, 24, 41). Moreover,G $alpha$ q/11 has been proposed to be of general importance in signalingto glucose transport, participating as a necessary factor in theregulation of this process by insulin as well as receptors whichcouple to heterotrimeric G proteins in a classical manner (23,24). However, it still remains possible that insulin and endothelinactivate glucose transport by distinct mechanisms, with only thelatter mediated by G $alpha$ q. Thus, in an effort to better understandthe downstream events leading to alterations in membrane proteintrafficking in 3T3-L1 adipocytes, we have assessed the role ofthe small G protein ARF6 in the regulation of glucose uptake byendothelin and insulin. To accomplish this, we developed a novelinducible system that allows for the efficient and synchronousexpression of genes in terminally differentiated 3T3-L1 adipocytes.We have used this system to confer expression of a dominant inhibitoryconstruct of ARF6, ARF6(T27N), in these cells. We show that endothelin-but not insulin-stimulated increases in hexose uptake and GLUT4translocation are dependent on ARF6, thus functionally distinguishingthe pathways through which each of the stimuli increase glucoseuptake.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Virus and general reagents. The recombinant adenovirus expressing Cre recombinase (AdCre) was a generous gift from Frank L. Graham, McMaster University(Hamilton, Ontario, Canada) (3). The GTPase-deficient, activatedG $alpha$ q(Q209L) mutant recombinant adenovirus was a generous gift fromJerrold M. Olefsky, University of California, San Diego (La Jolla)(1). The generation and characterization of the polyclonalsheep anti-GLUT4 and the polyclonal sheep anti-GLUT1 antiserahave been previously described (21). Affinity-purified rhodamine-conjugateddonkey anti-sheep antibody was purchased from Jackson ImmunoResearch(West Grove, Pa.). Affinity-purified rabbit anti-hemagglutinin(HA), mouse anti-ARF6, and all horseradish peroxidase (HRP)-conjugatedsecondary antibodies were obtained from Santa Cruz BiotechnologyInc. (Santa Cruz, Calif.). The rabbit anti-green fluorescent protein(GFP) antiserum was purchased from Clontech (Palo Alto, Calif.).Bovine serum albumin (BSA) was purchased from Calbiochem. [1,2-³H]-2-deoxy-D-glucose was purchased from NEN Life Sciences Products(Boston, Mass.). Endothelin 1 and all other chemicals were purchasedfromSigma.

Generation of plasmid constructs. The inducible plasmid generated in this study is a derivative of the murine retroviral vector pLNCX1, which contains a neomycinresistance (Neo^r) gene to allow for the selection of stably infected cells (ClontechLaboratories Inc., Palo Alto, Calif.). The loxP sequence 5' tothe Neo^r cassette was generated by annealing the synthetic oligonucleotides5'-GAT CCG CTA GCA GTT AAC CGG TAT AAC TTC GTA TAG CAT ACA TTATAC GAA GTT ATT TAA ATG-3' and 5'-GAT CCA TTT AAA TAA CTT CGTATA ATG TAT GCT ATA CGA AGT TAT ACC GGT TAA CTG CTA GCG-3' andcloning them into the BclI site in pLNCX1. The second loxP sequence,3' to the Neo^r cassette, was generated by annealing the synthetic oligonucleotides5'-GAT CAA TAA CTT CGT ATA GCA TAC ATT ATA CGA AGT TAT CAA TTGGCC TAG GTC TCG AGT A-3' and 5'-AGC TTA CTC GAG ACC TAG GCC AATTGA TAA CTT CGT ATA ATG TAT GCT ATA CGA AGT TAT T-3' and cloningthem between the unique BamHI and HindIII sites. Insertion ofthis loxP sequence also removed the cytomegalovirus immediate-earlypromoter region. Proper orientation and fidelity of the loxP siteswas determined through sequence analysis of the indicated regions.The resulting plasmid was designated pLPNPX1, following the standardnomenclature for retroviral constructs. The HA-tagged human ARF6(T27N)construct, a generous gift from Julie G. Donaldson, National Institutesof Health (Bethesda, Md.), and enhanced GFP (EGFP) from plasmidpEGFP-N1 (Clontech Inc.) were then cloned into pLPNPX1, usingthe unique XhoI/BglII sites and the XhoI/NotI sites, respectively.All constructs were sequenced, and no errors werefound.

Cell culture, retroviral infection, and adenoviral infection. 3T3-L1 fibroblasts were cultured and differentiated as described (19). Prior to analysis 9 days following the initiationof differentiation, adipocytes were serum starved for 2 h in LeibovitzL-15 medium containing 0.2% BSA at 37°C in roomair.

Stably transfected sublines of 3T3-L1 fibroblasts containing the indicated inducible retroviral vector were generated throughthe use of retrovirus-mediated gene transfer. To achieve this,a 60-mm-diameter culture of 293T cells was transiently transfectedusing calcium phosphate with 2 µg each of the two pantropic retroviralpackaging constructs, pVSV G and pCgp, a generous gift from MichaelH. Malim, University of Pennsylvania (Philadelphia), and a pLPNPX1derivative containing either EGFP or ARF6(T27N). Cell-free viralsupernatants were harvested at 24 h and used to infect 3T3-L1fibroblasts. Stably infected populations were selected 48 h laterin medium containing G418 (600 µg/ml [active concentration]),pooled, and maintained in G418-containing medium until initiationof differentiation or infection with AdCre, whichever came first.To induce expression in the transduced populations, fibroblastswere infected with AdCre at a multiplicity of infection of 4,000for 24 h at 37°C in a minimal volume of Dulbecco modified Eaglemedium containing 0.5% BSA. Differentiated adipocytes were infectedsimilarly for 48 h, with the initiation of infection beginningon day 3 of differentiation for AdCre infection and on day 6 forinfection with G $alpha$ q(Q209L). All experiments on adipocytes wereperformed 9 dayspostdifferentiation.

Glucose uptake and GLUT1 and GLUT4 translocation assays. The methods for measuring 2-deoxy-D-glucose uptake rates and plasma membrane GLUT1 and GLUT4 levels by the plasma membranesheets assay have been described elsewhere (16). Digital imageacquisition, processing, and automated quantitation of plasmamembrane fluorescence intensity were performed using MetaMorphimaging system software (Universal Imaging Corporation, West Chester,Pa.). This system of automated quantitation uses the signal obtainedby staining the lipid components of the remaining plasma membranesto create a mask that is then used to identify areas to measurethe fluorescence intensity from corresponding images displayingGLUT1 or GLUT4 staining. Using this method, six randomly selectedfields of view each containing 60 to 100 plasma membrane sheetswere analyzed per experiment. All experiments were performed aminimum of three times, and the data presented represent the average± standard error of the mean (SEM) of thesereplicates.

Protein immunoblotting and Northern analysis. For Western blot analysis of expressed proteins, 25 µg of total cellular lysate, obtained by lysis in 2% sodium dodecyl sulfate(SDS)-66 mM Tris (pH 7.5), was submitted to SDS-polyacrylamidegel (PAGE) electrophoresis on a 12.5% polyacrylamide gel underreduced conditions. Following transfer to polyvinylidene difluoridemembranes, the membranes were subjected to immunoblotting usingthe antibodies indicated in the figures and HRP-conjugated secondaryantibodies. Western blots were developed using enhanced chemiluminescence(Amersham Pharmacia Biotech). For Northern analysis of the transducedretroviral message, 5 µg of total cellular RNA was fractionatedby electrophoresis in a 0.8% agarose gel in the presence of 50%formamide. Following transfer to a nylon membrane, the retroviralmRNA was detected with a random-primed DNA probe generated toa 0.6-kb portion of the retroviral transcript 3' to the secondloxPsite.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Generation of a Cre-inducible retroviral vector. Technical limitations have made it difficult to conditionally express genes in differentiated 3T3-L1 adipocytes. Recombinantvectors based on retroviruses and adenovirus as well as electroporationare now frequently used to introduce genes into 3T3-L1 cells,but all suffer from serious deficiencies. Given these limitations,we sought to develop a new system for inducible expression thatutilizes many of the strengths of both retroviruses and adenovirusbut eliminates their drawbacks. Using the retroviral vector pLNCXas a backbone, annealed synthetic oligonucleotides were used tocreate loxP sites on either side of the Neo^r gene, generating pLPNPX1. In doing so, the original cytomegalovirusimmediate-early promoter was removed. This created a retroviralvector that, when inserted into the host cell's genome, generatesa single polycistronic mRNA transcribed from the viral promotercontained within the 5' long terminal repeat (LTR). This singlemRNA contains coding regions for both the Neo^r gene followed by the gene of interest. Since the Neo^r gene is first, it is translated and provides an efficient meansto select stably infected cells. Translation of the induciblegene is extremely rare due to the lack of an internal ribosomalentry site in the polycistronic mRNA (Fig. 1a). However, uponinfection of the cells with AdCre, homologous recombination betweenthe two loxP sites flanking the Neo^r gene removes this region, thereby moving the inducible cDNA intoposition as the first open reading frame and allowing it to beexpressed (Fig. 1a).

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FIG. 1. Schematic of inducible retroviral vector. (a) The retroviral vector, designated pLPNPX1, contains the retroviral LTRs and a selectable Neo^r from the retroviral vector pLNCX for selection of infected cells. The Neo^r gene is flanked by loxP sequences and immediately followed by a multiple cloning site into which the cDNA of interest can be cloned. Since the only promoter is in the 5' LTR, a single polycistronic message is generated from the integrated retrovirus which allows for the translation of the Neo^r gene but does not permit translation of the open reading frame cloned downstream of it. This provides for the efficient selection of infected cells without expression of the introduced gene product. When expression of the gene of interest is desired, the cells are infected with AdCre. The Cre recombinase catalyzes recombination between the two loxP sites, thus removing the Neo^r cassette and allowing translation of the foreign gene. (b) 3T3-L1 fibroblasts stably transduced with the inducible retrovirus were mock infected ( $-$ ) or infected with AdCre (+). Total RNA was collected 3 days following the infection and subjected to Northern blot analysis with the retroviral probe that falls outside the loxP sites. A representative hybridization pattern is presented, with the approximate locations of the molecular markers indicated. The two predominant species represent genomic transcripts before (3.8 kb) and after (2.6 kb) excision of the Neo^r cassette.

To demonstrate that only one transcript is generated from the inserted retrovirus and that the desired recombination eventoccurs as predicted, Northern blot analysis of the retroviraltranscript was performed. 3T3-L1 preadipocytes were infected witha recombinant retrovirus generated from a plasmid in which theARF6 cDNA was inserted into the multiple cloning site downstreamof the second loxP sequence in pLPNPX1. Since the insert is 0.6kb, the integrated retrovirus would be predicted to generate agenomic transcript of about 3.8 kb before Cre-catalyzed homologousrecombination and 2.6 kb after excision of the Neo^r cassette (Fig. 1a). As shown in Fig. 1b, Northern blot analysisof RNA extracted from stably transduced 3T3-L1 fibroblasts priorto infection with AdCre revealed a single RNA species of the expected~3.8-kb size. Three days following infection with AdCre, the transcriptsize was reduced by ~1.2 kb to ~2.6 kb (Fig. 1b), consistent withthe loss of the ~1.2-kb Neo^r gene contained between the loxP sites. Under these conditions,there was little detectable full-length transcript remaining,indicating excision in virtually all of the cells expressing theretroviral mRNA. To demonstrate the utility of this system forthe expression of genes of interest, we cloned a cDNA encodingGFP into the inducible retrovirus vector and used this recombinantretrovirus to generate pools of G418-resistant 3T3-L1 preadipocytes.Western blot analysis of lysates obtained from these cells priorto infection by AdCre showed no detectable GFP. However, 3 daysfollowing infection of the same polyclonal population of 3T3-L1fibroblasts with AdCre, GFP was easily detected by Western blotting(Fig. 2a). As expected, infection of parental, nontransgenic 3T3-L1fibroblasts did not lead to the expression of GFP. The time coursefor induction of GFP expression in 3T3-L1 fibroblasts was relativelyrapid, such that expression could be easily observed at 24 h followinginfection with AdCre, and by 48 h uniform, robust expression wasachieved (Fig. 2b). In differentiated 3T3-L1 adipocytes, the timerequired for induction of GFP expression was slightly longer,but a uniformly high level of expression was still obtained in85 to 90% of cells by 5 to 7 days following infection with AdCre(Fig. 2c). The increased time required for expression in differentiated3T3-L1 adipocytes is likely to reflect the relative resistanceof these cells compared to fibroblasts to infection with AdCre.

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FIG. 2. Expression of a reporter GFP can be tightly controlled with the AdCre-inducible retrovirus. (a) Wild-type (WT) 3T3-L1 fibroblasts or 3T3-L1 fibroblasts stably infected with a version of the inducible retrovirus designed to encode GFP were mock infected ( $-$ ) or infected with AdCre (+). Three days later, total cellular lysates were collected and subjected to SDS-PAGE and Western immunoblotting with anti-GFP antisera. A representative blot is presented. Size is indicated in kilodaltons (b) 3T3-L1 fibroblasts that express GFP in response to AdCre infection were fixed at various times following infection with AdCre at time zero (t = 0). A representative composite photomicrograph depicting the relative levels of GFP fluorescence at the indicated number of days (xd) following infection with AdCre is presented. (c) 3T3-L1 adipocytes that express GFP in response to AdCre were infected with AdCre at time zero, and the fluorescence due to GFP from the same field of view was monitored daily. A representative composite photomicrograph depicting the relative levels of GFP fluorescence at the indicated number of days following infection with AdCre is presented. In panels b and c, time zero represents the signal from cells immediately prior to infection.

We have taken advantage of this retroviral system that drives highly regulated expression of foreign gene products to studythe effects of ARF6(T27N) in 3T3-L1 adipocytes. Consistent withprior experience in other tissue culture systems, it was not possibleto obtain significant numbers of 3T3-L1 fibroblasts stably expressingARF6(T27N); constitutive expression of the mutant protein yieldedfew G418-resistant cells, and those that survived grew slowlyand displayed abnormal morphology (data not shown). For this reason,a cDNA encoding ARF6(T27N) was cloned into pLPNPX1, retroviruswas prepared by transient transfection, and 3T3-L1 preadipocyteswere infected with the recombinant retrovirus. Pools of G418-resistantcells were expanded and noted to be indistinguishable from parental3T3-L1 cells with respect to growth kinetics and morphology. Asshown in Fig. 3, Western immunoblot analysis of lysates obtainedfrom these cells indicated that they also displayed highly regulatedexpression of ARF6(T27N). In lysates probed with an antibody whichrecognizes the HA epitope tag fused to the carboxyl terminus ofthe ARF6(T27N) protein, expression of the epitope-tagged transgenewas detected only after Cre-catalyzed excision of the Neo^r cassette following infection with AdCre; no immunoreactive proteinwas detected in the GFP-expressing cell line (Fig. 3, top). UponWestern blotting with an antibody against ARF6, expression ofthe epitope-tagged ARF6(T27N), which displays slightly slowerelectrophoretic mobility than the endogenous ARF6, is visualizedonly following induction by AdCre (Fig. 3, bottom). Use of theARF6 antibody also allows us to estimate the level of overexpressionof the mutant protein at one to two times that of endogenous ARF6(Fig. 3). Though this modest level of overexpression is optimalfor the experiments described below because it minimizes the possibilityof nonspecific inhibition of other ARF-dependent pathways, wehave observed as much as 50- to 100-fold overexpression of otherproteins with this system (data not shown).

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FIG. 3. The expression of ARF6(T27N) can be tightly controlled by AdCre. 3T3-L1 preadipocytes were stably infected with a version of the inducible retrovirus designed to encode either GFP or ARF6(T27N) following AdCre infection. Adipocytes from these GFP and ARF6(T27N) lines were then either mock infected ( $-$ ) or infected with AdCre (+). Total cellular lysates were prepared 6 days later and subjected to SDS-PAGE and Western immunoblotting with the antisera indicated. Even following extended exposure, virtually no HA-tagged ARF6(T27N) could be detected prior to infection with AdCre. Sizes are indicated in kilodaltons.

Expression of a dominant inhibitory ARF6 protein does not block insulin-stimulated glucose uptake but inhibits uptake stimulated by the endothelin/G $alpha$ q pathway. 3T3-L1 adipocytes infected with virus containing cDNAs encoding either GFP or ARF6(T27N) were infected with AdCre, allowingexpression of the ectopically expressed proteins, and hexose uptakewas measured. Induction of expression of GFP by AdCre did notalter the rates of either basal or insulin-stimulated 2-deoxyglucoseuptake (Fig. 4a). Similarly, expression of ARF6(T27N) upon infectionwith AdCre did not affect significantly either basal or insulin-stimulated2-deoxyglucose uptake (Fig. 4b). The latter data are consistentwith what has been reported for another GTP-binding-deficientmutant of ARF6 (42). To exclude an effect of the dominant negativeARF6 on the sensitivity of the cell to insulin, 2-deoxyglucoseuptake was measured in the presence of submaximal insulin concentrations.Dominant negative ARF6 did not alter the ability of insulin tostimulate 2-deoxyglucose uptake at any concentration of the hormonetested (Fig. 4c and d).

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FIG. 4. Expression of a dominant negative mutant of ARF6 in 3T3-L1 adipocytes does not affect insulin-stimulated hexose uptake. Six days following induction of GFP (a and b) or ARF6(T27N) (c and d) expression by infection with AdCre, 3T3-L1 adipocytes were treated with the indicated concentration of insulin for 20 min or left in medium without hormone, and the uptake of 2-[³H]deoxyglucose was measured. Nonspecific uptake measured in the presence cytochalasin B in the absence of insulin was subtracted from all values. The results shown are the means ± SEM of four independent experiments, each performed in triplicate.

Since Gq-coupled receptors stimulate both the translocation of an ARF6-containing vesicular compartment and GLUT4-containingvesicles to the plasma membrane, we decided to test whether theGLUT4 translocation caused by treatment of 3T3-L1 adipocytes withendothelin 1 was dependent on ARF6. Endothelin 1 activates 2-deoxyglucoseuptake in 3T3-L1 adipocytes three- to fivefold; as expected, inductionof GFP expression by infection of control cells with AdCre didnot significantly alter this response (Fig. 5a). However, whenAdCre was used to initiate the expression of a dominant inhibitoryform of ARF6, the ability of endothelin 1 to stimulate 2-deoxyglucoseuptake was inhibited by ~60% (Fig. 5b).

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FIG. 5. Expression of a dominant inhibitory mutant of ARF6 in 3T3-L1 adipocytes inhibits the ability of endothelin-1 (ET-1) to stimulate hexose uptake. Six days following induction of GFP (a) or ARF6(T27N) (b) expression by infection with AdCre, 3T3-L1 adipocytes were treated with 10 nM endothelin 1 for 20 min or left in medium without agonist, and the uptake of 2-[³H]deoxyglucose was measured as in Fig. 4. The results shown are the means ± SEM of four independent experiments, each performed in triplicate. The asterisk denotes P = 0.0004 comparing endothelin 1-stimulated ARF6(T27N) 3T3-L1 adipocytes not infected and infected with AdCre. The endothelin 1-stimulated ARF6(T27N) 3T3-L1 adipocytes infected with AdCre are also significantly different (P = 0.02) compared to the endothelin 1-stimulated GFP cells infected with AdCre.

In principle, the effects of ARF6(T27N) on endothelin action might occur at the level of the receptor or at a point in thedownstream signaling pathway. G $alpha$ q/11, which is thought to mediatethe action of endothelin on hexose uptake, has also been implicatedas an important modulator of ARF6 (6). To determine whetherthe effect of ARF6(T27N) on endothelin-induced hexose uptake occursat a site downstream of the endothelin receptor, we bypassed thelatter by increasing 2- deoxyglucose uptake with an adenovirusexpressing a constitutively active form of G $alpha$ q, G $alpha$ q(Q209L). Expressionof G $alpha$ q(Q209L) in 3T3-L1 adipocytes in which GFP expression hadbeen induced stimulated glucose uptake about twofold (Fig. 6a).Activation of 2-deoxyglucose transport by G $alpha$ q(Q209L) was inhibitedby ARF6(T27N) to an extent similar to that seen following exposureof cells to endothelin (Fig. 5b and 6b). These data are most consistentwith the idea that endothelin produces its effects on hexose uptakevia G $alpha$ q, or the extremely homologous G $alpha$ 11 isoform, and that thesite of action of ARF6(T27N) is at or after the heterotrimericG protein.

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FIG. 6. Expression of a dominant negative mutant of ARF6 in 3T3-L1 adipocytes inhibits the ability of activated G $alpha$ q to stimulate hexose uptake. Three days following induction of GFP (a) or ARF6(T27N) (b) expression by AdCre, adipocytes were either mock infected (Basal) or infected with a recombinant adenovirus expressing G $alpha$ q(Q209L) (multiplicity of infection of ~20). The uptake of 2-[³H]deoxyglucose was measured 72 h later. The results shown are the means ± SEM of four independent experiments, each performed in duplicate. The asterisk denotes the statistically significant difference (P = 0.003) for G $alpha$ q-stimulated ARF6(T27N) cells not infected compared to infected with AdCre and that (P = 0.003) for G $alpha$ q-stimulated AdCre-infected ARF6(T27N) cells compared to similarly treated GFP cells.

Expression of a dominant negative ARF6 does not block insulin-stimulated GLUT4 or GLUT1 translocation but does inhibit GLUT4 translocation in response to endothelin. In the basal state, GLUT4 is sequestered in a perinuclear tubulovesicular compartment; upon insulin treatment, the transporterredistributes to the plasma membrane, such that it increases about10- to 20-fold on the cell surface (4). In 3T3-L1 adipocytes,another transporter isoform, GLUT1, is expressed in greater abundancethan GLUT4 and also retained in an intracellular pool. However,intracellular sequestration of GLUT1 is less efficient than thatfor GLUT4, such that insulin generates only a three- to fivefoldincrease in plasma membrane GLUT1. Nonetheless, this degree oftranslocation might well explain relatively modest increases inglucose transport, such as that produced by exposure of cellsto endothelin. To assess the extent of translocation of each ofthe transporters under the conditions described above, we usedthe plasma membrane sheets assay to monitor the levels of GLUT1and GLUT4 in the plasma membrane of 3T3-L1 adipocytes. Thus, 3T3-L1adipocytes in which GFP or ARF6(T27N) expression was induced weretreated with insulin or endothelin 1, and plasma membrane sheetswere prepared. As shown in Fig. 7a, both hormones readily increasedthe abundance of GLUT4 on the cell surface of control 3T3-L1 adipocytes.Quantitation of a series of experiments indicated that the patternof GLUT4 translocation in response to either insulin or endothelinwas similar to the ability of each of these stimuli to increasehexose uptake (compare Fig. 7b to Fig. 4 and 5). As expected,induction of GFP by infection of these cells with AdCre was withouteffect on the GLUT4 translocation evoked by treatment with insulinor endothelin. Similarly, expression of ARF6(T27N) did not reducethe ability of insulin to stimulate GLUT4 translocation (Fig.7c). In marked contrast, when infection of 3T3-L1 adipocytes byAdCre was used to turn on expression of the dominant inhibitoryform of ARF6, endothelin 1 was significantly blocked in its abilityto elicit GLUT4 translocation (Fig. 7c and d).

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FIG. 7. Expression of a dominant negative mutant of ARF6 in 3T3-L1 adipocytes inhibits the ability of endothelin 1 to stimulate GLUT4 translocation to the plasma membrane. Six days following induction of GFP (a and b) or ARF6(T27N) (c and d) expression by infection with AdCre, 3T3-L1 adipocytes were exposed to either 10 nM endothelin 1 (ET-1) or 100 nM insulin for 20 min. Plasma membrane sheets were prepared and subjected to immunofluorescence microscopy using polyclonal sheep anti-GLUT4 antibodies and rhodamine-conjugated anti-sheep secondary antibodies. Images were captured with a cooled charge-coupled device camera. (a and c) Composite photomicrographs of a representative experiment depicting the presence of GLUT4 on the plasma membrane under the noted experimental conditions. (b and d) Using a mask created from an identical field of view to identify areas containing plasma membrane, the mean fluorescence intensity from images was quantitated and is presented as the mean ± SEM of three independent experiments. The asterisk denotes the statistically significant difference (P = 0.05) for endothelin 1-stimulated ARF6(T27N) cells not infected compared to infected with AdCre.

Next, we examined whether endothelin 1 was capable of increasing the abundance of GLUT1 on the surface of 3T3-L1 adipocytes.Insulin stimulated the translocation of GLUT1 to the plasma membraneapproximately threefold, and this was unaffected by the expressionof either GFP or dominant inhibitory ARF6 (Fig. 8). In contrast,endothelin 1 did not stimulate GLUT1 translocation (Fig. 8). Inaddition, expression of ARF6(T27N) had no effect on the steady-statelevels of GLUT1 on the plasma membrane under basal or endothelin-stimulatedconditions (Fig. 8c and d).

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FIG. 8. Effect of endothelin 1 and ARF6(T27N) on the translocation of GLUT1 to the plasma membrane in 3T3-L1 adipocytes. Expression of GFP (a and b) or ARF6(T27N) (c and d) was induced in 3T3-L1 adipocytes, which were then treated with endothelin 1 (ET-1) or insulin, and plasma membrane sheets were prepared as in Fig. 7. Immunofluorescence microscopy was performed with polyclonal sheep anti-GLUT1 antisera. (a and c) Composite photomicrographs of a typical experiment depicting the presence of GLUT1 on the plasma membranes from cells treated as indicated following induction of expression with AdCre; (b and d) fluorescence intensity expressed as the mean ± SEM of three independent experiments.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In this study we have described a novel inducible system, useful for the synchronous and quantitative induction of gene productsin both dividing and terminally differentiated tissue culturecells, and used it to express a dominant inhibitory form of ARF6in 3T3-L1 adipocytes. This small GTP-binding protein has beenimplicated in both vesicular trafficking events and reorganizationof the actin cytoskeleton. Two key features have made ARF6 attractiveas a potential intermediate in the pathway by which extracellularfactors regulate glucose transport. First, ARF6 is required indiverse cell types for translocation of membrane protein froman endosomal-like compartment to the plasma membrane as well asfor regulated secretion in chromaffin cells (7, 8, 14,15, 18, 32, 34, 38). Second, though the precise guaninenucleotide exchange factors responsible for activation of ARF6continue to be source of some controversy, all likely candidatesdisplay dependency on phosphatidylinositides for maximal activity(10, 12). Moreover, there is some direct evidence that bothrecruitment of these exchange proteins to the plasma membraneand activation of ARF6 in the intact cell are dependent on PI3-kinase (25, 30, 39, 40). Importantly, stimulation ofGLUT4 translocation by insulin and possibly endothelin also dependson the generation of phosphatidylinositides (11, 22). Despitethese arguments, our data are in agreement with previous datathat do not support strongly a role for ARF6 in the insulin-dependentregulation of glucose transport. In one study, peptides derivedfrom the ARF6 sequence partially inhibited GLUT4 translocationin permeabilized 3T3-L1 adipocytes (27). However, subsequentlyit was reported that expression of a GTP-binding-deficient mutantof ARF6, ARF6(D125N), did not block insulin-stimulated glucoseuptake (42). In this report, we have confirmed the latter resultemploying a more widely used ARF6 dominant inhibitory mutant,ARF6(T27N). However, we also show that, unlike for insulin, theactivation of hexose uptake and GLUT4 translocation in responseto endothelin is strongly dependent on ARF6. This result has severalimplications: (i) it clearly indicates that the pathways by whichinsulin and endothelin activate glucose transport are distinct;(ii) these data suggest the existence of a novel pool of GLUT4that is responsive to endothelin; and (iii) they add weight tothe proposed link between heterotrimeric G protein signaling andARF6-dependentevents.

ARF6 is remarkable in its capacity to influence both vesicular trafficking and cytoskeleton rearrangements. There is muchevidence that expression of a constitutively active ARF6 leadsto the redistribution of an endosome-like compartment to the plasmamembrane (14, 15, 32, 34, 38). Expression of a dominantinhibitory form of ARF6, such as the ARF6(T27N) used in this study,leads to accumulation of the mutant protein in pericentriolarstructures and the prevention of movement of ligands from endosomesto the cell surface (14, 15, 32, 34). Constitutively activeARF6 stimulates the protrusion of peripheral membrane structuresrich in actin filaments but morphologically distinct from thoseelicited by other small G proteins such as Rac or CDC42 (13,33, 35, 43). The most likely explanation for ARF6's seeminglydiverse effects is that it plays a role in the elaboration ofnew plasma membrane structures, a process that requires cytoskeletalchanges as well as the delivery of membrane to the cell surface.Consistent with this idea, ARF6 has been shown to be involvedin Fc-mediated phagocytosis in macrophages and cell spreadingin fibroblasts (37, 44).

Several recent studies implicating heterotrimeric G proteins in ARF6 action provided the motivation to assess the role ofthis small G protein in endothelin action in adipocytes. The effectsof constitutively active ARF6 are mimicked by addition of aluminumfluoride to cells overexpression the wild-type form of the G protein(34). Aluminum fluoride is known to activate heterotrimericG proteins, and the likely target of the drug in its regulationof ARF6 is G $alpha$ q (2). Boshans et al. have shown that bombesincauses the loading of ARF6 with GTP and the redistribution ofARF6-containing endosomal vesicles to the plasma membrane (6).Moreover, this was accompanied by characteristic actin cytoskeletalrearrangements. Both processes were dependent on G $alpha$ q and mimickedby a constitutively active form of G $alpha$ q. The key finding in thepresent report, that ARF6(T27N) blocks endothelin- but not insulin-stimulatedGLUT4 translocation, provides strong support for the linkage betweenG $alpha$ q and ARF6 but further suggests that heterotrimeric rather thanprotein kinase receptor-initiated signaling pathways preferentiallycouple to ARF6. This is somewhat surprising in view of insulin'spotency in activating PI 3-kinase in 3T3-L1 adipocytes and theimportance of phosphatidylinositides to the activation ofARF6.

As noted above, the simplest explanation for the differential dependency of insulin and endothelin on ARF6 is that the twohormones elicit translocation of GLUT4 by different mechanisms.While it is possible that endothelin and insulin signaling convergedownstream of the former's requirement for ARF6, we favor theidea that the pathways are distinct. Imamura et al. have presentedevidence that microinjection of an antibody to either G $alpha$ q/11 orp110 $alpha$ , the catalytic subunit of PI 3-kinase, blocks both insulin-and endothelin-induced GLUT4 translocation (22, 23). In partialagreement with Imamura et al., Kanzaki et al. have presented evidencethat either microinjection of an antibody against G $alpha$ q/11 or expressionof the GTPase-activating proteins RGS4 (regulator of G proteinsignaling 4) and RGS16, which inhibit G $alpha$ q, also block insulin-stimulatedGLUT4 translocation in 3T3-L1 adipocytes (24). It should benoted, however, that other investigators have reported that wortmannin,an inhibitor of PI 3-kinase, does not interfere with endothelin-stimulatedhexose uptake (5, 24, 41). In any case, both Imamura etal. and Kanzaki et al. have interpreted their results as indicativeof a role for a Gq family member in the signaling cascade leadingfrom the insulin receptor to the stimulation of glucose uptake(23, 24). However, the observation that G $alpha$ q- but not insulin-stimulatedhexose uptake is blocked by a dominant inhibitory ARF6 arguesagainst this idea (Fig. 4 and 6). One possibility is that a G $alpha$ q-dependentbut ARF6 independent pathway accounts for this discrepancy. Inany case, insulin increases the levels of both GLUT4 and GLUT1at the plasma membrane, whereas endothelin affects only GLUT4,again emphasizing fundamental differences in the signaling pathwaysinitiated by these hormones (Fig. 7 and 8).

What then is the ARF6-sensitive compartment from which GLUT4 translocates in response to endothelin? While we cannot excludethe possibility that ARF6 functions exclusively as a signalingintermediate, we favor the notion that following exposure of cellsto endothelin, ARF6 regulates the trafficking of a pool of glucosetransporters in 3T3-L1 adipocytes. Considerable evidence favorsthe existence of multiple intracellular pools of GLUT4. In brownfat cells in the basal state, about 60% of the GLUT4 is foundin tubulovesicular elements distributed throughout the cell, about10% is in the region of the trans-Golgi network, and the remainderis elsewhere in the cell (36). Following insulin stimulation,the amount of GLUT4 in the tubulovesicular elements and in theregion of the trans-Golgi network both decreased by 50%, witha concomitant increase in transporter at all the cell surfaceand in classical endosomal structures. This has been interpretedas indicative of a distribution of GLUT4 between endosomes anda novel insulin-responsive compartment often referred to as GLUT4storage vesicles. For example, ablation of endosomes by loadingwith HRP and treatment with H₂O₂ and diaminobenzidine clearlydistinguishes a resistant pool of GLUT4 that is enriched in thesynaptobrevin/vesicle-associated membrane protein 2 (26). Inaddition, recent reports have provided evidence that either 5'-O-(3-thiotriphosphate)or the serine/threonine protein kinase Akt/protein kinase B stimulatestranslocation of distinct subsets of intracellular GLUT4 (17,28). Thus, a plausible explanation of the data presented inthis report is that endothelin and insulin provoke translocationof distinct pools of GLUT4. Since the magnitude of the insulinresponse is greater than that for endothelin, we cannot excludethe possibility that the endothelin-sensitive compartment is alsoresponsive to insulin, but we are unable to discern even a modestinhibition of the insulin effect by ARF6(T27N). The precise natureof the intracellular compartment in which endothelin-responsiveGLUT4 resides and which is regulated by ARF6 remains obscure.Our data indicate that endothelin regulates GLUT4 independentlyof GLUT1 trafficking, even though GLUT1 and GLUT4 have been shownto colocalize on intracellular membranes and insulin stimulatesthe redistribution of both isoforms to the plasma membrane. SinceGLUT1, which is believed to traffic primarily between the plasmamembrane and the endosomal system, is not influenced by endothelin,it is unlikely that the hormone simply effects a redistributionof general endosomal proteins. These data are consistent withthe endothelin/Gq/ARF6 pathway not affecting the endosomal systemin adipocytes but instead affecting a relatively specialized compartmentpossibly designed for the polarized delivery of membrane proteinto membraneprotrusions.

The inducible expression system described in this report combines advantageous aspects of retroviral and adenoviral deliverysystems while avoiding a number of their limitations. Initiationof expression of the desired construct can be efficiently andsynchronously initiated through the use of a single recombinantadenovirus. The system appears to be highly regulated, as retrovirus-infectedcells express little or no foreign product prior to recombination.However, following induction with AdCre, 85 to 90% of the cellsinitiate expression of the inducible product, with a time coursein fibroblasts that is similar to that obtained by transient transfections.The 3T3-L1 adipocytes used in this study take slightly longerto initiate expression than other dividing and nondividing differentiatedcell types that we have tested with this system (J. T. R. Lawrenceand M. J. Birnbaum, unpublished observations). We anticipate thatthis inducible expression system will have general utility, asrecombinant retroviruses are relatively simple to prepare, andonly a single recombinant adenovirus is required for expressionof any geneproduct.

	ACKNOWLEDGMENTS

We thank Frank L. Graham, McMaster University (Hamilton, Ontario, Canada), Jerrold M. Olefsky, University of California, SanDiego (La Jolla), and Julie G. Donaldson, National Institutesof Health (Bethesda, Md.) for the gift of reagents and the VectorCore of the Penn Diabetes Center (P30 19525) for amplificationof adenovirus. We also thank Michael P. Czech and Martha S. Jordanfor discussions and critical reading of themanuscript.

This work was supported by National Institutes of Health grants DK39615 (M.J.B.) and National Research Service Award for Trainingin Cell and Molecular Biology GM07229 (J.T.R.L.).

	FOOTNOTES

^* Corresponding author. Mailing address: Howard Hughes Medical Institute, University of Pennsylvania Medical School, 415 CurieBlvd., Room 322 CRB, Philadelphia, PA 19104. Phone: (215) 898-5001.Fax: (215) 573-9138. E-mail: birnbaum{at}mail.med.upenn.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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Bose, A., Cherniack, A. D., Langille, S. E., Nicoloro, S. M. C., Buxton, J. M., Park, J. G., Chawla, A., Czech, M. P. (2001). G{alpha}11 Signaling through ARF6 Regulates F-Actin Mobilization and GLUT4 Glucose Transporter Translocation to the Plasma Membrane. Mol. Cell. Biol. 21: 5262-5275 [Abstract] [Full Text]

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