Insulin Control of Glycogen Metabolism in Knockout Mice Lacking the Muscle-Specific Protein Phosphatase PP1G/RGL

doi:10.1128/MCB.21.8.2683-2694.2001

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Molecular and Cellular Biology, April 2001, p. 2683-2694, Vol. 21, No. 8
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.8.2683-2694.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Insulin Control of Glycogen Metabolism in Knockout Mice Lacking the Muscle-Specific Protein Phosphatase PP1G/R_GL

Yoichi Suzuki,¹^, Carita Lanner,¹ Jong-Hwa Kim,¹ Pier Giuseppe Vilardo,¹ Hong Zhang,¹ Jie Yang,¹ Lori D. Cooper,¹ Marcella Steele,¹ Andrew Kennedy,¹ Cheryl B. Bock,² Angus Scrimgeour,³ John C. Lawrence Jr.,³ and Anna A. DePaoli-Roach¹^,^*

Department of Biochemistry and Molecular Biology, Indiana University School of Medicine, Indianapolis, Indiana 46202¹; Comprehensive Cancer Center, Duke University Medical Center, Durham, North Carolina 27710²; and Department of Pharmacology, University of Virginia, School of Medicine, Charlottesville, Virginia 22908³

Received 13 October 2000/Returned for modification 27 November 2000/Accepted 17 January 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The regulatory-targeting subunit (R_GL, also called G_M) of the muscle-specific glycogen-associated protein phosphatase PP1Gtargets the enzyme to glycogen where it modulates the activityof glycogen-metabolizing enzymes. PP1G/R_GL has been postulatedto play a central role in epinephrine and insulin control of glycogenmetabolism via phosphorylation of R_GL. To investigate the functionof the phosphatase, R_GL knockout mice were generated. Animalslacking R_GL show no obvious defects. The R_GL protein is absentfrom the skeletal and cardiac muscle of null mutants and presentat ~50% of the wild-type level in heterozygotes. Both the leveland activity of C1 protein are also decreased by ~50% in the R_GL-deficientmice. In skeletal muscle, the glycogen synthase (GS) activityratio in the absence and presence of glucose-6-phosphate is reducedfrom 0.3 in the wild type to 0.1 in the null mutant R_GL mice,whereas the phosphorylase activity ratio in the absence and presenceof AMP is increased from 0.4 to 0.7. Glycogen accumulation isdecreased by ~90%. Despite impaired glycogen accumulation in muscle,the animals remain normoglycemic. Glucose tolerance and insulinresponsiveness are identical in wild-type and knockout mice, asare basal and insulin-stimulated glucose uptakes in skeletal muscle.Most importantly, insulin activated GS in both wild-type and R_GLnull mutant mice and stimulated a GS-specific protein phosphatasein both groups. These results demonstrate that R_GL is geneticallylinked to glycogen metabolism, since its loss decreases PP1 andbasal GS activities and glycogen accumulation. However, PP1G/R_GLis not required for insulin activation of GS in skeletal muscle,and rather another GS-specific phosphatase appears to beinvolved.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

In recent years, the generality that the activity of the type 1 serine/threonine protein phosphatases (PP1) is dictated bythe associated noncatalytic subunits has emerged. These ancillaryproteins are thought to target the catalytic component (C1) todistinct subcellular locales in proximity to substrates, to conferspecificity, and to regulate activity (10, 21, 33, 41).To date, more than 30 C1-binding polypeptides have been identifiedthat direct the enzyme to a variety of subcellular structures,including glycogen (6, 24, 25, 49, 59, 60), myosin(2), ribosomes (31), nuclei (4, 13), and neuronal structures(5). A subset of C1-binding proteins includes inhibitory proteinssuch as inhibitors 1 and 2 (48, 67) and DARPP-32 (46).

Four C1-glycogen-targeting subunits are presently known. R_GL, also called G_M, was the first glycogen-binding subunit of PP1identified (59), and the corresponding holoenzyme, PP1G/R_GL,consists of the 124-kDa R_GL protein (60) in association withC1. R_GL is exclusively expressed in skeletal and cardiac muscle(37, 60). The NH₂-terminal 240 amino acids contain bindingsites for glycogen and C1 (64), whereas a hydrophobic regionbetween residues 1063 and 1097 in the COOH terminus anchors theprotein to membrane (45, 60). Of the other three glycogen-targetingsubunits, G_L, a 33-kDa polypeptide, is specifically expressedin liver (24), whereas PTG/R5 and R6 are ubiquitously distributed(6, 25, 49). All three share homology with the NH₂-terminalregion of R_GL. The activity of liver PP1G/G_L is controlled allostericallyby glycogen phosphorylase (Ph) and by glucose-6-phosphate (G-6P)(1, 58), and expression of the G_L subunit is downregulatedin diabetic rats (23). Protein targeting to glycogen (PTG) interactswith glycogen-metabolizing enzymes (26) and has been implicatedin insulin control of glycogen synthase (GS) (49). Overexpressionof PTG in Chinese hamster ovary cells expressing the human insulinreceptor increased basal and insulin-stimulated GS activity (49).Neither insulin nor forskolin induced detectable PTG phosphorylation,arguing against such a mechanism for PTG regulation. Adenovirus-mediatedoverexpression of G_L, PTG, or R_GL in primary rat hepatocytes resultsin basal activation of GS (12), but only in cells overexpressingG_L or PTG was GS activated by insulin (27). Other studies havepostulated a mechanism whereby PTG would affect PP1 activity byrelieving inhibition by DARPP-32 (16). However, it has beenshown that neither I-1 nor DARPP-32 is required for insulin activationof GS (53). Thus, the mechanisms for control of PTG- and R6-containingphosphatases are largelyunknown.

In mammals, the major stores of glycogen are in skeletal muscle and liver. Although glycogen in these two tissues performsdifferent functions, both pools contribute to glucose homeostasis.Approximately 80% of postprandial, insulin-stimulated glucoseuptake is stored as glycogen in skeletal muscle (56). This insulin-stimulatedglycogen synthesis involves activation of both glucose transportand GS (39). Glycogen metabolism is controlled in large partby the coordinated regulation of the two enzymes responsible forits synthesis and breakdown, GS and Ph. GS is inactivated by acomplex, multisite phosphorylation mechanism involving severalprotein kinases, including GS kinase 3 (GSK-3) (38, 52). Theallosteric activator G-6P can restore full activity, so that theGS activity ratio in the absence and presence of G-6P ( $-$ /+ G-6Pactivity ratio) is used as a kinetic index of phosphorylationstate. Ph is activated by phosphorylation of a single site byphosphorylase kinase (PhK). Insulin promotes dephosphorylationand activation of GS, with no significant effect on Ph. Despiteextensive investigation over the last four decades, the exactmolecular mechanism(s) by which insulin activates GS in skeletalmuscle is not fully understood. Epinephrine causes phosphorylationof both GS and Ph, leading to their respective inactivation andactivation so that glycogen is degraded. Dephosphorylation ofthe key regulatory enzymes, GS, Ph, and PhK, is believed to becatalyzed primarily by glycogen-associated phosphatases (59).Also, association of R_GL with C1 has been shown to enhance activitytowards these three glycogen-metabolizing enzymes (33).

PP1G/R_GL has been postulated to play a central role in both insulin and epinephrine control of glycogen metabolism in skeletalmuscle, via phosphorylation of the R_GL-targeting subunit (20,47). Insulin control of PP1G/R_GL would be mediated by the insulin-stimulatedprotein kinase ISPK or p90^rsk which is itself regulated via the mitogen-activated protein kinasepathway (20). ISPK phosphorylates R_GL at site 1 in vitro, enhancingthe rate of dephosphorylation of GS and PhK, with no effect onthe activity towards Ph. Treatment of rabbits with insulin wasreported to increase the phosphorylation of site 1 (20). Thehypothesis for control of PP1G/R_GL by insulin was attractive,since this enzyme dephoshorylates GS at both the COOH- and NH₂-terminalsites that are responsive in vivo to the hormone (38). However,several reports have shown that the mitogen-activated proteinkinase pathway is not involved in insulin activation of GS (9,40). Nevertheless, the results of these studies do not precludethe possibility that PP1G/R_GL mediates insulin regulation of glycogenmetabolism by othermechanisms.

Newer models for the control of GS activity by insulin have centered on a role for the PI-3K pathway (17, 54) and controlof GSK-3, an important GS kinase whose activity is known to beinhibited by insulin. Stimulation of PI-3K by insulin would activateAkt/PKB which phosphorylates and inactivates GSK-3. Another pathwayactivated by insulin involves mTOR, the mammalian target for theimmunosuppressant drug rapamycin (9); rapamycin has been shownto oppose insulin-mediated activation of GS in muscle and 3T3-L1adipocytes (9, 54). Since rapamycin does not block insulin-inducedinactivation of GSK-3 (18), it is possible that mTOR could controlGS phosphorylation via aphosphatase.

To address the role of PP1G/R_GL in the hormonal control of glycogen metabolism in a more definitive manner, we have generatedR_GL knockout mice. Analysis of this animal model clearly demonstratesthat R_GL has an important role in glycogen synthesis but is notessential for insulin activation ofGS.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Materials. pBluescript II KS(+), pCR II, and pET15b were from Stratagene (La Jolla, Calif.), Invitrogen (Carlsbad, Calif.), and Novagen(Madison, Wis.) respectively. Aspergillus niger amyloglucosidase,yeast hexokinase, and yeast G-6P dehydrogenase were purchasedfrom Sigma (St. Louis, Mo.). Restriction enzymes were from NewEngland Biolabs (Beverly, Mass.). Porcine insulin was a gift fromEli Lilly Co. (Indianapolis, Ind.). The Puregene DNA isolationkit was from Gentra Systems (Minneapolis, Minn.). Taq polymerasewas purchased from Promega. Radioactively labeled nucleotides, $alpha$ -D-[U-¹⁴C]glucose-1-phosphate and UDP[U-¹⁴C]glucose were purchased from NEN Life Science Products (Boston,Mass.). Okadaic acid was from Roche Molecular Biochemicals (Indianapolis,Ind.). Oligonucleotides were synthesized by Life Technologies(Bethesda, Md.). Monoclonal anti-C1 antibodies that recognizeall isoforms were generously provided by Jackie Vandenheede (Universityof Leuven, Leuven, Belgium), and anti-GS antibodies were generouslyprovided by John C. Lawrence, Jr. (University of Virginia, Charlottesville).Antibodies to PTG and R6 were kindly provided by Alan Saltiel(Pfizer Global Research and Development, Ann Arbor, Mich.) andPatricia Cohen (University of Dundee, Dundee, United Kingdom),respectively. Anti-phosphorylated site 1 and site 2 R_GL antibodieswere a generous gift from Philip Cohen (University of Dundee).DNA sequencing was done at the Indiana University Biochemistryand Biotechnology Facility (Indianapolis) on an ABI PE-ABI 377XLlaser sequencer using fluorescent dideoxy terminators. Antiseraagainst mouse R_GL was produced by immunizing rabbits with recombinantHis-R_GL(1-262) protein. Other chemicals were purchased from Sigmaand Bio-Rad (Hercules, Calif.).

Construction of R_GL gene-disrupting targeting vector. A 129Sv mouse genomic DNA library made in Lambda DASH II was provided by Bi Feng (Lunenfeld Research Institute, Toronto, Ontario,Canada). Screening of 8.3 × 10⁵ plaques using rabbit R_GL cDNA (3.8 kb) (60) as a probe resultedin isolation of seven positive clones, four of which containedoverlapping sequences (37). Restriction mapping and sequenceanalysis revealed that one of the clones contained 785 nucleotidesthat code for exon 1, flanked by ~5 kb upstream and 11 kb downstream.To generate the targeting vector, an 0.8-kb HindIII-EcoRV fragment,which is upstream of exon 1, was inserted into the SalI site ofpBluescript II/NeoTK vector (Fig. 1) (7) which contains thephosphoglycerokinase (PGK) promoter driving the neo gene (PGK-neo)and the herpes simplex virus thymidine kinase gene (HSV-tk). A7.0-kb BsmI-BsmI fragment downstream of exon 1 was inserted atthe XhoI site of the vector. By this strategy, 785 bp coding for262 amino acids in exon 1, 50 bp upstream of the start ATG codon,and 16 bp of intron 1 were replaced by the neomycin resistancegene. The targeting vector was linearized at the NotI site andused for electroporation into embryonic stem (ES) cells.

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FIG. 1. Targeted disruption of the R_GL gene. (A) Maps of the mouse R_GL gene locus, the targeting vector, and the disrupted R_GL gene locus. Restriction sites BsmI (Bs), EcoRV (E), HindIII (H), and PstI (P) are shown. Arrowheads indicate the positions of the PCR primers (ADPR266 and ADPR267). Thick bars below the map of the disrupted locus represent the positions of the probes used for Southern blot analysis. PGK, phosphoglycerokinase gene promoter; HSV-tk, herpes simplex virus thymidine kinase gene. (B) Genotyping of wild-type, heterozygous, and homozygous R_GL mutant mice. Primers from the R_GL and neo genes generated 1.2 and 0.9-kb fragments for the wild type (WT) and the R_GL knockout (KO) gene.

Generation of R_GL knockout mice. Culture of ES cells and isolation of homologous recombinants were performed according to standard protocols (32). Briefly,10⁷ CCE, E14, or R1 ES cells were transfected with 25 to 50 µg ofthe linearized vector. The cells were cultured under selectionin G418 and ganciclovir. Resistant colonies were expanded in 98-wellplates. Screening for homologous recombinants was performed byPCR methods as described previously (32). Oligonucleotides 5'-TTCTATCGCCTTCTTGACGAGTTC-3'(ADPR266; in the neo gene) and 5'-TCCATGATGAGTACTACATCCACT-3'(ADPR267; in the R_GL gene) were used as primers (Fig. 1). Sevenpositive clones were identified and subjected to Southern blotanalysis to confirm the structure of the targeted region. ES cellgenomic DNA was digested with PstI. The 5' external probe andthe internal probe shown in Fig. 1 and the neo gene were usedas probes. All seven ES cell clones were confirmed to containthe targeted disruption and used to generate R_GL knockout mice,by standard procedures (32), utilizing C57BL/6J blastocystsand pseudopregnant females as foster mothers. Chimeric mice werescreened by PCR and by Southern blotting for the presence of thedisrupted R_GL allele and mated with C57BL/6J mice to produce F₁heterozygous mice. Heterozygotes for the disrupted gene were identifiedby PCR using digit samples. Confirmed heterozygous F₁ mice werebackcrossed with C57BL/6J mice or mated with siblings to generatenull mutant mice. Some of the chimeric mice were also crossedwith wild-type 129SvJ, and the resulting F₁ heterozygotes werebackcrossed with 129SvJ to generate genetically defined mice.All mice were maintained in temperature and humidity-controlledconditions with a 12-h light-12-h dark cycle and were allowedfood and water ad libitum. The R_GL chimeric mice were generatedby David A. Williams at Indiana School of Medicine, Indianapolis,and by Cheryl Bock at Duke Comprehensive Cancer Center, TransgenicFacility, Durham, N.C.

Southern blot analysis. Genomic DNA from ES cells was prepared with the Puregene DNA isolation kit. Genomic DNA was isolated from mouse tail by theproteinase K digestion method. Mouse tail pieces (1 to 2 cm) wereclipped and digested in a solution containing 100 mM NaCl, 10mM Tris-HCl (pH 7.8), 1% sodium dodecyl sulfate, 200 µg of proteinaseK per ml at 57°C overnight. After two chloroform-isoamyl alcohol(24:1) extractions, the DNA was precipitated with ethanol. GenomicDNA (10 to 20 µg) digested with PstI (~5 U/µg or more) was resolvedby electrophoresis in 0.5% agarose gels and transferred to nitrocellulosemembranes (BA-85; Shleicher & Schuell). DNA fragment probes wereradiolabeled with ³²P using the Megaprime DNA labeling system(Amersham).

Western blot analysis. For the various biochemical determinations, unless otherwise indicated, normally fed animals were sacrificed in the earlyafternoon. Mice were anesthetized by intraperitoneal injectionof sodium pentobarbital (0.1 mg/g of body weight). Skeletal muscleof hind legs and heart were excised quickly, freeze-clamped inliquid nitrogen, and stored at $-$ 80°C till use. For Western blotanalyses, frozen tissue samples were homogenized in 10 volumes(wt/vol) of a solution containing 50 mM Tris-HCl (pH 7.5) (25°C),0.5 mM EDTA, 2 mM EGTA, 1% Triton X-100, 0.1 mM N-p-tosyl-L-lysine chloromethyl ketone, 2 mM benzamidine, 0.5 mMphenylmethylsulfonyl fluoride, and 10 µg of leupeptin per ml witha Tissue Tearer model 285-370 (Biospec Products Inc.) at maximalsetting for 20 s. The homogenates were centrifuged at 600 × gfor 5 min. The resultant supernatants were subjected to sodiumdodecyl sulfate-polyacrylamide gel electrophoresis. The proteinson the gels were transferred to nitrocellulose membranes whichwere then incubated with the appropriate antibodies. Binding ofthe antibody was detected either by ¹²⁵I-labeled protein A or by horseradish peroxidase-conjugated secondaryantibody and enhanced chemiluminescence. Levels of protein expressionwere quantitated by densitometric scanning of thefilms.

Enzyme activity assays. Ph phosphatase activity was assayed essentially as described previously (67) except that the total volume of the reactionmixture was reduced to 40 µl. The same supernatant samples usedfor the Western blot analysis were diluted 100-fold with a solutioncontaining 50 mM Tris-HCl (pH 7.2), 0.2% $beta$ -mercaptoethanol, 0.1mM EDTA, and 1 mg of bovine serum albumin per ml. Ten-microliterportions of the diluted samples were used for determination ofphosphatase activity, utilizing 1 mg of [³²P]Ph a per ml as a substrate in the presence or absence of 4 nMokadaic acid. One unit is defined as the amount of enzyme thatreleases 1 nmol of phosphate per min. For GS and Ph assays, tissuesamples were homogenized in 20 volumes of buffer (50 mM Tris-HCl[pH 7.8], 10 mM EDTA, 2 mM EGTA, 100 mM NaF, 2 mM benzamidine,0.1 mM N-p-tosyl-L-lysine chloromethyl ketone, 50 mM $beta$ -mercaptoethanol,0.5 mM phenylmethylsulfonyl fluoride, and 10 µg of leupeptin perml) using a Polytron homogenizer (Kinematica) for 20 s. Aftercentrifugation at 3,600 × g for 5 min, 30 µl of the supernatantwas used for GS and Ph assays. GS activity was determined by measuringincorporation of [¹⁴C]glucose from UDP-[¹⁴C]glucose into glycogen as described by Thomas et al. (61) inthe absence or presence of 7.2 mM G-6P. Ph activity was assayedby measuring incorporation of [¹⁴C]glucose from [¹⁴C]glucose-1-phosphate (28) into glycogen in the absence or presenceof 2 mM AMP. One unit of GS is the amount of enzyme that incorporates1 µmol of [¹⁴C]glucose from UDP-[U-¹⁴C]glucose into glycogen per min, and 1 U of Ph is the amount ofenzyme that incorporates 1 µmol of [¹⁴C]glucose from [U-¹⁴C]glucose-1-phosphate per min. Activity ratios represent the activitymeasured in the absence of the allosteric effector (G-6P for GSor AMP for Ph) divided by that in the presence of the allostericeffector.

For determination of the effects of insulin on GS, Ph, and phosphatase activities and glycogen content, anesthetized 17 to20-week-old R_GL null mutant mice and wild-type littermates fastedfor 6 h (8:00 a.m. till 2:00 p.m.) were injected in the tail veinwith 2 U of insulin/kg of body weight. After 5 min, animals weresacrificed, and skeletal muscle was rapidly removed and frozenin liquid nitrogen. GS phosphatase activity was measured by utilizingpartially purified phosphorylated GS and by monitoring the changein the GS $-$ /+ G-6P activity ratio between zero time and after15 min of incubation with muscle extract, following the proceduredescribed by Villar-Palasi (62). Responsiveness of the animalsto insulin was confirmed by determination of blood glucose levelsbefore and after insulin administration. Under the conditionsused, the blood glucose decreased by ~40% in both groups. Proteinconcentration was determined by the Bradford method (14) usingbovine serum albumin asstandard.

Determination of glycogen content. Samples of frozen tissues (30 to 90 mg) were hydrolyzed in 0.3 ml of 30% (wt/vol) KOH solution in a boiling water bath for30 min. At 10 and 20 min of the incubation, tubes were shakenby hand to facilitate the digestion. After cooling to room temperature,0.1 ml of 1 M Na₂SO₄ and 0.8 ml of ethanol were added, the sampleswere boiled again for 5 min to facilitate precipitation of glycogenand then centrifuged at 10,000 × g for 5 min. The glycogen pelletwas dissolved in 0.2 ml of water, and two additional ethanol precipitationswere performed. The final pellet was dried and dissolved in 0.2ml of 0.3-mg/ml amyloglucosidase in 0.2 M sodium acetate buffer(pH 4.8) and incubated for 3 h at 40°C. The reaction mixture wasthen diluted two- to fivefold with water. To determine the glucoseconcentration, 5 µl of the diluted sample was added to 0.2 mlof the glucose assay solution which contains 0.3 M triethanolamine-KOH(pH 7.5), 1 mM ATP, 0.9 mM $beta$ -NADP, and 5 µg of G-6P dehydrogenaseper ml. The absorbance at 340 nm was determined before and afteraddition of 1 µg of hexokinase (11). Glycogen content was expressedas micromoles of glucosyl units per gram (wetweight).

Glucose and insulin tolerance tests. Glucose and insulin tolerance tests were performed on homozygous null mutant mice and wild-type littermates at different ages,6 to 8, 14 to 18, and 40 to 48 weeks. For glucose tolerance tests,animals were fasted for 16 h. Glucose (2 mg/g of body weight)was administered intraperitoneally. Blood samples were collectedfrom the tail at various times, and blood glucose was measuredusing a Glucometer Elite (Ames). For insulin tolerance tests,6-h-fasted animals were injected intraperitoneally with 1 mU ofporcine insulin per g. Blood glucose levels were monitored asdescribed above for the glucose tolerancetest.

Other procedures. 2-Deoxyglucose uptake in mouse diaphragm muscle was measured as previously described (57). Whole-body glucose disposal studiesin euglyemic hyperinsulinemic mice were performed by Alain Baronat Indiana University, as previously described (30). Serum lactateand triglyceride levels were measured in the Immunology Core Facilityof the Diabetes Research and Training Center at IndianaUniversity.

Statistical analyses. Statistical analyses were performed using the StatView program. Significance was assessed using the unpaired Student's t test.Results are expressed as the mean ± standard error (SE) of thenumber of animals indicated in the figurelegends.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Generation of R_GL knockout mice. The strategy to generate R_GL knockout mice was to disrupt the gene by replacing exon 1 which codes for the first 261 residues(785 bp) with the neomycin resistance gene (Fig. 1A). By thisapproach, the translational initiation codon, the C1 and glycogen-bindingdomains, and phosphorylation sites Ser48 and Ser67 would be removed.Even if exon 1 were skipped, the resulting mRNA starting at exon2 would be out of frame. Furthermore, since intron 1 is far removedfrom the promoter (more than 27 kb), it is unlikely that a transcriptcould be expressed. A screen of 195 resistant cell clones gave7 PCR positives, all of which were confirmed by Southern blotting.All seven lines were used to generate knockout mice. Twenty-fourchimeras were obtained, 12 of which had high percentage of agouticoat color (75 to 100%) and were positive for the disruption byPCR analysis. Nine were males, and mating with C57BL/6 mice revealedthat seven were fertile, six of which transmitted the targetedallele to their offspring. Genotyping by PCR shows a 900-bp amplifiedDNA fragment for the disrupted allele and a 1,235-bp fragmentfor the wild type (Fig. 1B). Southern blots of PstI digests indicatedan 18-kb fragment for the disrupted allele and a 26-kb fragmentfor the wild type (data not shown). Mating of animals heterozygousfor the disrupted R_GL allele has generated homozygous null mutantmice.

Analysis of 167 F₂ mice showed that the percentages of wild-type (+/+), heterozygous (+/ $-$ ), and homozygous null ( $-$ / $-$ ) R_GLmice were 32, 45, and 23%, respectively. No significant differencein this ratio was observed between males and females, indicatingthat the R_GL gene is located on an autosome and that the knockoutis not lethal in utero. All animals, heterozygotes as well ashomozygotes, macroscopically appeared normal with no obvious developmentalor morphological defects and grew at a rate indistinguishablefrom that of wild-type littermates (Fig. 2D). The heart to bodyweight ratios are also within the normal range.

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FIG. 2. Analysis of expression of R_GL and C1 in wild-type and knockout mice. (A) Skeletal muscle extracts were subjected to immunoblotting with anti-R_GL (top) or anti-C1 (bottom) antibodies. (B) Quantitation by densitometric scanning of the autoradiogram shown in panel A, expressed as a percentage of the mean of the wild type ± SE (n = 6 to 8 per group). (C) Ph phosphatase activity was measured in the presence of 4 nM okadaic acid (OA) in skeletal muscle extracts as described in Materials and Methods. The number of animals in each group is indicated in each bar. Statistical significance was assessed by Student's t test (**, P < 0.01). (D) Growth curves of wild-type (open circles) and R_GL null mutant (closed circles) mice with 3 to 19 animals per point. The means ± SE are shown. +/+, wild type; +/ $-$ , heterozygotes, $-$ / $-$ , homozygote null mutants.

Analysis of PP1G/R_GL expression in knockout mice and wild-type littermates. Western immunoblotting analysis of skeletal (Fig. 2A and B) and cardiac (not shown) muscle extracts using mouse R_GL antibodiesindicated that the protein was absent from the homozygous animalsand present at ~50% of the wild-type level in heterozygotes. R_GL-deficientmice had a 60% reduction in the level of C1 in skeletal muscle(Fig. 2A and B), and a significant 25% reduction was also observedin the heterozygous animals. These results indicate that the functionalgene is disrupted, that PP1G/R_GL accounts for a large proportionof PP1 in striated muscles, and that the presence of the regulatoryR_GL is linked to the expression level of C1. Consistent with reducedC1 protein, the type 1 phosphatase activity was also decreased,with activity towards Ph $alpha$ reduced by ~60% in the R_GL null miceand by 30% in heterozygotes (Fig. 2C). The activity towards GSphosphorylated in the site 3 region was decreased by 40% in thehomozygotes. Although not as pronounced, reductions in R_GL, C1,and phosphatase activity were also observed in heart (data notshown), consistent with the ~10-fold-lower level of expressionof R_GL in this tissue (37, 60).

Effect of ablation of PP1G/R_GL on glycogen metabolism. To determine the effect of PP1G/R_GL deficiency on the glycogen-metabolizing enzymes, GS and Ph activities were measured inskeletal muscle extracts. The GS $-$ /+ G-6P activity ratio was reducedfrom 0.3 in the wild-type littermates to 0.1 in the R_GL null mutantsand to 0.17 in the heterozygotes (Fig. 3A). Conversely, the activitystate of Ph, measured as the activity ratio in the absence andpresence of AMP, increased from 0.37 in the wild type to 0.7 inthe homozygous mutant mice and to 0.54 in the heterozygotes (Fig.3C). The total GS activity, as determined by activity measuredin the presence of G-6P, was also reduced by ~30% (Fig. 3B), aswas the protein level monitored by Western immunoblotting. Thetotal Ph activity, measured in the presence of AMP, was unaffectedin both heterozygous and homozygous mutants (Fig. 3D). Similareffects were observed in five independent knockout lines of mixedBL57 and 129Sv background and in both male and female animals,indicating that there are no gender differences. Consistent withthe altered GS and Ph activities, the glycogen content was dramaticallydecreased in the null mutant mice of both genetic backgroundsto ~10% of the wild-type level and to ~40% in the heterozygouslittermates (Fig. 4A). Similar changes in GS and Ph activitiesand glycogen levels were observed in null mice generated fromF₃ heterozygotes obtained after backcrossing the chimeras andsubsequent generations with 129Sv mice, suggesting that the effectsof the R_GL ablation are independent of the genetic background.PP1/R_GL is therefore a significant GS and Ph phosphatase, determiningthe phosphorylation state and activity of the glycogen-metabolizingenzymes. The extremely low glycogen level in the R_GL null mutantmay indirectly be responsible for the reduced amount of GS protein.All the GS in skeletal muscle is bound to glycogen whose low contentin the knockout mice may limit GS association, leading to lowerstability and enhanced degradation. It is interesting though,that even in the R_GL null mutants, all of the GS present was boundto glycogen. In contrast to GS, only 50% of the Ph in the muscleis bound to glycogen, so that its stability may be less dependenton association with the polysaccharide.

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FIG. 3. GS and Ph activity in skeletal muscle of wild-type and R_GL knockout mice (A) GS activity was assayed in the absence ( $-$ ) and presence (+) of G-6P in supernatant (after centrifugation at 3,600 × g for 5 min) of skeletal muscle from wild-type (+/+), R_GL heterozygous (+/ $-$ ), and homozygous ( $-$ / $-$ ) mice. (B) Total GS activity measured in the presence of 7.2 mM G-6P, expressed as nanomoles per minute per milligram of protein. (C) Ph activity was assayed in the absence ( $-$ ) and presence (+) of 2 mM AMP. (D) Total Ph activity measured in the presence of AMP, expressed as micromoles per minute per milligram of protein. The means ± SE are shown. Statistical significance was assessed by Student's t test (**, P < 0.01). The number of animals analyzed is shown inside the bars.

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FIG. 4. Glycogen content in skeletal muscle and liver. Glycogen content in skeletal muscle (A) and liver (B) of wild-type (+/+), R_GL heterozygous (+/ $-$ ), and homozygous ( $-$ / $-$ ) mice was determined by an alkaline lysis method as described in Materials and Methods. Glycogen concentration is expressed as micromoles of glycosyl units per gram (wet weight). The means ± SE are shown. Statistical significance was assessed by Student's t test (**, P < 0.01). The number of animals analyzed is shown inside the bars.

Since glycogen accumulation was impaired in skeletal muscle, its level in the liver was measured to determine whether thisorgan might have been compensating. As shown in Fig. 4B, the glycogenlevels in the livers of the null mutants were not significantlydifferent from those of the wild-typemice.

Glucose and insulin responsiveness in R_GL knockout mice. Since ablation of R_GL impairs glycogen accumulation in skeletal muscle, reportedly a major organ for glucose disposal, a criticalquestion was whether the R_GL null mutant animals were hyperglycemicand/or insulin resistant. Three approaches were taken to addressthis issue. First, blood glucose levels were measured in bothfasted and fed male and female mice of different ages. As shownin Fig. 5 and Table 1, the basal blood glucose levels for 14-to 18-week-old mice were, as expected, lower after overnight fasting,but no significant differences were detected between wild-typeand knockout mice, in either males or females. Similar resultswere obtained with animals 6 to 8 or 40 to 48 weeks old (not shown).Second, we evaluated the glucose and insulin tolerance after challengingwith a bolus of either glucose (2 mg/g) or insulin (1 U/kg). Thetime course of blood glucose clearance after glucose administrationwas indistinguishable between the wild-type and knockout mice(Fig. 5). Similarly, the blood glucose response to insulin treatmentwas the same in wild-type littermates and knockout animals. Againthese results were the same for males and females and for animalsof different ages and with a 129Sv background (not shown). Third,the basal and insulin-stimulated whole-body glucose disposal ineuglycemic hyperinsulinemic clamped conscious mice (30) wasvery similar in knockout and wild-type animals. In addition, nosignificant differences were observed in serum insulin, lactate,and triglyceride levels (Table 1).

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FIG. 5. Glucose and insulin tolerance tests. Glucose tolerance tests (GTT) were performed on 14- to 18-week-old 16-h-fasted, male and female wild-type (open circles) and R_GL null mutant (open squares) mice. Insulin tolerance tests (ITT) were performed a week later on the same mice except that they were fasted only for 6 h from 8:00 a.m. till 2:00 p.m. Six wild-type and eight null mutant males and four wild-type and 4 null mutant females were used.

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TABLE 1. Comparison of blood component levels in wild-type and R_GL knockout mice^a

Although the older mice had not demonstrated any obvious metabolic defects when fed a normal diet, we investigated the possibilitythat a high-fat diet could provoke abnormalities in glucose disposal.Both male and female, wild-type and knockout mice were subjectedfor a period of 20 weeks to a high-fat diet (Biosev) in which57% of the caloric intake is derived from fat. Body weight, bloodglucose levels, and food consumption were monitored weekly. Weightgain (~50%), increases in blood glucose levels (~30%), and foodintake (no significant increase) were not different between theknockout and wild-type littermate animals. Glucose and insulintolerance curves at the end of the feeding period were similarin both groups, although the response was blunted compared tothat before the high-fat diet, indicating that all animals hadbecome somewhat insulinresistant.

Insulin control of glycogen metabolism in R_GL knockout mice and wild-type littermates. Muscle PP1G has been postulated to play a key role in the insulin-induced activation of glycogen synthase. In order to addressthis crucial issue, wild-type and R_GL knockout mice were injectedintravenously with 2 U of insulin/kg for 5 min. Insulin treatmentresulted in a twofold activation of skeletal muscle GS in bothcontrol and R_GL-deficient mice (Fig. 6A), with no changes in glycogenPh (Fig. 6B). Glycogen content was also increased more than twofoldin the knockout mice (Fig. 7A). In absolute amount, the increasesin glycogen in wild-type and mutant mice were very similar. Inthe wild-type animals, the final level (including the relativelysmall increment) was not statistically significantly differentfrom the high initial level. It should be noted that such a shorttime of insulin stimulation would not cause large changes in glycogenaccumulation. Western immunoblotting also showed that insulintreatment increased the electrophoretic mobility of GS in muscleextracts from wild-type and R_GL-deficient mice, consistent withdephosphorylation of the protein (Fig. 6C). This finding confirmsthat the increase in GS activity was not due to carryover of allostericeffector G-6P from the extract into the assay (which involvesmore than 100-fold dilution). From these results, it is clearthat both GS and glycogen syntheses are still stimulated by insulinin the absence of R_GL. Even though R_GL was not required for insulinactivation of GS, we investigated whether it was phosphorylatedin response to the hormone. Western immunoblotting with phospho-specificantibodies against phosphorylated site 1 or site 2 (63) revealedthat the phosphorylation of neither was altered by insulin treatment,at times when GS was activated (Fig. 6D). Quantitation of blotsfrom five animals in each group gave values of 89.7 ± 9.2 (site1) or 88.1 ± 9.5 (site 2), expressed as a percentage of the non-insulin-treatedsamples normalized for total R_GL present.

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FIG. 6. GS and Ph activity in insulin-treated mice. (A and B) GS and Ph activity ratios were measured in skeletal muscle extracts as described in the legend to Fig. 3. The mice were treated with insulin (hatched bars) or not treated with insulin (open bars). Statistical significance was assessed by Student's t test (**, P < 0.01). The number of animals analyzed is shown inside the bars. (C) Muscle extracts from control and insulin-treated mice were immunoblotted with anti-GS antibodies. (D) Muscle extracts from wild-type mice, control and insulin treated, were immunoblotted with antibodies that specifically recognize R_GL phosphorylated at Ser48 (P-Ser48), R_GL phosphorylated at Ser67 (P-Ser67), or nondiscriminating antibodies (R_GL). Three representative independent samples per treatment are shown. +/+, wild type; $-$ / $-$ , R_GL null mutant mice.

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FIG. 7. Insulin-stimulated glycogen accumulation and GSK-3, PTG, and R6 levels in wild-type and R_GL knockout mice. (A) Glycogen content was measured as described in the legend to Fig. 4 in wild-type (+/+) and R_GL homozygous knockout ( $-$ / $-$ ) mice with (hatched bars) and without (open bars) insulin treatment. The number of experiments is indicated inside the bars. Statistical significance was assessed by Student's t test (*, P < 0.05). (B) Three representative samples from wild-type and R_GL knockout mice were analyzed by immunoblotting with antibodies against GSK-3 $beta$ , PTG, and R6. The numbers to the left show molecular size markers (in kilodattons).

Since the R_GL knockout mice responded normally to insulin stimulation, one possibility is altered expression of some of theother components of the insulin signaling pathway, such as GSK-3,or the other two known glycogen-associated PP1-binding proteins,PTG and R6. As shown in Fig. 7B, Western blot analyses indicatedthat the levels of PTG, R6, and GSK-3 $beta$ were unchanged in the knockoutanimals. It has also been reported that overexpression of R_GLin L6 cultured cells resulted in a twofold increase in insulin-stimulatedglucose transport (50). We therefore investigated whether theR_GL deficiency affected glucose uptake by in vitro analysis ofisolated hemidiaphragm muscles. The results revealed no differencesin basal and insulin-stimulated 2-deoxyglucose uptake betweenwild-type and knockout mice (Fig. 8).

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FIG. 8. Insulin stimulation of 2-deoxy[2-³H]glucose (2DG) uptake in hemidiaphragms from control and R_GL knockout mice. Hemidiaphragms were incubated at 37°C for 15 min with or without 250 mU of insulin per ml. The hemidiaphragms were then incubated with insulin (hatched bars) or without insulin (open bars) in medium containing 5 mM 2DG for 10 min. The results presented are the mean values ± SE of eight experiments. Statistical significance was assessed by Student's t test (*, P < 0.02).

Insulin-stimulated GS phosphatase activity in wild-type and R_GL knockout mice. If R_GL is not required for insulin activation of GS, some other mechanism must be operating. Activation of GS could resultfrom inhibition of protein kinase activity or activation of aGS phosphatase distinct from PP1G/R_GL. Decreased GSK-3 activity,by itself, cannot account for activation of GS (39), so we determinedwhether an insulin-stimulated phosphatase was present in R_GL knockoutmice. With Ph as a substrate, no increase in activity was detectedin either mutant mice or wild-type littermates (Fig. 9A). However,utilizing partially purified GS in an assay that couples dephosphorylationwith changes in the activity ratio (62), we detected a phosphataseactivity that was stimulated ~2-fold by insulin in both wild-typeand R_GL knockout mice (Fig. 9B). Not only is PP1G/R_GL dispensablefor insulin activation of GS, but a distinct insulin-activatedphosphatase is present in mouse skeletal muscle. This enzyme isnot PP2A, since it was detectable in the presence of 4 nM okadaicacid, conditions that completely inhibit 2A activity. The phosphataseis unlikely to be a divalent cation-requiring enzyme such as PP2Cor PP2B, because the extracts and the assays contained 2 mM EGTA.Thus, we believe that it is a type 1 form. It is also unlikelyto be the PTG-associated phosphatase, since this enzyme acts onPh as substrate (15), whereas the insulin-stimulated form appearsto be specific for GS.

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FIG. 9. Insulin-stimulated GS phosphatase. (A) Ph phosphatase in skeletal muscle extracts of non-insulin-treated (open bars) and insulin-treated (hatched bars) mice was measured as described in the legend to Fig. 4. (B) GS phosphatase was measured by the dephosphorylation-activation coupled assay as described in Materials and Methods. The results are expressed as the difference ( $Delta$ ) between the GS $-$ /+ G-6P activity ratios measured after 15 min of incubation of GS with tissue extract and that at zero time, normalized by protein concentration. Statistical significance was assessed by Student's t test (*, P < 0.05; **, P < 0.01). The number of animals analyzed is indicated inside the bars.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The most important outcome of this study is to demonstrate that R_GL is genetically linked to striated muscle glycogen accumulationbut is not essential for insulin control of glycogen metabolism.Analyses of the knockout mice demonstrate that R_GL directs phosphataseactivity towards glycogen-metabolizing enzymes since GS activityis reduced and Ph activity is enhanced in the null mutant mice.Correspondingly, muscle glycogen stores are significantly reducedto only 10% of those in wild-type animals. However, despite theimpaired glycogen accumulation, the animals remain normoglycemicand are insulinresponsive.

Animals homozygous for disruption of the R_GL gene have a substantial (60%) decrease in overall muscle C1 protein and PP1 activity,indicating that a phosphatase containing R_GL represents a significantproportion of the enzyme in skeletal muscle. Conversely, targetedoverexpression of R_GL in the skeletal muscle of mice resultedin an increase in the levels of C1 protein (22; Y. Suzuki andA. A. DePaoli-Roach, unpublished results). These observationsargue that the basal level of C1 protein depends on its associationwith regulatory subunits. Although the level of the protein canbe controlled at different stages, we favor a mechanism involvingstabilization of the protein. This hypothesis is supported bythe observation that overexpression of C1 in COS1 cells producesmostly insoluble protein associated with lysosomal structures,whereas coexpression with either R_GL or inhibitor 2 (data notshown) generates higher levels of soluble and active enzyme. Infact, the proposed chaperone function of the phosphatase inhibitor2 (3) most likely reflects a similar phenomenon whereby formationof a cytosolic form of PP1, the ATP-Mg-dependent phosphatase,also stabilizesC1.

Our results raise some critical questions about the role of muscle glycogen in blood glucose homeostasis (19, 56). Glycogendeposition in muscle is widely perceived to be the primary fateof ingested glucose. With this premise, one might have predictedthat animals impaired in their ability to accumulate glycogenin muscle would become hyperglycemic. This is not the case, suggestingthat other mechanisms for glucose homeostasis must be operating.One important consideration, however, is the degree to which studiesof mice are an accurate reflection of human metabolism and physiology,and we cannot exclude the possibility that skeletal muscle glycogenaccumulation in humans has a different impact on blood glucoselevels than in rodents. This caveat, of course, is valid for allof the numerous genetically altered mouse models that have recentlybeen constructed to probe insulin action and whole-body glucosemetabolism (for recent reviews see references 35 and 36).Shulman and colleagues (56) in fact have concluded that muscleglycogen is the predominant fate of ingested glucose in humans,at least under the conditions of hyperglycemic hyperinsulinemicclamps, and that impaired glycogen synthesis correlates with type2 diabetes. They are also of the opinion that glucose transportis the rate-limiting step for glycogen accumulation, which isdefective in the diabetic condition. The R_GL knockout mice, however,have normal basal and insulin-stimulated glucose transport butreduced glycogen content supporting the view that the glycogen-metabolizingenzymes play critical roles in glycogen accumulation (8, 39).It will be interesting to examine mouse models in which muscleglycogen accumulation is completely defective or in which insulingsignaling to GS is specifically ablated. For example, geneticelimination of the novel insulin-stimulated GS phosphatase describedin this work might achieve the lattergoal.

Glucose is not being accumulated as excess fat, since lean and fat masses as determined by dexascan are similar in wild-typeand R_GL knockout mice, as is the respiratory quotient (VCO₂/VO₂)over a 24-h period (data not shown). Liver glycogen is not elevated,so the liver is not compensating. Since food consumption is nodifferent between wild-type and R_GL null animals, a simplisticquestion relates to the fate of the ingested calories. However,the apparent paradox is minimized if one considers that the caloricequivalent of the muscle glycogen in the mouse is less than 2%of a daily ~15-kcal intake, based on a glycogen content of 2.5mg/g for a 25-g mouse. Therefore, muscle glycogen in mice doesnot actually represent a significant caloric reserve comparedto food consumption. Glycogen is continuously used for local contractileactivity and is replaced by incoming glucose, directly after meals,or indirectly from the liver via glycogenolysis or gluconeogenesisduring fasting. The R_GL null mutant mice appear to have a lowerglycogen set point, consistent with GS being inactivated and Phactivated. As demonstrated by the normal basal and insulin-stimulated2-deoxyglucose uptake, glucose enters the cells normally and presumablyis stored as glycogen. However, hyperactive Ph may cause rapiddegradation, resulting in a lower steady-state glycogen concentration.Thus, insulin stimulation promotes glucose uptake normally inthe R_GL knockout mice, and the overall lower glycogen contentis most likely due to the altered activities of GS and/orPh.

The studies with the R_GL-deficient mice clearly show that the muscle-specific PP1G, although important for basal glycogenaccumulation, is dispensable for insulin-induced activation ofGS. Together with our finding of an insulin-stimulated phosphataseboth in the knockout and wild-type animals, there is compellingevidence that an enzyme distinct from PP1G/R_GL is responsiblefor activation of GS. Thus, the mechanism of an insulin-inducedphosphorylation of R_GL and activation of the associated phosphatasecan be discounted, consistent with a recent report (63) thatin rat skeletal muscle phosphorylation of Ser48 is not increasedin response to insulin. Furthermore, since our initial communication(22) that GS was activated by insulin in R_GL-deficient mice,other reports argue against a role for R_GL in insulin controlof glycogen metabolism (43, 66). Our studies are not in agreementwith the report that overexpression or depletion of R_GL in L6cells affected activation of GS and glucose uptake by insulin(50). The observation that neither insulin activation of GSnor basal or insulin-stimulated glucose uptake is altered in theR_GL null mice indicates that PP1G is not involved in regulationof glucose transport. Rasmussen et al. (51) were also unableto reproduce the effect of overexpressed R_GL protein on glucosetransport.

Recently it has been proposed that R_GL acts as a scaffold that binds both GS and C1 and that this association is requiredfor GS activation and for $beta$ -adrenergic control of GS (42). Ouranimal studies show that activation of GS can occur in the absenceof R_GL, indicating that association with R_GL is not essentialfor control of GS activity in vivo. Furthermore, even in the R_GLnull mutant muscle, all the GS is still bound to glycogen implyingthat R_GL is not needed for thisassociation.

The work presented suggests that a phosphatase distinct from PP1G/R_GL mediates insulin activation of GS. Although the identityof this insulin-stimulated phosphatase is not known, it is likelyto be a novel enzyme. We can exclude the possibility that it isa type 2A, 2B, or 2C enzyme, since it was detected in the presenceof 4 nM okadaic acid and 2 mM EGTA, conditions that would inhibitthe activity of those forms. Preliminary data indicate that thephosphatase activity was not detectable in the presence of 200nM okadaic acid, suggesting that it is a type 1 enzyme. Obviouscandidates would be enzymes containing the other two glycogen-bindingsubunits, PTG and R6. No regulatory mechanisms for these proteinshave been identified so far. Overexpression of PTG increased bothbasal and insulin-stimulated GS activity (49). However, we considerit unlikely that the insulin-stimulated phosphatase activity wedetected is associated with PTG or R6, because their expressionis not restricted to insulin-responsive tissues. In addition andmost importantly, insulin was shown to stimulate the PTG phosphataseactivity towards Ph (15), whereas the insulin-stimulated phosphatasewe identified appears to be specific for GS. Insulin does notaffect phosphorylase activity, consistent with the inability todetect stimulation of phosphatase activity towards Ph (Fig. 9).Neither PTG nor R6 functionally compensates for the loss of R_GL,since loss of R_GL results in low basal muscle glycogen storageand PTG and R6 protein levels are not upregulated in the knockoutmice. The implication is that the various glycogen-associatedphosphatases are not redundant, even though PTG and R6 are presentin skeletal muscle at ~10% of the level of R_GL (37, 60). Therefore,the insulin-stimulated protein phosphatase may be a form of PP1,involving association of C1 with some other regulatory subunit,either novel or already known in some othercontext.

Several studies over the last few years have attempted to link mutations in the human R_GL (PPP1R3) gene with type 2 diabetes.However, the frequency of the initially reported polymorphismat codon 905 (29) was shown to be identical in normal and diabeticpopulations. More recently, adenovirus-mediated expression ofAsp905 and Tyr905 human R_GL in L6 cells indicated no differencesin glycogen synthesis (51). Another substitution at codon 883and a variant in an ATTTA motif in the 3' untranslated regionof the human R_GL gene have also been found (66). Polymorphismsin the ATTTA element appear to correlate with lower expressionof the protein, insulin resistance, and type 2 diabetes (65).At least on the basis of our studies showing that mice lackingR_GL are neither diabetic nor insulin resistant, one might questionwhether subtle modifications of the human protein would causean aberrant phenotype. Most notably, the small reduction in thelevel of R_GL observed in subjects carrying the ATTTA spacing polymorphismis unlikely to be responsible for the defective insulin responsesassociated with diabetes. Similarly, it is not likely that putativealterations of R_GL function in the other coding variants are criticallyinvolved in the etiology of type 2diabetes.

If R_GL is not required for insulin activation of GS or glucose transport, a key question is whether it is involved in otherregulatory processes. Is it necessary or involved in the $beta$ -adrenergiccontrol of glycogen metabolism? A main function of glycogen inskeletal muscle is to provide fuel for contraction. Since theglycogen content is extremely low in the R_GL knockout mice, onecan ask whether these animals will be able to sustain exerciseand whether R_GL is involved in the neuronal activation of GS,such as occurs during contraction and exercise. R_GL has also beenproposed to control $beta$ -adrenergic-induced phosphorylation of phospholambanin heart (45, 63). Since this phosphorylation reduces theinhibitory effect of phospholamban on the sarcoplasmic reticulum-associatedCa²⁺-ATPase (34), it may be that the R_GL knockout mice have an increasedcardiac performance, a phenotype observed in the phospholambannull mice (44). Work is in progress to address these importantand interestingquestions.

	ACKNOWLEDGMENTS

This work was supported in part by National Institutes of Health Grant DK36569 and by a research grant from the American DiabetesAssociation.

We thank Suzanne Baugh and Paula Ladd for their technical assistance in some of the work presented. We are indebted to DavidA. Williams and Cheryl Bock for generating the R_GL chimeric mice.We are grateful to Alain Baron (Amylin San Diego, Calif.) andMark Heiman (Eli Lilly Co.) for performing glucose clamping anddetermining body composition and metabolic rates, respectively.We thank Alan Saltiel (Pfizer Global Research and Development),Patricia Cohen and Philip Cohen (University of Dundee) for theirgenerous gifts of PTG, R6, and phospho-R_GL antibodies, respectively.We are particularly grateful to Peter J. Roach and Robert A. Harrisfor discussion of the work and for criticism of themanuscript.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Biochemistry and Molecular Biology, Indiana University School of Medicine,635 Barnhill Dr., Indianapolis, IN 46202-5122. Phone: (317) 274-1585.Fax: (317) 274-4686. E-mail: adepaoli{at}iupui.edu.

Present address: Department of Medical Genetics, Tohoku University School of Medicine, Sendai 980-77,Japan.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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