Phosphoenolpyruvate Carboxykinase Is Necessary for the Integration of Hepatic Energy Metabolism

doi:10.1128/MCB.20.17.6508-6517.2000

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Molecular and Cellular Biology, September 2000, p. 6508-6517, Vol. 20, No. 17
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Phosphoenolpyruvate Carboxykinase Is Necessary for the Integration of Hepatic Energy Metabolism

Pengxiang She, Masakazu Shiota, Kathy D. Shelton, Roger Chalkley, Catherine Postic, and Mark A. Magnuson^*

Department of Molecular Physiology and Biophysics, Vanderbilt University School of Medicine, Nashville, Tennessee 37232

Received 29 March 2000/Accepted 5 May 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

We used an allelogenic Cre/loxP gene targeting strategy in mice to determine the role of cytosolic phosphoenolpyruvate carboxykinase(PEPCK) in hepatic energy metabolism. Mice that lack this enzymedie within 3 days of birth, while mice with at least a 90% globalreduction of PEPCK, or a liver-specific knockout of PEPCK, areviable. Surprisingly, in both cases these animals remain euglycemicafter a 24-h fast. However, mice without hepatic PEPCK develophepatic steatosis after fasting despite up-regulation of a varietyof genes encoding free fatty acid-oxidizing enzymes. Also, markedalterations in the expression of hepatic genes involved in energymetabolism occur in the absence of any changes in plasma hormoneconcentrations. Given that a ninefold elevation of the hepaticmalate concentration occurs in the liver-specific PEPCK knockoutmice, we suggest that one or more intermediary metabolites maydirectly regulate expression of the affected genes. Thus, hepaticPEPCK may function more as an integrator of hepatic energy metabolismthan as a determinant ofgluconeogenesis.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Gluconeogenesis is the process whereby glucose is formed from noncarbohydrate metabolic substrates such as lactate and alanine.This metabolic pathway occurs predominately in the liver and kidneyand is essential for the production of glucose during extendedfasting when glycogen stores have been depleted (18, 23).A key step in gluconeogenesis is the formation of phosphoenolpyruvatefrom oxaloacetate, which is catalyzed by phosphoenolpyruvate carboxykinase(PEPCK). This reaction has long been thought to be essential forgluconeogenesis since it bypasses the thermodynamically unfavorableconversion of pyruvate to phosphoenolpyruvate by pyruvate kinase(20). Although both a cytosolic and a mitochondrial isoformof PEPCK are expressed in rodents, the cytosolic isoform accountsfor over 95% of the activity in the liver and kidney (30, 45).

Several lines of evidence have led to the widely held notion that PEPCK is the rate-determining step in hepatic and renalgluconeogenesis. First, the cytosolic isoform of PEPCK is adaptivelyregulated at the transcriptional level in a manner that correlateswith alterations in gluconeogenic flux (5, 12, 25, 47).Second, treatment of fasted animals with 3-mercaptopicolinic acid,a PEPCK inhibitor, causes hypoglycemia (8). Third, overexpressionof PEPCK in both cell lines and transgenic mice causes eitherincreased gluconeogenesis or hyperglycemia (37, 44). However,other data suggest that gluconeogenic flux is determined by alterationsin activities of multiple enzymes, not just PEPCK. Indeed, inone study both pyruvate carboxylase and pyruvate kinase were suggestedto play a greater role in determining gluconeogenic flux in isolatedrat hepatocytes than PEPCK (13). Also, results of a perfusedrat liver study indicated that pyruvate carboxylase rather thanPEPCK is a primary rate-determining step for gluconeogenesis (10).

Energy metabolism in the liver involves the interconversion of carbohydrates, lipids, and amino acids. The pathways involvedare regulated by multiple mechanisms. First, allosteric effectorsor covalent modifications affect the activity of certain enzymes.Second, substrate availability itself may play an essential role.Third, hormones and other extrahepatic effectors regulate theexpression of genes encoding various enzymes. However, the mechanismsthat regulate flux between different pathways have not been thoroughlyelucidated. Since PEPCK catalyzes a reaction near the intersectionof several fundamentally important pathways, the absence of thisenzyme might have unpredictable effects on the accumulation ofspecific metabolites. Moreover, excess hepatic glucose productionis a major factor contributing to fasting hyperglycemia in bothtype 1 and type 2 diabetes mellitus (6, 7). Thus, knowledgeof how gluconeogenesis is regulated is of both fundamental andclinicalimportance.

To gain greater insights into the role of PEPCK in both gluconeogenesis and hepatic energy metabolism, we used an allelogenicCre/loxP gene targeting strategy to generate mice that had variabledegrees of impaired PEPCK gene expression. In addition, by intercrossingmice with a conditional PEPCK gene locus with a line of albumin(Alb)-cre transgenic animals, we were also able to produce micewith a liver-specific PEPCK gene knockout. Studies of these miceindicate that while PEPCK has a much lower than expected effecton gluconeogenesis, the enzyme plays an unexpected role in integratingmetabolic pathways in theliver.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Targeting vector. The targeting vector shown in Fig. 1A contains a phosphoglycerol kinase (pgk)-neomycin resistance (neo) gene cassette, a pgk-herpessimplex virus type 1 thymidine kinase (tk) gene cassette, andthree loxP sites. The vector was assembled in pNTK(A) using loxPsites from pBS246 (39) and mouse PEPCK gene fragments isolatedfrom a 129/SvJ Bac genomic DNA clone (46). The long arm of thetargeting vector, a 6-kb KpnI fragment, was ligated into the ClaIsite of pBS.LP, thereby forming BSLP.PEPCK.LA. A 1-kb excisableKpnI DNA fragment containing exons 4 and 5 was ligated into theClaI site of pNTK(A), thereby forming mPEP.B3. The short arm ofthe targeting vector was a 2.1-kb KpnI/XbaI fragment that wasligated into the BamHI site of mPEP.B3, forming mPEP.K2. Afterdestroying a SalI site in mPEP.K2, the 6-kb SalI fragment of BSLP.PEPCK.LAwas cloned into the remaining SalI site of mPEP.K2, creating thefinal construct, mPEPCK.KO2. The correct assembly of mPEPCK.KO2was confirmed by DNA sequencing.

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FIG. 1. pck alleles generated by gene targeting and Cre-mediated recombination. (A) Top, partial map of the pck^w allele. Exons are indicated as solid rectangles. The location of the DNA fragment used as the Southern hybridization probe is shown. Middle, map of the PEPCK gene targeting vector. The vector contains a pgk-neo cassette, a pgk-tk cassette, and three loxP sites (triangles). Two of the loxP sites flank neo, and the third is located between exons 4 and 5 in the PEPCK gene. The pck^lox+neo allele was generated by homologous recombination (HR) in ES cells. Bottom, the pck^lox and pck^del alleles, derived from pck^lox+neo by Cre-mediated recombination. Exons 4 and 5 and neo were excised by Cre microinjection of single-cell pck^lox+neo/w embryos. (B and C) PCR genotype analysis. Tail DNA was amplified by both primer pair W (5'-TCTGTCAGTTCAATACCAATCT-3'), 5'-AATGTTCTCTGCAAGTCCTGGTG-3') and primer pair D (5'-ATCAGCTTTAGTCGTCTCTGGT-3', 5'-AATGTTCTCTGCAAGTCCTGGTG-3') or primer pair F (5'-TCTGTCAGTTCAATACCAATCT-3', 5'-AGCCTCTGTTCCACATACACTTCA-3'. The amplified alleles and their sizes are shown on the right and left, respectively. (D) Western blot analysis of liver homogenates from pck^w/w (lane 1), pck^del/w (lane 2), and pck^del/del (lane 3) mice.

Gene targeting and production of chimeras. Fifty micrograms of the targeting vector was linearized with NotI and then electroporated into 5 × 10⁷ TL-1 embryonic cells (ES) cells, which were derived from 129/SvEvTacmice (22). Southern blot analysis of several clones resistantto both G418 and ganciclovir revealed one clone, 2D7, that hadundergone the desired recombination event (data not shown). TheES cell clone was microinjected into C57BL/6 blastocysts, whichwere then implanted into pseudopregnant female recipients to producechimeras. Germ line transmission of the targeted pck^lox+neo allele was confirmed by Southern blotting and PCR analysis (datanotshown).

Conversion of the pck^lox+neo allele to a pck^lox or pck^del allele. The pck^lox+neo allele was converted to both a pck^lox and a pck^del allele by pronuclear microinjection of supercoiled pBS185 (39), a cytomegalovirus-Creexpression plasmid, into single-cell mouse embryos derived frommating pck^lox+neo males with superovulated B6D2 F₁ hybrid female (1, 35).

Genotype analysis. Four different pck alleles (pck^w, pck^lox+neo, pck^lox, and pck^del [w and del denote wild type and deletion, respectively]) were routinelydistinguished by PCR analysis (Fig. 1B and C). pck^w and pck^lox were detected using primers 5'-TCTGTCAGTTCAATACCAATCT-3' and5'-AATGTTCTCTGCAAGTCCTGGTG-3'. A 518-bp fragment was generatedfrom pck^w, and a 620-bp fragment was generated from pck^lox. For the pck^lox+neo allele, a 360-bp fragment was amplified using 5'-TCTGTCAGTTCAATACCAATCT-3'and 5'-AGCCTCTGTTCCACATACACTTCA-3'. The pck^del allele was detected as a 815-bp fragment using primers 5'-ATCAGCTTTAGTCGTCTCTGGT-3'and 5'-AATGTTCTCTGCAAGTCCTGGTG-3'. The Alb-cre transgene (35)was detected by PCR with primers 5'-ACCTGAAGATGTTCGCGATTATCT-3'and 5'-ACCGTCAGTACGTGAGATATCTT-3', which yielded a 370-bpfragment.

Animals. All mice were specific pathogen free, maintained on a 12-h light-dark cycle, and fed a standard rodent chow (Purina Mills,Inc., St. Louis, Mo.). Treatment and housing of animals met guidelinesof the American Association for the Accreditation of LaboratoryAnimal Care, and the protocols were approved by the VanderbiltInstitutional Animal Care and UseCommittee.

Northern blot analysis. Total RNA was isolated using TRIzol (Life Technologies, Inc., Grand Island, N.Y.). Northern blot analysis was performed aspreviously described (28). The PEPCK probe was a 569-bp HindIII-EcoRIfragment spanning exons 1 to 4 of the mouse cDNA. cDNA clonesfor rat CYP4A1, rat CYP4A1, and mouse medium-chain fatty acylcoenzyme A (acyl-CoA) dehydrogenase were provided D. Kelly (Departmentof Internal Medicine, Washington University). Probes for pyruvatecarboxylase, fructose-1,6-bisphosphatase, and glucose-6-phosphatasewere prepared from human, pig, and rat cDNA clones, respectively.Probes (numbers in parentheses are those of the IMAGE consortiumclones from which clones were prepared) for malonyl-CoA decarboxylase(692290), very long-chain fatty acyl-CoA dehydrogenase (2236538),long-chain fatty acyl-CoA dehydrogenase (2225775), acyl-CoA oxidase(1972335), carnitine octanoyltransferase (1451465), carnitineacetyltransferase (1889414), and enoyl- CoA hydratase-L-3-hydroxyacyl-CoAdehydrogenase bifunctional protein (2076790), cytosolic (2064729)and mitochondrial (1972463) aspartate aminotransferase, cytosolic(329958) and mitochondrial (2192286) malate dehydrogenase, citratesynthase (335882), isocitrate dehydrogenase (2136389), succinyl-CoAsynthetase (2099765), lactate dehydrogenase (1451692), alanineaminotransferase (1886916), and glyceraldehyde-3-phosphate dehydrogenase(716832) were obtained from Research Genetics, Inc., Huntsville,Ala., and verified by DNA sequencing prior to use. The relativeabundance of each mRNA was corrected for loading differences,using cyclophilin cDNA as a controlprobe.

PEPCK activity measurements and Western blot analysis. PEPCK activity was measured using an NADH-coupled system to quantitate the conversion of phosphoenolpyruvate into oxaloacetateand subsequent conversion to malate (45). All assays were performedwithin 3 h of removal of tissue from the animal. Activity wasexpressed as milliunits per milligram of protein in liver supernatant(1 mU = 1 nmol of oxaloacetate produced/min). The protein contentwas determined using a Bradford assay kit (Bio-Rad, Hercules,Calif.), with bovine serum albumin as a standard. Western blotanalysis was performed as previously described (16). A sheepanti-PEPCK antiserum (a gift from D. K. Granner, Vanderbilt University)was used at a 1:5,000dilution.

In vivo glucose kinetics. Glucose turnover rates and gluconeogenic index in the form of plasma [¹⁴C]glucose specific activity derived from [¹⁴C]lactate were measured as previously described (29), usingmice in which both jugular and carotid catheters had been surgicallyimplanted 5 days prior to study. The experimental protocol involveddepriving animals of food for 26 h, followed by an experimentalperiod of 220 min, which consisted both of a 100-min equilibrationperiod ( $-$ 100 to 0 min) and a 120-min experiment period. Basalglucose turnover and gluconeogenic index were determined by 2-µCibolus injection and constant infusion at 0.5 µCi/min of high-pressureliquid chromatography-purified [3-³H]glucose (NEN Life Science Products, Boston, Mass.) for 220 minand constant infusion at 0.1 µCi/min of [U-¹⁴C]lactate (NEN Life Science Products) for 120 min beginning at0 min. Blood samples were withdrawn from a carotid artery catheterat $-$ 30, 0, 30, 60, 90, and 120 min. Liquid chromatography wasused to purify radioactive glucose in plasma. The samples weredeproteinized by passage through a 9- by 190-mm column filledwith 14-µm sulfonate polystyrene cation-exchange resin (BensonBH-4, Reno, Nev.) at a flow rate 2.2 ml/min.

Endurance exercise study. Male mice that had been fasted for 24 h were acclimated to a treadmill for 2 min each at 13.4 and 16.1 meters/min and thenrun to exhaustion at 18.8 meters/min. Blood glucose concentrationwas measured with a Hemocue (Mission Viejo, Calif.) glucose meterimmediately before, at 30 min, and at the end of theexercise.

Analytical procedures. Plasma insulin, glucagon, and corticosterone concentrations were determined by radioimmunoassay using a rat insulin kit (LincoResearch, St. Louis, Mo.), a rat glucagon kit (Linco Research),and a Coat-A-Count rat corticosterone kit (DPC, Los Angeles, Calif.),respectively. Plasma free fatty acid (FFA) concentrations weremeasured with a NEFA C kit (Wako Pure Chemical Industries, Osaka,Japan). Plasma triglyceride concentrations were measured usinga colorimetric kit (Sigma, St. Louis, Mo.). Plasma glucose, lactate,glycerol, $beta$ -hydroxybutyrate (BHBA), and hepatic malate concentrationswere determined by enzymatic assays using microassay procedures(3). Hepatic glycogen and triglyceride contents were analyzedas described elsewhere (3, 40). All results are presentedas the mean ± standard error of the mean. Statistical significancewas determined by one-way analysis of variance. P values of lessthan 0.05 were considered statisticallysignificant.

Nucleotide sequence accession number. The sequences altered in the pck^lox allele were deposited in GenBank (accession number AF220498).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Targeting of the mouse pck gene. We designed a Cre/loxP gene targeting strategy that allowed the creation of three different alleles of the pck gene from asingle gene targeting event in ES cells (Fig. 1A). The parentalpck^lox+neo allele contains three loxP sites and a neo cassette. Two of theloxP sites flank a pgk-neo cassette which is located between exons3 and 4, whereas a third loxP site lies downstream of exon 5.After its introduction into mice, the pck^lox+neo allele was further modified by Cre-mediated recombination insingle-cell pck^lox+neo embryos. Partial recombination yielded a conditional allele (pck^lox) that lacks neo but retains two loxP sites flanking exons 4 and5. Complete recombination produced a null pck allele (pck^del) that contains a single loxP site and lacks exons 4 and 5. Thegeneration of each allele was confirmed by both PCR (Fig. 1B andC) and Southern blot analysis (data notshown).

Interbreeding of animals that were heterozygous for either the pck^lox+neo or pck^lox allele yielded mice that were homozygous for each of these twoalleles. In both cases the mice were viable, thereby enablingPEPCK activity and protein content to be determined from boththe liver and kidney after a 24-h fast. PEPCK activity and proteinamount in the pck^lox/lox mice did not differ significantly from those of wild-type mice(Fig. 2A and B). In contrast, PEPCK activity and protein massin pck^{lox+neo/lox+neo} mice, which contains a neo cassette between exons 3 and 4, wasreduced to about ~10 and 20% of normal in the liver and kidney,respectively (Fig. 2A and B). Thus, the pck^lox+neo allele is functionally attenuated, presumably due to interferencewith normal RNA processing as been observed in other genes thatretain a neo cassette within an intron (27). Plasma glucoseconcentrations in fed and 24-h-fasted mice that were homozygousfor the pck^lox+neo allele did not differ from those in mice with two pck^w alleles (Fig. 2C). However, the relative liver mass in pck^{lox+neo/lox+neo} mice after a 24-h fast was increased by 30% (5.6% ± 0.4% versus4.3% ± 0.1% of body weight for wild-type mice, P < 0.004, n =8 to 10). Content of malate, a tricarboxylic acid (TCA) cycleintermediate, in fasting mice was 5.4-fold greater in the liver(1.57 ± 0.21 versus 0.29 ± 0.01 µM/g, P < 0.001, n = 6 to 7) and2.4-fold greater in the kidney (0.36 ± 0.04 versus 0.15 ± 0.01µM/g, P < 0.001, n = 6 to 7) of pck^{lox+neo/lox+neo} mice than in wild-type mice. Plasma FFA concentrations in 24-h-fastedpck^{lox+neo/lox+neo} mice were not different from that in control mice (1,345 ± 123versus 1161 ± 74 µEq/liter n = 7 to 9).

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FIG. 2. Analysis of PEPCK expression in mice that are homozygous for the pck^lox+neo and pck^lox alleles and that are compound heterozygotes of pck^lox+neo and pck^del alleles. (A) Hepatic and renal PEPCK activity in pck^{lox+neo/lox+neo} and pck^lox/lox mice fasted for 24 h. ***, P < 0.001, n = 4. (B) Western blot analysis of liver and kidney tissues from 24-h-fasted mice. Lanes 1, 2, and 3 represent pck^w/w, pck^{lox+neo/lox+neo}, and pck^lox/lox mice, respectively. (C) Plasma glucose concentration in pck^{lox+neo/lox+neo} and pck^lox+neo/del mice at fed and 24-fasted states (n = 7 to 9). (D) Northern blot analysis of liver, kidney, and brown and white adipose tissues (BAT and WAT) from 24-h-fasted mice. Lanes 1 and 2 represent pck^w/w and pck^lox+neo/del mice, respectively. cyclo., cyclophilin.

Characterization of pck null pups. Mice that were homozygous null for PEPCK (i.e., pck^del/del) were obtained by interbreeding of pck^del/w mice. Genotype analysis of 97 1-day-old pups revealed 22 pck^w/w (22.7%), 49 pck^del/w (50.5%), and 26 pck^del/del mice (26.8%), consistent with Mendelian inheritance. Westernblot analysis of liver extracts confirmed the absence of PEPCKin pck^del/del mice. PEPCK protein content was decreased by approximately one-halfin pck^del/w pups, indicating the lack of any significant compensatory changesin gene transcription (Fig. 1D). All pck^del/del pups died within 3 days of birth, mostly at days 2 and 3. Priorto becoming moribund, pck^del/del pups became lethargic and pale and were smaller than heterozygousnull or normal littermates. Necropsy of the dead pck^del/del pups revealed empty stomachs and palelivers.

One-day-old pck^del/del mice were markedly hypoglycemic, with plasma glucose concentrations of 32 ± 7 mg/dl compared to control valuesof 90.3 ± 7.9 mg/dl. FFA concentrations were ~2-fold greater inpck^del/del pups, but plasma lactate concentrations were unchanged (Table1). Hepatic glycogen content in pck^del/del pups was only 38% of that in wild-type pups, although hepaticglycogen content of fetuses removed at embryonic day 20 did notdiffer among the three genotypes (553 ± 11 µM/g in pck^w/w pups, 594 ± 26 in pck^del/w pups, and 551 ± 24 in pck^del/del pups, n = 3 to 6) and, in all cases, was greater than in postnatalday 1 (P1) pups (P < 0.001). Hepatic malate concentration was10-fold greater in livers of the pck^del/del pups than in those of wild-type pups (Table 1). While the malateconcentration was increased in the pck^del/w pups, although to a lesser degree, there were no differencesin the plasma glucose, FFA, lactate, and hepatic glycogen concentrationsof these animals compared to pck^w/w pups (Table 1).

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TABLE 1. Plasma and hepatic metabolites in 1-day-old pck^del/del and pck^del/w pups^a

PEPCK mRNA abundance was decreased by 42 and 33% in liver and brown adipose tissue of pck^del/w pups (P < 0.01, n = 4), respectively, compared to wild-type pups.Consistent with prior studies of the developmental expressionof PEPCK (41), PEPCK mRNA in kidneys of 1-day-old pups was notdetected by Northern blot analysis for either wild-type or knockoutpups (data not shown). The body weight of pck^del/del pups was 6.8% less than that of pck^w/w pups at P1 (P < 0.05).

Adult heterozygous pck null mice. To assess the impact of the loss of one functional pck allele, we performed further studies on 8- to 10-week-old animals thatwere heterozygous null for PEPCK (pck^del/w). Hepatic PEPCK activities of fed and 24-h-fasted pck^del/w mice were 60 and 52%, respectively, of that of control animals(Table 2), indicating that a single functional pck allele inliver was only minimally capable of compensating for the lossof the second allele. Similarly, renal PEPCK activity in pck^del/w mice was approximately two-thirds of control level at both fed(7.4 ± 1.0 versus 10.6 ± 0.8 mU/mg of protein, P < 0.04, n = 4)and 24-h-fasted (23.2 ± 0.9 versus 39.4 ± 4.1 mU/mg of protein,P < 0.01, n = 4) states. Mitochondrial PEPCK activity in the liverwas less than 2% of the total PEPCK activity and did not differbetween pck^del/w and pck^w/w mice (data not shown). PEPCK mRNA abundance was decreased by35% in liver and by 33% in kidney in 24-h-fasted mice (data notshown). However, plasma glucose concentrations did not differat either fed or fasted states (Table 2). Both hepatic (Table2) and muscle (data not shown) glycogen contents were also similar.No significant differences were found in plasma FFA, BHBA, lactate,insulin, and hepatic malate concentrations between the two genotypesat both fed and fasted states (Table 2).

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TABLE 2. Plasma insulin concentration, plasma and hepatic metabolite concentrations, and hepatic PEPCK activity in fed and 24-h-fasted pck^del/w and pck^w/w mice^a

Characterization of compound heterozygotes. Given the lack of any effect of fasting on the plasma glucose concentration in either the pck^{lox+neo/lox+neo} or pck^del/w mice, we proceeded to intercross pck^{lox+neo/lox+neo} mice with pck^del/w mice. By doing so, we produced compound heterozygotes (pck^lox+neo/del) that had 95, 90, and almost 100% reductions of PEPCK gene expressionin liver, kidney, and adipose tissues, respectively, as judgedNorthern blot analysis (Fig. 2D). Plasma glucose concentrationsin both fed and 24-h-fasted mice were no different from thosein wild-type mice (Fig. 2C). However, in this case the relativeliver mass in pck^lox+neo/del mice after a 24-h fast was increased by 65% (7.1% ± 0.1% of bodyweight) and their livers were pale atnecropsy.

Liver-specific knockout of PEPCK. Since liver is the major site of gluconeogenesis, we proceeded to generate liver-specific PEPCK knockout (i.e., pck^lox/lox+Alb-cre) mice by mating pck^lox/lox with animals that express cre in the liver under control of thealbumin promoter. Genotype analysis of 126 mice at weaning revealedfrequencies of 72 pck^lox/lox mice and 54 pck^lox/lox+Alb-cre mice (P < 0.11 according to chi-square test). Southernblot analysis of tissue DNA from 6-week-old pck^lox/lox+Alb-cre mice showed over 80% conversion of the pck^lox to pck^del allele in the liver, with no sign of recombination in other tissues(data not shown), consistent with previous studies (35). Tofurther assess the efficiency of recombination within hepatocytes,both Western and Northern blot analyses were performed. PEPCKmRNA and protein amounts in 6-week-old pck^lox/lox+Alb-cre mice were markedly reduced (Fig. 3), cytosolic PEPCKactivity was undetectable, and mitochondrial PEPCK activity wasnot altered (data not shown). PEPCK mRNA abundance in kidney andbrown adipose tissues of pck^lox/lox+Alb-cre mice was unaffected (Fig. 3A). The small amount of residualPEPCK protein and mRNA detected in the livers of adult animalsby both of these assays is likely due to a nonhepatocyte source,since a previous study of the Alb-cre mice showed them to confercomplete recombination by 6 to 8 weeks of age (35). However,recombination using this transgene was age dependent since PEPCKprotein levels decreased only by ~70 and ~80% at 1 and 7 daysafter birth, respectively, in pck^lox/lox+Alb-cre mice (data not shown).

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FIG. 3. Liver-specific recombination in pck^lox/lox+Alb-cre (lanes 1) and pck^lox/lox (lanes 2) mice. (A) Northern blot analysis of overnight-fasted 5- to 6-week-old mice; BAT, brown adipose tissue; cyclo., cyclophilin. (B) Western blot analysis of liver tissue from overnight-fasted mice.

Euglycemia in liver-specific PEPCK knockout mice at rest. Plasma glucose concentrations in pck^lox/lox+Alb-cre mice at both fed and fasted states were not different from those in pck^lox/lox control mice (Table 3). However, fed (postabsorptive) hepaticglycogen content in the livers of PEPCK knockout mice was only56% of the level in control mice, and glycogen was depleted completelyin 24-h-fasted animals (Table 3). Plasma concentrations of thegluconeogenic substrates, lactate and glycerol, did not differbetween the two genotypes, while fasting plasma alanine concentrationwas increased by 25% in pck^lox/lox+Alb-cre mice.

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TABLE 3. Body and liver weight, plasma hormone concentrations, and plasma and hepatic metabolite concentrations in fed and 24-h-fasted pck^lox/lox and pck^lox/lox+Alb-cre mice^a

Given the normal plasma glucose concentrations in pck^lox/lox+Alb-cre mice after fasting, we measured concentrations of plasma hormonesinvolving regulation of energy metabolism (Table 3). Both fedand fasting insulin concentrations were not different betweenthe two genotypes, nor were the fasting glucagon and corticosteroneconcentrations, despite hepatic malate concentrations that wereincreased 5.5- and 9-fold at the fed and fasted states, respectively,in pck^lox/lox+Alb-cre mice (Table 3).

The plasma glucose concentration in pck^lox/lox+Alb-cre pups was less than that in pck^lox/lox pups at P1 (31.7 ± 4.6 versus 62.3 ± 3.1 mg/dl, n = 8 to 14,P < 0.0001). However, plasma glucose concentrations did not differbetween the two genotypes at P3 and P7 (data not shown). Hepaticglycogen content in pck^lox/lox+Alb-cre pups was decreased by 50% at P1 and by 85% at P3 (datanotshown).

To further determine the effect of the lack of hepatic PEPCK on whole body glucose metabolism, we performed a study of basalglucose kinetics in 26-h-fasted pck^lox/lox+Alb-cre mice. During the entire 220-min experimental period,plasma glucose concentrations in the liver-specific PEPCK knockoutmice did not differ from the control values. The [3-³H]glucose-measured glucose turnover rate and specific activityof plasma [¹⁴C]glucose were also not different (Table 4).

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TABLE 4. Basal glucose kinetics in pck^lox/lox pck^lox/lox+Alb-cre mice after a 26-h fast^a

Since pck^lox/lox+Alb-cre mice are able to maintain normal glucose metabolism at rest, we tested their response to exercise, a maneuverthat increases peripheral glucose utilization. At 30 min and atthe end of the exercise, blood glucose concentrations in the knockoutmice fell to approximately half of the level in controls (Fig.4). While the exercise endurance time between the two genotypesdid not reach the defined statistically significant level (50.6± 7.3 versus 71.4 ± 6.8, P < 0.07, n = 5), the animals lackinghepatic PEPCK appeared to be less tolerant of exercise than thepck^lox/lox controls.

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FIG. 4. Changes of blood glucose concentrations during exercise in pck^lox/lox+Alb-cre mice. ***, P < 0.001 versus pck^lox/lox at each time point; n = 5.

Impaired lipid metabolism and up-regulation of genes encoding enzymes of energy metabolism in mice lacking hepatic PEPCK. The liver weights in pck^lox/lox+Alb-cre mice were increased by 18 and 71% in the fed and 24-fasted states, respectively, comparedto pck^lox/lox mice (Table 3 and Fig. 5B). Oil red O and hematoxylin-eosinstaining of liver sections from pck^lox/lox+Alb-cre mice showed larger lipid droplets and vacuoles, respectively(Fig. 5D and F). Although not different in fed mice, hepatic triglyceridecontent in the 24-h-fasted pck^lox/lox+Alb-cre mice was increased by 94% compared with controls. Fastingplasma FFA and triglyceride concentrations were also greater inthe knockout mice than in the controls. In contrast, the plasmaBHBA concentration was less in the knockout mice (Table 3), suggestinga possible decrease in FFA $beta$ oxidation in livers of the knockoutmice. Hepatic malonyl-CoA concentrations were not different betweenthe two genotypes at the fasted state (Table 3).

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FIG. 5. Hepatic steatosis in 24-h-fasted pck^lox/lox+Alb-cre mice. (A and B) Necropsy indicates increased liver size with pale color in ~9-week-old pck^lox/lox+Alb-cre mice compared to pck^lox/lox mice. (C and D) Oil red O histochemistry for neutral lipids in liver sections. Larger lipid droplets (red) are shown in livers of pck^lox/lox+Alb-cre mice than in those of pck^lox/lox mice. (E and F) Hematoxylin-eosin histological staining for liver sections. Open circles in liver sections of pck^lox/lox+Alb-cre mice suggest lipid vacuoles. Scale bars in panels C to F represent 50 µm.

To begin to determine the basis for abnormalities in the regulation of lipid metabolism in these mice, malonyl-CoA decarboxylasemRNA abundance was assessed and found to be increased by 71% inlivers of the knockout mice (Fig. 6A). The mRNA levels for themitochondrial and peroxisomal FFA $beta$ -oxidation enzymes, acyl-CoAoxidase, very long-chain fatty acyl-CoA dehydrogenase, and long-chainfatty acyl-CoA dehydrogenase were increased by 551, 320, and 214%,respectively. The mRNA levels for medium-chain fatty acyl-CoAdehydrogenase, carnitine acetyltransferase, and enoyl-CoA hydratase-L-3-hydroxyacyl-CoAdehydrogenase bifunctional protein were also increased, but tosmaller extents (Fig. 6A). There was no change in the mRNA abundancefor microsomal FFA $omega$ -oxidation enzyme, CYP4A1, and CYP4A4 (datanot shown). Palmitate $beta$ -oxidation activity in liver homogenateswas also increased by 16% (P < 0.01 [data not shown]), consistentwith elevated mRNA abundance for FFA oxidation enzymes.

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FIG. 6. Altered gene expression for energy metabolism enzymes in 24-h-fasted pck^lox/lox+Alb-cre mice. Northern blots were first probed with the specific cDNA; then the membranes were stripped and reprobed with cyclophilin cDNA. The relative abundance for each mRNA was normalized to the cyclophilin mRNA level. (A) Lipid-metabolizing enzymes. MCD, malonyl-CoA decarboxylase; VLCAD, very long-chain fatty acyl-CoA dehydrogenase; LCAD, long-chain fatty acyl-CoA dehydrogenase; MCAD, medium-chain fatty acyl-CoA dehydrogenase; COT, carnitine octanoyltransferase; CAT, carnitine acetyltransferase; ACO, acyl-CoA oxidase; PBE, enoyl-CoA hydratase-L-3-hydroxyacyl-CoA dehydrogenase bifunctional protein. (B) Gluconeogenic, TCA cycle, and other enzymes. cAAT and mAAT, cytosolic and mitochondrial aspartate aminotransferase, respectively; cMDH and mMDH, cytosolic and mitochondrial malate dehydrogenase, respectively; CS, citrate synthase; IDH, isocitrate dehydrogenase; SCS, succinyl-CoA synthetase; LDH, lactate dehydrogenase; ALT, alanine aminotransferase; PC, pyruvate carboxylase; G6Pase, glucose-6-phosphatase; FBPase, fructose-1,6-bisphosphatase; GAPDH, glyceraldehyde-3-phosphate dehydrogenase. *, P < 0.05, **, P < 0.01, and ***, P < 0.001; n = 4.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

We used an allelogenic Cre/loxP gene targeting strategy to determine role of cytosolic PEPCK in hepatic gluconeogenesis andenergy metabolism. This strategy enabled the creation of a seriesof three functionally distinct pck alleles from a single ES cellline. In addition, since one of the alleles created was conditional,by intercrossing these animals with a line of Alb-cre transgenicmice that we have previously described (35), we were also ableto generate mice with a liver-specific knockout ofPEPCK.

PEPCK is essential for life. The initiation of PEPCK gene expression and gluconeogenesis occur at birth since suckling rodent pups are thought to dependon gluconeogenesis for glucose production (2, 11). Thus,the facts that pck^del/del mice die within 3 days of birth and that 1-day-old pck-null pupsare markedly hypoglycemic suggest impaired gluconeogenesis. Moreover,the lack of differences in fetal liver glycogen content betweenthe pck^del/del and pck^w/w fetuses, but decreased glycogen content and plasma glucose concentrationsin 1-day-old pck^del/del pups, is also consistent with impaired gluconeogenesis in theseknockout pups. However, it is not entirely clear whether the causeof death in these pups is actually hypoglycemia. First, glucose-6-phosphataseknockout mice, which have impaired hepatic and renal gluconeogenesisas well as severe hypoglycemia, do not die until 5 weeks of age(24). Second, the liver-specific PEPCK knockout (pck^lox/lox+Alb-cre) mice, which at day 1 exhibited hypoglycemia as severeas that in the pck^del/del animals, survived and were euglycemic by 3 days of age. Thus,it remains possible that other factors besides hypoglycemia contributeto the earlier death of PEPCK knockout pups. Indeed, since PEPCKimmunoreactivity has been detected in a variety of cells and tissues(48), it is possible that the animals die as a result of lossof PEPCK in one or more of these celltypes.

Fasted mice with diminished PEPCK gene expression are euglycemic at rest. The Cre/loxP strategy used in this study involved placement of a neo cassette between exons 3 and 4 of the PEPCK gene andits subsequent removal by cre plasmid microinjections after germline transmission. However, the mice that retained the neo cassettehave a functionally impaired allele that proved to be valuablein assessing the control strength of PEPCK on gluconeogenesis.Interestingly, both pck^{lox+neo/lox+neo} and pck^lox+neo/del mice were viable and did not exhibit any abnormality of bloodglucose concentrations after a 24-h fast. Indeed, the fact thatmice with a 90% reduction of PEPCK expression globally, as wellas animals with a total knockout of hepatic PEPCK, are able tomaintain euglycemia after fasting clearly indicates that thisenzyme exerts a much weaker control of gluconeogenesis than previouslythought. Considering that the isotopic studies in pck^lox/lox+Alb-cre mice showed that these animals had similar glucose turnoverrates and plasma [¹⁴C]glucose specific activities (derived from [¹⁴C]lactate) as wild-type mice, this conclusion is virtually inescapable.However, while the isotopic studies indicate that resting micewithout hepatic PEPCK remain capable of synthesizing almost thesame amount of glucose as a normal animal, how this is achievedremainsunclear.

The liver and kidney are the only two gluconeogenic tissues. In humans, the contribution of renal glucose production duringthe postabsorptive state to systemic glucose appearance has beenreported to vary from 5 to 28% (9, 42). The kidney can contributemore than 50% of total glucose production during either a 5- to6-week starvation in humans (33) or insulin-induced hypoglycemiain dogs (4). Thus, we cannot rule out the possibility thatnet glucose production in the kidney increases to compensate fordiminished hepatic glucose production in pck^lox/lox+Alb-cre mice although PEPCK gene expression in the kidney ofpck^lox/lox+Alb-cre mice isunchanged.

It is also possible that the liver in pck^lox/lox+Alb-cre mice is still capable of converting lactate to glucose, although there isno known pathway other than via PEPCK for the conversion of oxaloacetateto phosphoenolpyruvate. Mitochondrial PEPCK, even though it accountsfor only ~2% of total PEPCK activity, may be sufficient to maintainsufficient gluconeogenesis during fasting, provided there is noadditional stress such as exercise. There is little reason tothink that the thermodynamically unfavorable conversion of pyruvateto phosphoenolpyruvate by pyruvate kinase occurs in these mice,although this possibility may need to be directlytested.

Hepatic gluconeogenesis may also be activated by enhanced pyruvate carboxylation, malate-aspartate shuttle, TCA cycle, andoxidative phosphorylation and ATP production (14, 19, 32).The increased hepatic mRNA levels for pyruvate carboxylase, alanineaminotransferase, mitochondrial malate dehydrogenase, cytosolicmalate dehydrogenase, cytosolic aspartate aminotransferase, citratesynthase, and succinyl-CoA synthetase in pck^lox/lox+Alb-cre mice (Fig. 6B) after a 24-h fast are all consistent withthispossibility.

Glycerol is normally considered a minor gluconeogenic substrate since it accounts for only ~3% of overall glucose presentin the postabsorptive state (31). Plasma glycerol is derivedfrom adipose tissue as a result of lipolysis, which probably isenhanced in fasted pck^lox/lox+Alb-cre mice as suggested by increased plasma FFA concentration,thereby increasing glycerol availability. On the other hand, becauseof the increased hepatic triglyceride content in the knockoutmice, more plasma glycerol would be phosphorylated by hepaticglycerol kinase for esterification of fatty acid in the liverof the knockout mice during fasting. Moreover, plasma glycerolconcentrations are not changed in pck^lox/lox+Alb-cre mice. Thus, it is unlikely that a compensatory increasein gluconeogenesis from glycerol occurs in thesemice.

It should also be pointed out that futile cycling of substrates (e.g., glucose and fructose-6-phosphate cycling) might leadto an overestimation of the measurement of glucose turnover asdetermined by [3-³H]glucose, with glucose utilization in peripheral tissues actuallybeing decreased. Since the plasma glucose concentration reflectsthe balance of glucose production and utilization, a decreasein glucose utilization would help maintain glucose homeostasiseven if glucose production were diminished in pck^lox/lox+Alb-cre mice. It is also possible that increased plasma FFA inpck^lox/lox+Alb-cre mice compete with glucose for metabolism in tissues likeskeleton muscle, a major organ of glucose consumption, therebyimpairing glucose utilization in this tissue (36).

Despite a normal fasting glucose concentration at rest, blood glucose concentrations of pck^lox/lox+Alb-cre mice decreased with exercise. The exercise response patternof blood glucose concentrations in the control and knockout miceis similar to that observed in a study of fed rats treated with3-mercaptopicolinic acid (17). Since the mice were fasted for24 h before exercise, glycogen stores would not be expected tocontribute substantially to glucose production. Thus, the diminishedblood glucose concentration in pck^lox/lox+Alb-cre mice after 30 min of exercise probably reflects inadequategluconeogenic flux in the face of increased peripheral glucoseutilization. It has previously been shown that the glucose appearancerate in control rats is increased ~2-fold during submaximal exercisebut decreased in 3-mercaptopicolinic acid-treated rats (43).Therefore, the exercise study demonstrates that the liver-specificPEPCK knockout mice have limited gluconeogeniccapacity.

While additional studies may be required to confirm our experimental interpretations, the results we have obtained are consistentwith the conclusion that PEPCK is much less effective in determininggluconeogenic flux than previously thought. Instead of a singledominant control point, these results support the concept of multienzymeregulation of the gluconeogenic pathway (13, 34). This differencemay have significant implications for the development of strategiesto inhibit the excess hepatic glucose production that occurs intype 2 diabetesmellitus.

Impaired lipid metabolism in liver-specific PEPCK knockout mice. While these studies strongly suggest that PEPCK exerts much less control of gluconeogenesis than previously thought, the findingof marked steatosis pck^lox/lox+Alb-cre mice during fasting indicates that the enzyme has a previouslyunsuspected role in regulating hepatic lipid metabolism. The increasedhepatic triglyceride accumulation in pck^lox/lox+Alb-cre mice may result from the 60% increased plasma FFA concentrationin these mice. The hepatic steatosis in pck^lox/lox+Alb-cre mice may also be caused by a decrease in hepatic FFAoxidation, as suggested by lower plasma BHBA concentration despiteincreased plasma FFA concentration in these animals. Malonyl-CoAis a potent inhibitor of carnitine palmitoyltransferase I, thekey enzyme for transport of FFA into mitochondria for oxidation(26). Moreover, the concentration of malonyl-CoA in muscle iscorrelated positively with the sum of citrate and malate concentrations(38). However, the fasting hepatic malonyl-CoA concentrationin pck^lox/lox+Alb-cre mice was not increased, presumably due to increased malonyl-CoAdecarboxylase, as indicated by RNAanalysis.

It is also surprising that the expression of genes encoding FFA-oxidizing enzymes both in mitochondria and in peroxisomesis actually elevated in pck^lox/lox+Alb-cre mice during fasting. mRNA abundance for both acyl-CoAoxidase and fatty acyl-CoA dehydrogenases was elevated severalfoldin the liver-specific knockout mice. Acyl-CoA oxidase is an importantenzyme for peroxisomal FFA oxidation, and acyl-CoA oxidase knockoutmice also have severely fatty livers (15). Fatty acyl-CoA dehydrogenasesare also important enzymes for mitochondrial FFA oxidation, asdemonstrated by the mortality rates of long-chain fatty acyl-CoAdehydrogenase knockout mice (21). The mechanism(s) responsiblefor the increased expression of the genes encoding these enzymesis not known. The activation of peroxisome proliferation-activatedreceptor alpha (PPAR $alpha$ ) signaling by long-chain acyl-CoA, as suggestedby studies of the acyl-CoA oxidase knockout mice (15), doesnot provide an explanation because the expression of other genesknown to be regulated by PPAR $alpha$ , such as the CYP4A1, CYP4A3, andcarnitine octanoyltransferase genes, is not altered in pck^lox/lox+Alb-cremice.

This finding, as well as the lack of significant alterations in plasma hormone concentrations, suggests that alterations inthe concentrations of metabolic intermediates may affect expressionof numerous genes encoding various enzymes involved in energymetabolism. Indeed, the markedly elevated expression of genesencoding hepatic FFA oxidation enzymes stands in direct contradictionto the fatty liver phenotype in pck^lox/lox+Alb-cremice.

Concluding statements. This study provides new and unexpected insights into the role of PEPCK in regulating hepatic energy metabolism. While fastingplasma glucose concentrations are normal in mice with greatlydiminished PEPCK gene expression, the absence of PEPCK causesimpaired lipid metabolism and marked alterations in the expressionof a variety of hepatic genes involved in energy metabolism. Thesechanges occur in the absence of alterations in plasma concentrationsof major hormones. Thus, PEPCK appears to play a vital role inthe integration of multiple pathways of energy metabolism, a functionthat has not heretofore been attributed to thisenzyme.

	ACKNOWLEDGMENTS

We thank D. Wasserman, P. Flakoll, Y. Fujimoto, E. P. Donahue, M.-Y. Zhu, and J. Lindner for help and advice in performingthese studies, and we thank A. D. Cherrington and D. K. Grannerfor reading the manuscript and providing comments. We are alsoindebted to A. Saha (Boston University) for measuring malonyl-CoAand to D. Kelly (Washington University) for providing cDNA forCYP4A3, CYP4A1, andMCAD.

This study was supported by funding from the National Institutes of Health (grant DK42502). P. She is a recipient of a JDFIpostdoctoralfellowship.

	FOOTNOTES

^* Corresponding author. Mailing address: 702 Light Hall, Vanderbilt University School of Medicine, Nashville, TN 37232-0615.Phone: (615) 322-7006. Fax: (615) 322-7236. E-mail: mark.magnuson{at}mcmail.vanderbilt.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
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