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Effects of Insulin Deficiency or Excess on Hepatic Gluconeogenic Flux During Glycogenolytic Inhibition in the Conscious Dog

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

	ABSTRACT

TOP ABSTRACT INTRODUCTION RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 
The direct acute effects of insulin on the regulation of hepatic gluconeogenic flux to glucose-6-phosphate (G6P) in vivo may be masked by the hormone’s effects on net hepatic glycogenolytic flux and the resulting changes in glycolysis. To investigate this possibility, we used a glycogen phosphorylase inhibitor (BAY R3401) to inhibit glycogen breakdown in the overnight-fasted dog, and the effects of complete insulin deficiency or a fourfold rise in the plasma insulin level were assessed during a 5-h experimental period. Hormone levels were controlled using somatostatin with portal insulin and glucagon infusion. After the control period, plasma insulin infusion 1) was discontinued, creating insulin deficiency; 2) increased fourfold; or 3) was continued at the basal rate. During insulin deficiency, glucose production and the plasma level and net hepatic uptake of nonesterified free fatty acids increased, whereas during hyperinsulinemia they decreased. Net hepatic lactate uptake increased sixfold during insulin deficiency and 2.5-fold during hyperinsulinemia. Net hepatic gluconeogenic flux increased more than fourfold during insulin deficiency but was not reduced by hyperinsulinemia. We conclude that in the absence of appreciable glycogen breakdown, an acute gluconeogenic effect of hypoinsulinemia becomes manifest, whereas inhibition of the process by a physiologic rise in insulin was not evident.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

Insulin, a key inhibitor of hepatic glucose production, has effects on both glycogenolysis and gluconeogenesis (1). In the overnight-fasted dog, the basal hepatic sinusoidal insulin level is close to the half maximally effective concentration required for inhibition of net hepatic glycogenolytic flux (NHGLY) (2). Thus, small changes in the hepatic insulin concentration have large and rapid effects on glycogenolysis. Gluconeogenesis (defined as the synthesis and subsequent release of glucose from noncarbohydrate precursors) can be acutely reduced by insulin through a redirection of the carbons derived from gluconeogenic flux to glucose-6-phosphate (G6P; G6P neogenesis) to hepatic glycogen rather than blood glucose (1,3). Thus, insulin can alter gluconeogenesis indirectly, without necessarily affecting G6P neogenesis, through an action on glycogen metabolism.

In contrast to its sensitive effects on glycogen metabolism, physiological changes in insulin in vivo seem to have little acute effect on hepatic gluconeogenic flux to G6P (1,3–6). The effect that insulin does have on gluconeogenic flux to G6P in the liver seems to be secondary to its actions on muscle, fat, and the pancreas through decreased lactate, amino acid, free fatty acid, and glycerol availability and the inhibition of glucagon release. However, during conditions in which insulin levels are chronically deficient (in an absolute or relative sense), such as long-term fasting or diabetes, gluconeogenic flux to G6P and the gluconeogenic rate are known to be significantly increased (7,8). The explanation for this paradox is not clear.

Fructose-2,6-bisphosphate (F2,6P₂) is an activator of the glycolytic enzyme 6-phosphofructo-1-kinase (PFK-1) and inhibitor of the gluconeogenic enzyme fructose-1,6-bisphosphatase (FBP-1) and thus plays an important role in the regulation of carbon flux through these pathways (Fig. 1). The level of hepatic F2,6P₂ is determined by the activity of a bifunctional enzyme (PFK-2/FBP-2) as well as by the availability of substrate (fructose-6-phosphate [F6P]) for the bifunctional enzyme reaction. Insulin opposes the action of cAMP-dependent protein kinase, causing the dephosphorylation of the bifunctional enzyme and thus an increase in F2,6P₂. As a result, PFK-1 is activated, FBP-1 is inactivated, and thus F1,6P₂ levels increase. This leads to activation of the glycolytic enzyme pyruvate kinase. In addition, insulin treatment has been shown to reduce the activity of the gluconeogenic enzymes phosphoenol pyruvate carboxykinase (PEPCK) and pyruvate carboxylase (PC). Thus, in vitro, treatment of hepatocytes with insulin increases glycolysis and decreases gluconeogenic flux. Conversely, inhibition of glycogenolysis by insulin can decrease F2,6P₂ by reducing G6P and F6P concentrations (7,8). This would be expected to decrease glycolysis and stimulate gluconeogenic flux to G6P. Indeed, during a euglycemic-hyperinsulinemic clamp in which hepatic insulin levels were increased, a fall in net glycogen breakdown resulted in decreased net hepatic lactate release and increased gluconeogenic flux to G6P from lactate (1,9). Thus, in vivo, the secondary consequences of insulin’s actions on glycogen metabolism would seem to offset its direct effects on gluconeogenesis and glycolysis. This may explain the apparent inability of an acute rise in insulin to inhibit gluconeogenic flux to G6P in the overnight-fasted dog.

View larger version (17K): [in this window] [in a new window]   FIG. 1. The key enzymes of the hepatic glycolytic, gluconeogenic, and glycogenolytic substrate cycles. Substrates: glucose (GLC), G6P, glucose-1-phosphate (G1P), uridine diphosphoglucose (UDPG), glycogen (GLY), F6P, F2,6P2, F1,6P2, phosphoenol pyruvate (PEP), and pyruvate (PYR). Enzymes: glucokinase (GK), G6Pase, glycogen synthase (GS), glycogen phosphorylase (GP), PFK-1, FBP-1, PFK-2/FBP-2, L-type pyruvate kinase (PK), PC, and PEPCK. F2,6P2 is an activator of PFK-1 and inhibitor of FBP-1.

To investigate the ability of insulin to acutely alter gluconeogenic flux to G6P in vivo in the absence of its effects on glycogenolysis and the attendant changes in glycolytic flux, we used a glycogen phosphorylase inhibitor. This compound (BAY R3401) has been demonstrated effectively to inhibit NHGLY (11–14) and provided a means to determine the effect of a fourfold rise in the plasma insulin level or complete insulin deficiency on hepatic gluconeogenic flux to G6P and glucose production during a 5-h experimental period in the overnight-fasted dog under conditions in which large changes in hepatic glycogen breakdown were prevented.

	RESEARCH DESIGN AND METHODS

TOP ABSTRACT INTRODUCTION RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 
Animal care and surgical procedures.
Experiments were conducted on 18 overnight-fasted conscious mongrel dogs (20–28 kg) of either sex. Housing and diet have been described previously (1). The surgical facility met the standards published by the American Association for the Accreditation of Laboratory Animal Care, and the protocols were approved by the Vanderbilt University Medical Center Animal Care Committee. All dogs underwent a laparotomy 2 weeks before the experiment to implant infusion catheters into the jejunal and splenic veins, sampling catheters into the portal and hepatic veins and the femoral artery, and Doppler flow probes around the hepatic artery and portal vein, as described elsewhere (1). Each dog was used for only one experiment. All dogs studied had 1) leukocyte count <18,000/mm³, 2) a hematocrit >35%, 3) a good appetite, and 4) normal stools.

Experimental design.
Intraportal catheters (splenic and jejunal) were used for the infusion of insulin (Lilly, Indianapolis, IN) and glucagon (Lilly). Angiocaths (Deseret Medical, Becton-Dickinson, Sandy, UT) were inserted percutaneously into leg veins for [3-³H]glucose (DuPont NEN, Boston, MA), indocyanine green (Sigma, St. Louis, MO), and peripheral glucose (50% Dextrose; Baxter Healthcare Corporation, Deerfield, IL) infusion. Animals were allowed to rest quietly in a Pavlov harness for 30 min before the experiments started. Each of the three protocols consisted of an equilibration period (-120 to -40 min), a basal period (-40 to 0 min), and an experimental period (0–300 min). At -120 min, a priming dose of [3-³H]glucose (50 µCi) was given, and constant infusions of [3-³H]glucose (0.4 µCi/min) and indocyanine green (0.07 mg/min) were started. At the same time, a constant infusion of somatostatin (SRIF; 0.8 µg · kg^-1 · min^-1) was started in a peripheral vein to inhibit endogenous pancreatic hormone secretion, and constant intraportal glucagon (0.5 ng · kg^-1 · min^-1) and insulin (300 µU · kg^-1 · min^-1) infusions were started to replace basal secretion of these hormones. Also at -120 min, a glycogen phosphorylase inhibitor (BAY R 3401; 10 mg/kg in a 0.5% methyl cellulose/water solution) was given orally or intragastrically, depending on whether a stomach catheter had been implanted during surgery (there was no difference in the effectiveness of the drug with one route or the other). Shortly thereafter, a variable glucose infusion was begun to maintain euglycemia in the presence of the glycogen phosphorylase inhibitor. [3-³H]glucose infusion rates were modified in accordance with the cold glucose infusion rates to minimize changes in the specific activity. During the experimental period three insulin infusion rates were used: protocol 1 (basal insulin [control, n = 6]), no change was made in the insulin infusion rate over the course the experiment; protocol 2 (insulin deficiency [n = 6]), beginning at 0 min, the intraportal insulin infusion was stopped, resulting in 5 h of hypoinsulinemia; and protocol 3 (insulin excess [n = 6]), beginning at 0 min, the intraportal insulin infusion rate was increased to (1.2 mU · kg^-1 · min^-1), resulting in 5 h of hyperinsulinemia.

Immediately after the final sampling time, each animal was anesthetized and sections of three liver lobes were freeze-clamped in situ and stored at -70°C as previously described (1). All animals were then killed, and the correct position of the catheter tips was confirmed.

Analytical procedures.
Hematocrit; plasma glucose, [³H]glucose, glucagon, insulin, cortisol, and nonesterified free fatty acids (NEFAs); and blood alanine, glycine, serine, threonine, lactate, glutamine, glutamate, glycerol, ß-hydroxybutyrate, and hepatic glycogen concentrations were determined as previously described (1). Hepatic glycogen content was measured as previously described (15). Hepatic tissue glucose, G6P, and F6P were measured fluorometrically by standard enzymatic methods (16,17) after deproteinization with 3% perchloric acid.

Calculations.
Net hepatic balances (NHBs) were calculated with the arteriovenous (A-V) difference method using the following formula: NHB = Load_out - Load_in where Load_out = [H] · HF and Load_in = [A] · AF + [P] · PF and where [H], [A], and [P] were the substrate concentrations in hepatic vein, femoral artery, and portal vein blood or plasma, respectively, and HF, AF, and PF were the blood flow in the hepatic vein, hepatic artery, and portal vein, as determined by the ultrasonic flow probes. With this calculation, a positive value represents net output by the liver, whereas a negative value represents net hepatic uptake. Plasma glucose and [³H]glucose values were multiplied by 0.73 to convert them to blood glucose values as validated elsewhere (15). Net fractional substrate extraction by the liver was calculated by NHB/Load_in. The approximate insulin and glucagon levels in plasma entering the liver sinusoids were calculated using the formula [A] · %AF + [P] · %PF, where [A] and [P] were arterial and portal vein hormone concentrations, respectively, and %AF and %PF were the respective percentage contributions of arterial and portal flow to total hepatic blood flow.

Tracer-determined whole-body glucose production (R_a) was measured using a primed, constant infusion of [3-³H]glucose. Data calculation was carried out using the two-compartment model described by Mari (18), using canine parameters reported by Dobbins et al. (19).

For calculation of unidirectional hepatic glucose uptake (HGU), the net [³H]glucose uptake was divided by the arterial [³H]glucose specific activity. The above calculation is based on the assumption that intrahepatic uptake of glucose occurs before glucose production so that the plasma glucose specific activity is not diluted. Even if this assumption is not correct, the drop in specific activity across the liver is very small; thus, the assumption is of little consequence. Unidirectional hepatic glucose release (HGR) was determined by adding HGU to net hepatic glucose output.

Gluconeogenesis, as classically defined, is the synthesis and subsequent release of glucose from noncarbohydrate precursors. Carbon produced from flux through the gluconeogenic pathway does not necessarily have to be released as glucose; it can also be stored in glycogen. Therefore, we make a distinction between gluconeogenic flux to G6P (conversion of precursors to G6P: G6P neogenesis) and gluconeogenesis (release of glucose derived from gluconeogenic flux).

Gluconeogenic flux to G6P was determined by summing the net hepatic uptake rates of the gluconeogenic precursors (alanine, glycine, serine, threonine, glutamine, glutamate, glycerol, lactate, and pyruvate) and dividing by 2 to account for the incorporation of three carbon precursors into the six-carbon glucose molecule. Net hepatic gluconeogenic flux was determined by subtracting the summed net hepatic output rates (when such occurred) of the substrates noted above (in glucose equivalents) and glucose oxidation (GO) from gluconeogenic flux to G6P. GO was assumed to be 0.2 mg · kg^-1 · min^-1 throughout each experiment. In other experiments, GO varied from this estimate by no more than 0.1 mg · kg^-1 · min^-1 under widely varying conditions (S. Satake, M.C. Moore, A.D.C., unpublished observations); thus, any changes in GO that might have occurred in the present experiments should have been small and of little consequence to our estimates. A positive number represents net gluconeogenic flux to G6P, whereas a negative number indicates net glycolytic flux.

NHGLY was estimated by subtracting net hepatic gluconeogenic flux from net hepatic glucose balance (NHGB). A positive number therefore represents net glycogen breakdown, whereas a negative number indicates net glycogen synthesis.

Ideally, the gluconeogenic flux rate would be calculated using unidirectional hepatic uptake and output rates for each substrate, but this would be difficult, as it would require the simultaneous use of multiple stable isotopes, which could themselves induce a mild perturbation of the metabolic state. Therefore, NHB was used instead, necessitating consideration of the limits of this approach. There is little or no production of gluconeogenic amino acids or glycerol by the liver, so in this case the compromise is of little consequence. Such is not the case, however, for lactate. Our estimate of the rate of gluconeogenic flux to G6P will be quantitatively accurate only if we assume that lactate flux is unidirectional at a given moment (i.e., either in or out of the liver). In a given cell, this does not seem like an unreasonable assumption in light of the reciprocal control of gluconeogenesis or glycogenolysis (8). Katz and Jungermann suggested, however, that there is spatial separation of metabolic pathways so that gluconeogenic periportal hepatocytes primarily synthesize glucose and glycogen from lactate and other noncarbohydrate precursors, whereas glycolytic perivenous hepatocytes predominantly consume plasma glucose, which is incorporated into glycogen, oxidized, or released as lactate or other glycolytic substrates (20,21). Therefore, it is possible that under normal nutritional conditions in a net sense, hepatic gluconeogenic and glycolytic flux occurs simultaneously, with lactate output or uptake occurring in different cells. To the extent that flux occurs in both directions simultaneously, the A-V difference method will underestimate gluconeogenic flux to G6P. It should be noted, however, that net hepatic gluconeogenic flux and NHGLY can be calculated accurately without concern for the assumptions related to whether simultaneous gluconeogenic and glycolytic substrate flux occurs.

The total net contribution (TNC) of carbon to hepatic glycogen was determined using the average net hepatic glycogen synthetic rate during the experimental period to predict the total net accumulation of glycogen during that period (300 min) using the following formula: TNC (mg glycogen/g liver) = net hepatic glycogen synthesis (mg · kg^-1 · min^-1) · time (min)/liver weight (g/kg body wt).

Statistical analysis.
The data were analyzed for differences from the basal period and for differences from the control group. Statistical comparisons were carried out using two-way ANOVA (JMP IN Software, SAS Institute Inc.). One-way ANOVA comparison tests were used post hoc when significant F ratios were obtained. The level of significance was P < 0.05 (two-sided test).

	RESULTS

TOP ABSTRACT INTRODUCTION RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 
In the control group, the arterial and hepatic sinusoidal plasma insulin levels remained basal and unchanged throughout the study (5 and 15 µU/ml, respectively; Fig. 2). In the insulin deficiency group, the arterial and sinusoidal insulin levels fell to 1 ± 0 and 1 ± 1 µU/ml, respectively (P < 0.05), whereas in the insulin excess group these levels rose to 20 ± 1 and 66 ± 3 µU/ml, respectively (P < 0.05). The arterial and hepatic sinusoidal glucagon levels remained basal and unchanged in each group (Fig. 2).

View larger version (27K): [in this window] [in a new window]   FIG. 2. Arterial and hepatic sinusoidal plasma insulin and glucagon in 18-h–fasted conscious dogs during the basal (-40 to 0 min) and experimental (0–300 min) periods (mean ± SE; n = 6; *P < 0.05 vs. basal; P < 0.05 vs. control group). , control; , hypoinsulinemia; , hyperinsulinemia.

View larger version (25K): [in this window] [in a new window]   FIG. 3. Arterial plasma glucose level and NHB in 18-h–fasted conscious dogs during the basal (-40 to 0 min) and experimental (0–300 min) periods (mean ± SE; n = 6; *P < 0.05 vs. basal; P < 0.05 vs. control group). , control; , hypoinsulinemia; , hyperinsulinemia.

Endogenous glucose appearance (R_a) in the control group was reduced relative to normal as a result of phosphorylase inhibition but did not change significantly over time. During insulin deficiency, R_a increased to 2.85 ± 0.13 mg · kg^-1 · min^-1 (P < 0.05), whereas during insulin excess it was completely inhibited (P < 0.05; Table 1). The rate of glucose disappearance (R_d) did not change in the control or insulin deficiency groups, whereas during insulin excess it increased significantly from 2.48 ± 0.42 in the basal period to 10.55 ± 2.05 mg · kg^-1 · min^-1 during the last hour of the study (P < 0.05; Table 1). Glucose clearance, an index of the avidity with which tissues take up glucose, was unchanged in the control group, tended to fall during insulin deficiency, and rose almost fivefold (P < 0.05) during insulin excess (Table 1).

The arterial blood lactate level did not change significantly in any group, although there was a tendency for it to fall slightly and then rise modestly (Fig. 4). Net hepatic lactate uptake (NHLU) did not change significantly over time in the control group but increased more than sixfold in the insulin deficiency group (rising from 1.42 ± 1.61 to 8.84 ± 1.11 µmol · kg^-1 · min^-1; P < 0.05) and rose modestly in the insulin excess group (2.06 ± 1.22 to 5.04 ± 0.62 µmol · kg^-1 · min^-1; P < 0.05; Fig. 4).

View larger version (27K): [in this window] [in a new window]   FIG. 4. Arterial blood lactate level and NHB in 18-h–fasted conscious dogs during the basal (-40 to 0 min) and experimental (0–300 min) periods (mean ± SE; n = 6; *P < 0.05 vs. basal; P < 0.05 vs. control group). , control; , hypoinsulinemia; , hyperinsulinemia.

View larger version (32K): [in this window] [in a new window]   FIG. 5. Arterial blood gluconeogenic individual amino acid level (alanine, serine, threonine, glycine, glutamate, and glutamine), net hepatic gluconeogenic amino acid uptake, and change from basal gluconeogenic amino acid hepatic fractional extraction in 18-h–fasted conscious dogs during the basal (-40 to 0 min; 0.13 ± 0.03, 0.11 ± 0.03, and 0.13 ± 0.03 in the control, hypoinsulinemia, and hyperinsulinemia groups, respectively) and experimental (0–300 min) periods (mean ± SE; n = 6; *P < 0.05 vs. basal; P < 0.05 vs. control group). , control; , hypoinsulinemia; , hyperinsulinemia.

View larger version (27K): [in this window] [in a new window]   FIG. 6. Arterial blood glycerol level and net hepatic uptake in 18-h–fasted conscious dogs during the basal (-40 to 0 min) and experimental (0–300 min) periods (mean ± SE; n = 6; *P < 0.05 vs. basal; P < 0.05 vs. control group). , control; , hypoinsulinemia; , hyperinsulinemia.

View larger version (26K): [in this window] [in a new window]   FIG. 7. Arterial plasma nonesterified free fatty acid level and net hepatic uptake in 18-h–fasted conscious dogs during the basal (-40 to 0 min) and experimental (0–300 min) periods (mean ± SE; n = 6; *P < 0.05 vs. basal; P < 0.05 vs. control group). , control; , hypoinsulinemia; , hyperinsulinemia.

View larger version (33K): [in this window] [in a new window]   FIG. 8. Hepatic gluconeogenic flux to G6P, net hepatic gluconeogenic flux, and NHGLY change from basal in 18-h–fasted conscious dogs during the basal (-40 to 0 min; gluconeogenic flux to G6P: 1.05 ± 0.17, 0.78 ± 0.09, and 0.86 ± 0.07; net gluconeogenic flux: 0.58 ± 0.26, 0.31 ± 0.17, and 0.47 ± 0.11; net glycogenolytic flux: -0.30 ± 0.32, -0.46 ± 0.39, and -0.81 ± 0.28 mg · kg-1 · min-1 in the control, hypoinsulinemia, and hyperinsulinemia groups, respectively) and experimental (0–300 min) periods (mean ± SE; n = 6; *P < 0.05 vs. basal; P < 0.05 vs. control group). , control; , hypoinsulinemia; , hyperinsulinemia.

Hepatic gluconeogenic flux to G6P did not change significantly over time in the control group (1.05 ± 0.17 and 1.15 ± 0.17 mg · kg^-1 · min^-1 in the two periods). During insulin deficiency, however, it rose twofold, from 0.78 ± 0.09 to 1.59 ± 0.14 mg · kg^-1 · min^-1 (P < 0.05), whereas during insulin excess it did not change significantly. The changes in gluconeogenic flux to G6P between the basal period and the last hour of the experiment were 0.10 ± 0.10, 0.81 ± 0.16, and 0.21 ± 0.13 mg · kg^-1 · min^-1 in the control, insulin deficiency, and insulin excess groups, respectively (P < 0.05; Figs. 8 and 9).

View larger version (31K): [in this window] [in a new window]   FIG. 9. Change from basal values in hepatic gluconeogenic flux to G6P and net hepatic gluconeogenic flux during the last hour of the experimental period (240–300 min) in 18-h–fasted conscious dogs (mean ± SE; n = 6; P < 0.05 vs. control group). , control; , hypoinsulinemia; , hyperinsulinemia.

	DISCUSSION

TOP ABSTRACT INTRODUCTION RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 
To examine insulin’s acute action on gluconeogenic flux to G6P in the absence of its effects on glycogenolytic flux, we inhibited glycogen breakdown using a glycogen phosphorylase inhibitor. The drug used in these studies, BAY R3401, was previously shown to effectively suppress glycogenolysis in hepatocytes (11), in perfused intact liver (11), and in the whole animal (rat and dog) (12–14). The active metabolite of BAY R3401 reduces glycogenolysis both by facilitating inactivation of the enzyme through allosteric inhibition and by dephosphorylation of glycogen phosphorylase a (11). In the dog, after administration of BAY R3401, inhibition of NHGLY resulted in a decrease in hepatic glucose production and net hepatic lactate balance (NHLB) but had no effect on the metabolism (level or NHB) of other gluconeogenic precursors, NEFAs, pancreatic or adrenal hormones, or hepatic blood flow (14). Whereas glucose R_a decreased 50%, glucose R_d and clearance were unaffected, indicating that the portion of the drug that passed the liver had little or no effect on muscle glycogen metabolism. These data suggest that BAY R3401 reduces hepatic glycogenolysis through a direct inhibitory action on glycogen phosphorylase and that it acts without producing other direct metabolic alterations.

Without the use of a phosphorylase inhibitor in the present study, complete insulin deficiency would have resulted in a large and rapid increase in glycogen breakdown. In a previous study in which hepatic sinusoidal insulin levels were selectively reduced by 75% (there was no decrease in arterial insulin level), NHGLY rose more than sixfold (to 5.39 mg · kg^-1 · min^-1) within 30 min (10). In the present study, when insulin was made completely deficient, net hepatic glycogen synthesis, which was evident during the basal period, slowly decreased until eventually a minimal rate of net glycogen breakdown was evident (0.71 ± mg · kg^-1 · min^-1 during the last hour of the experiment). As a result, insulin deficiency in the present study resulted in only a slight (30 mg/dl) rise in the plasma glucose level, rather than the two- to threefold increase that was expected during insulin deficiency in the absence of BAY R3401 (10). Glucose inhibits hepatic glucose production independent from insulin (22); thus, with the phosphorylase inhibitor present, the effect of insulin deficiency on gluconeogenic flux to G6P could be assessed, for the most part, without the confounding effects attributable to glycogenolysis and marked hyperglycemia, because carbon flux into G6P from plasma glucose or glycogen would reduce the ability of insulin deficiency to increase gluconeogenic flux.

With glycogenolytic flux inhibited, insulin deficiency caused significant increases in gluconeogenic flux to G6P and net hepatic gluconeogenic flux, which were evident within 3 h. During the basal period, there was no gluconeogenic contribution to NHGB (there was slight net glucose uptake); however, gluconeogenesis (the flux of gluconeogenically derived glucose into plasma) became evident during insulin deficiency, accounting for 65% of net hepatic glucose output by the end of the study. Gluconeogenic flux to G6P, as estimated using the A-V difference technique, was previously shown to decrease by 50% during selective hepatic insulin deficiency (the arterial insulin level was unchanged) (10). This finding was mainly due to a switch from NHLU to output, presumably reflecting the increase in glycolysis caused by augmented glycogen breakdown. In the present study, when glycogen breakdown was inhibited, insulin deficiency resulted in a twofold rise in hepatic gluconeogenic flux to G6P. This was due to a doubling of net hepatic glycerol uptake and a sixfold increase in NHLU. The increase in glycerol uptake was the result of an increase in substrate availability, which in turn resulted from increased lipolysis. The effect on lactate uptake was due to an increase in the fractional extraction of lactate by the liver and an increase in the supply of lactate from nonhepatic tissues. The latter is evident from the lack of a decrease in the blood lactate level despite an increase in NHLU. An effect on the fractional extraction of lactate by the liver could have resulted from the direct effect of insulin deficiency per se or from the rise in NEFA, which may itself have stimulated NHLU. Regardless of the mechanisms by which it occurred, there was more than a fourfold increase in net hepatic gluconeogenic flux when insulin was made deficient.

Gluconeogenic amino acid levels and uptake rates were unchanged during insulin deficiency and thus did not affect the carbon flux rates. Because insulin is generally considered to increase protein synthesis and decrease protein breakdown, insulin deficiency might have been expected to cause a rise in blood amino acid levels. Although whole-body protein breakdown seems to increase during insulin deficiency, some investigators have found that protein synthesis is normal or increased (23), possibly explaining why we observed no change in the gluconeogenic amino acid levels even when insulin was deficient.

In contrast to insulin deficiency, insulin excess did not seem to alter gluconeogenic flux to G6P or the net gluconeogenic carbon flux in the presence of the phosphorylase inhibitor. Previous studies have shown that NHGLY is quickly suppressed when increments in plasma insulin are created (1). Therefore, it was hoped that in the present study phosphorylase inhibition before elevation in insulin would prevent significant additional effects of the hormone on glycogenolysis. Indeed, NHGLY was already completely suppressed by the drug before the fourfold rise in plasma insulin; therefore, the hormone did not further inhibit glycogen breakdown.

In these studies, we found no inhibition of gluconeogenic flux to G6P after 5 h of a fourfold rise in plasma insulin level. In fact, there was a twofold rise in net gluconeogenic flux, an increase similar to that seen in the control group. In keeping with the anabolic effects of insulin on protein synthesis and breakdown (23), we observed an 40% decrease in arterial gluconeogenic amino acid levels. However, an equivalent increase in the fractional extraction of these amino acids by the liver prevented a fall in their net hepatic uptake rates (Fig. 5). Insulin has previously been reported to stimulate amino acid uptake by the liver (23). Net hepatic glycerol uptake tended to decrease during insulin excess as a result of the fall in blood glycerol secondary to the inhibition of lipolysis (Fig. 6). This was counterbalanced by a slight increase in NHLU (Fig. 4); thus, no net effect of the rise in insulin on gluconeogenic flux to G6P was observed even after 5 h of hyperinsulinemia.

In previous studies conducted in isolated hepatocytes and perfused rat liver, BAY R3401 significantly reduced G6P levels (11). Because net hepatic glycogen synthesis increased 1.63 mg · kg^-1 · min^-1 during hyperinsulinemia whereas net HGU increased only 1.25 mg · kg^-1 · min^-1, an insulin-mediated decrease in net hepatic gluconeogenic flux would have resulted in a decrease in G6P levels. In fact, net gluconeogenic flux increased 0.38 mg · kg^-1 · min^-1 in this group, resulting in no decline in G6P levels compared with the control. It is possible, therefore, that the buffering capacity of the liver to prevent critically low G6P levels did not permit an insulin-mediated inhibition of gluconeogenic flux to G6P, because a decline in F2,6P₂, associated with low G6P levels, could counteract the direct effects of insulin and prevent a decrease in gluconeogenic flux to G6P. It is possible that inhibition of gluconeogenic flux to G6P by insulin would be unmasked if in conjunction with hyperinsulinemia and the phosphorylase inhibitor the glucose level was increased, providing an alternate means for supplying glycolytic intermediates. We can nevertheless conclude that the rise in insulin inhibited gluconeogenesis per se (as opposed to G6P neogenesis) because glucose production was fully suppressed (Table 1). In the present study, therefore, the inhibition of gluconeogenesis caused by the increase in insulin was secondary to activation of glycogen synthesis rather than a decrease in gluconeogenic flux to G6P per se. This is in keeping with previous studies that have shown that on refeeding after an extended fast, 40–60% of glycogen is synthesized from gluconeogenic substrates, despite a rise in insulin (21).

HGU occurs by flux through glucokinase, with insulin stimulating uptake by activating glycogen synthase (24) and thereby providing a "pull mechanism" (21). Thus, as expected, HGU, the net direct contribution of plasma glucose to glycogen, and net hepatic glycogen synthesis were greatest during hyperinsulinemia. In contrast, during insulin deficiency, the liver switched from net HGU to output and net glycogen synthesis to breakdown. HGR is dependent on glucose-6-phosphatase (G6Pase), and the G6Pase catalytic subunit is thought to be a major control point in the G6Pase reaction (25). Using a subgroup of four of the six animals from each group in these experiments, induction of G6Pase catalytic subunit mRNA expression was determined and reported by Hornbuckle et al. (25). After 5 h of insulin treatment, the G6Pase catalytic subunit mRNA was 30% of that in the control group, in agreement with the observed decrease in hepatic glucose production, and the 30% increase in hepatic tissue glucose level. Conversely, G6Pase catalytic subunit mRNA expression rose to fourfold that in the control group during insulin deficiency, and correspondingly HGR was 2.8 times greater than the control, although in the presence of BAY R3401 the majority of the glucose released was gluconeogenic rather than glycogenolytic.

Insulin can regulate the fate of hepatic G6P indirectly through its effects on lipolysis. Plasma free fatty acids have been shown to increase hepatic gluconeogenesis (26–29) and to decrease whole-body glucose utilization (30). Whereas some studies have demonstrated increased glucose production in response to elevated NEFAs (31,32), others have failed to do so, presumably as a result of a compensatory decrease in NHGLY (26,28,33,34). The mechanisms by which an increase in NEFAs affects gluconeogenesis, glycolysis, and NHLB most likely include a rise in NEFA oxidation and thus an increase in the mitochondrial ratios of [acetyl CoA]/[CoA] and [NADH]/[NAD⁺] (30,35,36). Such an increase would inhibit the pyruvate dehydrogenase complex, increase citrate (an inhibitor of PFK-1 and PFK-2), and thereby decrease F2,6P₂ and F1,6P₂ concentrations. This in turn would result in decreased glycolysis and increased gluconeogenic flux to G6P (7,8,30). Generation of acetyl CoA or long-chain fatty acetyl CoA could also increase PC activity, and a rise in free fatty acid oxidation would supply the reducing equivalents (NADH) and energy (ATP) necessary for gluconeogenic flux (30,35–39). In addition, free fatty acids have been reported to stimulate PEPCK gene transcription (40).

Given the potential effects of free fatty acids on glycolytic and gluconeogenic fluxes, a rise in NEFAs, such as occurs with insulin deficiency, would be expected to reduce NHLB and stimulate net gluconeogenic flux. Previously, when selective hepatic insulin deficiency was created so that arterial insulin and thus NEFA levels did not change, NHGLY was stimulated and net hepatic lactate output increased to 9 µmol · kg^-1 · min^-1 (10). Conversely, during insulin deficiency in the present study when the NEFA level doubled and glycogenolysis was inhibited, lactate was taken up by the liver at a net of 9 µmol · kg^-1 · min^-1. This was associated with an increase in fatty acid oxidation as indicated by a threefold rise in ß-OHB level and increased net hepatic ß-OHB output. Additional investigation will be required to determine whether the effect of insulin deficiency on gluconeogenic flux to G6P was due to direct hepatic insulin action or was the result of insulin’s indirect peripheral effects, because the increase in gluconeogenic flux to G6P was the result of increased hepatic glycerol and lactate uptake, and both occurred in conjunction with an increase in lipolysis and NEFA level.

Previous studies have shown that a fall in NEFAs results in increased net hepatic lactate output, decreased glucose production (to the extent that G6P-derived carbon exits the liver as lactate instead of glucose), and decreased gluconeogenic flux to G6P (to the extent that lactate uptake no longer contributes to the process). This was demonstrated by Sindelar et al. (9), who found that a selective increase in arterial insulin (no change in portal vein insulin) led to a decrease in NEFA levels and resulted in the redirection of glycogenolytically derived carbon to lactate rather than glucose. However, when free fatty acid levels were prevented from falling during a selective increase in arterial insulin (41) or insulin was increased selectively in the liver so that NEFA levels did not change (9), an increase in net hepatic lactate output did not occur. In the present study, although during hyperinsulinemia the net hepatic uptakes and levels of NEFA and ß-OHB decreased by 90%, there was no increase in net hepatic lactate output. This supports the conclusion of Sindelar et al. that the change in lactate balance caused by a change in NEFAs was the result of an effect on the routing of glycogenolytically derived carbon (41). Although there was a moderate increase in net HGU during hyperinsulinemia, this was probably directed to glycogen. Even though a fall in NEFA level accompanied the increase in insulin, we did not observe a decrease in hepatic gluconeogenic flux to G6P or net gluconeogenic flux.

Insulin has been demonstrated to acutely inhibit gluconeogenic flux to G6P in vitro (7,8), and the process is known to be chronically increased by fasting (42) and diabetes (43,44). Conversely, acute effects of physiological changes in insulin on gluconeogenic flux to G6P in vivo have been difficult to demonstrate. The present experiments were designed, therefore, to investigate whether inhibiting glycogen breakdown in the presence of changes in insulin would allow an acute effect of the hormone on gluconeogenic flux to G6P to be observed. This was found to be the case during insulin deficiency, when an increase in gluconeogenic flux to G6P (and gluconeogenesis) was observed when the offsetting increase in glycogen breakdown was prevented. Whether this was due to low hepatic insulin receptor activation or an increase in plasma NEFA concentration or both remains unclear. During hyperinsulinemia, inhibition of gluconeogenic flux to G6P was not observed, however, despite inhibition of glycogen breakdown before insulin treatment. It is possible that the basal rate of gluconeogenic flux in the overnight-fasted euglycemic state cannot be acutely reduced by physiological levels of insulin. Gluconeogenesis itself was inhibited by the rise in insulin, but this was the result of redirection of gluconeogenically derived carbon to glycogen instead of plasma glucose. These data demonstrate that in the acute setting, the effects of insulin on glycogenolytic flux dominate changes in gluconeogenic flux to G6P.

	ACKNOWLEDGMENTS

 
This research was supported in part by National Institutes of Health Grants R37-DK18243 and DK14507 and the Clinical Nutrition Research Unit Grant P30-DK26657. D.S.E. was supported by the Vanderbilt Molecular Endocrinology Training Program (5 T 32 DK07563-12).

This work was presented in part at the 59th Annual Meeting of the American Diabetes Association, Chicago, IL, June 1999.

We thank Jon Hastings, Angelina Penaloza, Wanda Snead, Patrick Donahue, and Yang Ying for excellent technical support.

	FOOTNOTES

 
Address correspondence and reprint requests to Dale Edgerton, Department of Molecular Physiology and Biophysics, 702 Light Hall, Vanderbilt University School of Medicine, Nashville, TN 37232. E-mail: dale.edgerton{at}vanderbilt.edu.

Received for publication 10 January 2002 and accepted in revised form 5 July 2002.

A-V, arteriovenous; ß-OHB, ß-hydroxybutyrate; G6P, glucose-6-phosphate; G6Pase, glucose-6-phosphatase; GO, glucose oxidation; HGR, hepatic glucose release; HGU, hepatic glucose uptake; NEFA, nonesterified free fatty acid; NHB, net hepatic balance; NHGB, net hepatic glucose balance; NHGLY, net hepatic glycogenolytic flux; NHLB, net hepatic lactate balance; PC, pyruvate carboxylase; PEPCK, phosphoenol pyruvate carboxykinase; TNC, total net contribution.

	REFERENCES

TOP ABSTRACT INTRODUCTION RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 

1. Edgerton DS, Cardin S, Emshwiller M, Neal D, Chandramouli V, Schumann WC, Landau BR, Rossetti L, Cherrington AD: Small increases in insulin inhibit hepatic glucose production solely caused by an effect on glycogen metabolism. Diabetes50 :1872 –1882,2001[Abstract/Free Full Text]
2. Cherrington AD, Edgerton D, Sindelar DK: The direct and indirect effects of insulin on hepatic glucose production in vivo. Diabetologia41 :987 –996,1998[Medline]
3. Chiasson JL, Liljenquist JE, Finger FE, Lacy WW: Differential sensitivity of glycogenolysis and gluconeogenesis to insulin infusions in dogs. Diabetes25 :283 –291,1976[Abstract]
4. Yki-Jarvinen H, Helve E, Sane T, Nurjhan N, Taskinen MR: Insulin inhibition of overnight glucose production and gluconeogenesis from lactate in NIDDM. Am J Physiol256 :E732 –E739,1989[Abstract/Free Full Text]
5. Hellerstein MK, Neese RA, Schwarz JM, Turner S, Faix D, Wu K: Altered fluxes responsible for reduced hepatic glucose production and gluconeogenesis by exogenous glucose in rats. Am J Physiol272 :E163 –E172,1997[Abstract/Free Full Text]
6. Shikama H, Ui M: Glucose load diverts hepatic gluconeogenic product from glucose to glycogen in vivo. Am J Physiol235 :E354 –E360,1978
7. Hue L: Regulation of gluconeogenesis in liver. In Handbook of Physiology: The Endocrine Pancreas and Regulation of Metabolism. Jefferson L, Cherrington A, Eds. New York, Oxford University Press,2001 , p.649 –657
8. Pilkis SJ, Granner DK: Molecular physiology of the regulation of hepatic gluconeogenesis and glycolysis. Annu Rev Physiol54 :885 –909,1992[Medline]
9. Sindelar DK, Balcom JH, Chu CA, Neal DW, Cherrington AD: A comparison of the effects of selective increases in peripheral or portal insulin on hepatic glucose production in the conscious dog. Diabetes45 :1594 –1604,1996[Abstract]
10. Sindelar DK, Chu CA, Venson P, Donahue EP, Neal DW, Cherrington AD: Basal hepatic glucose production is regulated by the portal vein insulin concentration. Diabetes47 :523 –529,1998[Abstract]
11. Bergans N, Stalmans W, Goldmann S, Vanstapel F: Molecular mode of inhibition of glycogenolysis in rat liver by the dihydropyridine derivative, BAY R3401: inhibition and inactivation of glycogen phosphorylase by an activated metabolite. Diabetes49 :1419 –1426,2000[Abstract]
12. Cardin S, Jackson PA, Edgerton DS, Neal DW, Coffey CS, Cherrington AD: Effect of vagal cooling on the counterregulatory response to hypoglycemia induced by a low dose of insulin in the conscious dog. Diabetes50 :558 –564,2001[Abstract/Free Full Text]
13. Flattem N, Igawa K, Shiota M, Emshwiller MG, Neal DW, Cherrington AD: Alpha- and beta-cell responses to small changes in plasma glucose in the conscious dog. Diabetes50 :367 –375,2001[Abstract/Free Full Text]
14. Shiota M, Jackson PA, Bischoff H, McCaleb M, Scott M, Monohan M, Neal DW, Cherrington AD: Inhibition of glycogenolysis enhances gluconeogenic precursor uptake by the liver of conscious dogs. Am J Physiol273 :E868 –E879,1997[Abstract/Free Full Text]
15. Moore MC, Cherrington AD, Cline G, Pagliassotti MJ, Jones EM, Neal DW, Badet C, Shulman GI: Sources of carbon for hepatic glycogen synthesis in the conscious dog. J Clin Invest88 :578 –587,1991[Medline]
16. Lloyd B, Burrin J, Smythe P, Alberti KG: Enzymic fluorometric continuous-flow assays for blood glucose, lactate, pyruvate, alanine, glycerol, and 3-hydroxybutyrate. Clin Chem24 :1724 –1729,1978[Abstract/Free Full Text]
17. Michal G: D-glucose 6-phosphate and D-fructose 6-phosphate: D-glucopy-ranose 6-phosphate and D-fructofuranose 6-phosphate. In Methods of Enzymatic Analysis. Bergmeyer HU, Bergmeyer J, Grabl M, Eds. Basel, John Wiley & Sons,1981 , p.191 –198
18. Mari A: Estimation of the rate of appearance in the non-steady state with a two-compartment model. Am J Physiol263 :E400 –E415,1992[Abstract/Free Full Text]
19. Dobbins RL, Davis SN, Neal DW, Cobelli C, Cherrington AD: Pulsatility does not alter the response to a physiological increment in glucagon in the conscious dog. Am J Physiol266 :E467 –E478,1994[Abstract/Free Full Text]
20. Jungermann K, Katz N: Functional specialization of different hepatocyte populations. Physiol Rev69 :708 –764,1989[Abstract/Free Full Text]
21. Radziuk J, Pye S: Hepatic glucose uptake, gluconeogenesis and the regulation of glycogen synthesis. Diabetes Metab Res Rev17 :250 –272,2001[Medline]
22. Tappy L, Chiolero R, Berger M: Autoregulation of glucose production in health and disease. Curr Opin Clin Nutr Metab Care2 :161 –164,1999[Medline]
23. Wolfe RR, Volpi E: Insulin and protein metabolism. In Handbook of Physiology: The Endocrine Pancreas and Regulation of Metabolism. Jefferson L, Cherrington A, Eds. New York, Oxford University Press,2001 , p.735 –757
24. Taylor R, Shulman GI: Regulation of hepatic glucose uptake. In Handbook of Physiology: The Endocrine Pancreas and Regulation of Metabolism. Jefferson L, Cherrington A, Eds. New York, Oxford University Press,2001 , p.787 –802
25. Hornbuckle LA, Edgerton DS, Ayala JE, Svitek CA, Oeser JK, Neal DW, Cardin S, Cherrington AD, O’Brien RM: Selective tonic inhibition of G-6-Pase catalytic subunit, but not G-6-P transporter, gene expression by insulin in vivo. Am J Physiol Endocrinol Metab281 :E713 –E725,2001[Abstract/Free Full Text]
26. Boden G, Chen X, Capulong E, Mozzoli M: Effects of free fatty acids on gluconeogenesis and autoregulation of glucose production in type 2 diabetes. Diabetes50 :810 –816,2001[Abstract/Free Full Text]
27. Stingl H, Krssak M, Krebs M, Bischof MG, Nowotny P, Furnsinn C, Shulman GI, Waldhausl W, Roden M: Lipid-dependent control of hepatic glycogen stores in healthy humans. Diabetologia44 :48 –54,2001[Medline]
28. Roden M, Stingl H, Chandramouli V, Schumann WC, Hofer A, Landau BR, Nowotny P, Waldhausl W, Shulman GI: Effects of free fatty acid elevation on postabsorptive endogenous glucose production and gluconeogenesis in humans. Diabetes49 :701 –707,2000[Abstract]
29. Chen X, Iqbal N, Boden G: The effects of free fatty acids on gluconeogenesis and glycogenolysis in normal subjects. J Clin Invest103 :365 –372,1999[Medline]
30. Randle PJ: Regulatory interactions between lipids and carbohydrates: the glucose fatty acid cycle after 35 years. Diabetes Metab Rev14 :263 –283,1998[Medline]
31. Saloranta C, Franssila-Kallunki A, Ekstrand A, Taskinen MR, Groop L: Modulation of hepatic glucose production by non-esterified fatty acids in type 2 (non-insulin-dependent) diabetes mellitus. Diabetologia34 :409 –415,1991[Medline]
32. Boden G, Jadali F: Effects of lipid on basal carbohydrate metabolism in normal men. Diabetes40 :686 –692,1991[Abstract]
33. Johnston P, Hollenbeck C, Sheu W, Chen YD, Reaven GM: Acute changes in plasma non-esterified fatty acid concentration do not change hepatic glucose production in people with type 2 diabetes. Diabet Med7 :871 –875,1990[Medline]
34. Puhakainen I, Yki-Jarvinen H: Inhibition of lipolysis decreases lipid oxidation and gluconeogenesis from lactate but not fasting hyperglycemia or total hepatic glucose production in NIDDM. Diabetes42 :1694 –1699,1993[Abstract]
35. Friedmann B, Goodman EH Jr, Weinhouse S: Effects of insulin and fatty acids on gluconeogenesis in the rat. J Biol Chem242 :3620 –3627,1967[Abstract/Free Full Text]
36. Williamson JR, Browning ET, Scholz R: Control mechanisms of gluconeogenesis and ketogenesis. I. Effects of oleate on gluconeogenesis in perfused rat liver. J Biol Chem244 :4607 –4616,1969[Abstract/Free Full Text]
37. Williamson JR, Kreisberg RA, Felts PW: Mechanism for the stimulation of gluconeogenesis by fatty acids in perfused rat liver. Proc Natl Acad Sci U S A56 :247 –254,1966[Free Full Text]
38. Randle PJ, Priestman DA, Mistry SC, Halsall A: Glucose fatty acid interactions and the regulation of glucose disposal. J Cell Biochem55 :1 –11,1994[Medline]
39. Bahl JJ, Matsuda M, DeFronzo RA, Bressler R: In vitro and in vivo suppression of gluconeogenesis by inhibition of pyruvate carboxylase. Biochem Pharmacol53 :67 –74,1997[Medline]
40. Antras-Ferry J, Robin P, Robin D, Forest C: Fatty acids and fibrates are potent inducers of transcription of the phosphenolpyruvate carboxykinase gene in adipocytes. Eur J Biochem234 :390 –396,1995[Medline]
41. Sindelar DK, Chu CA, Rohlie M, Neal DW, Swift LL, Cherrington AD: The role of fatty acids in mediating the effects of peripheral insulin on hepatic glucose production in the conscious dog. Diabetes46 :187 –196,1997[Abstract]
42. Landau BR, Wahren J, Chandramouli V, Schumann WC, Ekberg K, Kalhan SC: Contributions of gluconeogenesis to glucose production in the fasted state. J Clin Invest98 :378 –385,1996[Medline]
43. Roden M, Petersen KF, Shulman GI: Nuclear magnetic resonance studies of hepatic glucose metabolism in humans. Recent Prog Horm Res56 :219 –237,2001[Abstract]
44. Dostou J, Gerich J: Pathogenesis of type 2 diabetes mellitus. Exp Clin Endocrinol Diabetes109 :S149 –S156,2001

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