Activities of glucokinase and hexokinase in mammalian and avian livers

J C Stanley; G L Dohm; B S McManus; E A Newsholme

doi:10.1042/bj2240667

Glycogen synthesis in the perfused liver of adrenalectomized rats

Biochemical Journal ◽

10.1042/bj1560585 ◽

1976 ◽

Vol 156 (3) ◽

pp. 585-592 ◽

Cited By ~ 17

Author(s):

P D Whitton ◽

D A Hems

Keyword(s):

Intact Animal ◽

Glycogen Synthesis ◽

Hepatic Metabolism ◽

Hepatic Glycogen ◽

Perfused Liver ◽

Short Term ◽

Glycogen Accumulation ◽

Glycogen Deposition ◽

Adrenalectomized Rats

1. A total loss of capacity for net glycogen synthesis was observed in experiments with the perfused liver of starved adrenalectomized rats. 2. This lesion was corrected by insulin or cortisol in vivo (over 2-5h), but not by any agent tested in perfusion. 3. The activity of glycogen synthetase a, and its increase during perfusion, in the presence of glucose plus glucogenic substrates, were proportional to the rate of net glycogen accumulation. 4. This complete inherent loss of capacity for glycogen synthesis after adrenalectomy is greater than any defect in hepatic metabolism yet reported in this situation, and is not explicable by a decrease in the rate of gluconegenesis (which supports glycogen synthesis in the liver of starved rats). The short-term (2-5h) stimulatory effect of glucocorticoids in the intact animal, on hepatic glycogen deposition, may be mediated partly through insulin action, although neither insulin or cortisol appear to act directly on the liver to stimulate glycogen synthesis.

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Arrestin domain-containing 3 (Arrdc3) modulates insulin action and glucose metabolism in liver

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1922370117 ◽

2020 ◽

Vol 117 (12) ◽

pp. 6733-6740 ◽

Cited By ~ 2

Author(s):

Thiago M. Batista ◽

Sezin Dagdeviren ◽

Shannon H. Carroll ◽

Weikang Cai ◽

Veronika Y. Melnik ◽

...

Keyword(s):

Messenger Rna ◽

Insulin Action ◽

Hepatic Glucose Production ◽

Glycogen Synthesis ◽

Glucose Production ◽

Hepatic Glycogen ◽

Glycogen Accumulation ◽

Hepatic Glucose ◽

Glucose Output

Insulin action in the liver is critical for glucose homeostasis through regulation of glycogen synthesis and glucose output. Arrestin domain-containing 3 (Arrdc3) is a member of the α-arrestin family previously linked to human obesity. Here, we show thatArrdc3is differentially regulated by insulin in vivo in mice undergoing euglycemic-hyperinsulinemic clamps, being highly up-regulated in liver and down-regulated in muscle and fat. Mice with liver-specific knockout (KO) of the insulin receptor (IR) have a 50% reduction inArrdc3messenger RNA, while, conversely, mice with liver-specific KO ofArrdc3(L-Arrdc3KO) have increased IR protein in plasma membrane. This leads to increased hepatic insulin sensitivity with increased phosphorylation of FOXO1, reduced expression of PEPCK, and increased glucokinase expression resulting in reduced hepatic glucose production and increased hepatic glycogen accumulation. These effects are due to interaction of ARRDC3 with IR resulting in phosphorylation of ARRDC3 on a conserved tyrosine (Y382) in the carboxyl-terminal domain. Thus,Arrdc3is an insulin target gene, and ARRDC3 protein directly interacts with IR to serve as a feedback regulator of insulin action in control of liver metabolism.

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DISTRIBUTION OF NEWLY SYNTHESIZED AMYLASE IN MICROSOMAL SUBFRACTIONS OF GUINEA PIG PANCREAS

The Journal of Cell Biology ◽

10.1083/jcb.30.3.519 ◽

1966 ◽

Vol 30 (3) ◽

pp. 519-530 ◽

Cited By ~ 22

Author(s):

P. Siekevitz ◽

G. E. Palade

Keyword(s):

Guinea Pig ◽

High Speed ◽

Specific Activity ◽

Specific Radioactivity ◽

Enzymic Activity ◽

Pellet Fraction ◽

Light Region ◽

Centrifuge Tube ◽

In Vivo Labeling

Amylase distribution was studied in guinea pig pancreas microsomes fractionated by centrifuging, for 2 hr at 57,000 g in a linear 10 to 30% sucrose gradient, a resuspended high speed pellet obtained after treating microsomes with 0.04% deoxycholate (DOC).1 Amylase appeared in the following positions in the gradient: (a) a light region which contained ∼35% of total enzymic activity and which coincided with a monomeric ribosome peak; (b) a heavy region which contained ∼10% of enzymic activity in a sharp peak but which had very little accompanying OD260 absorption; (c) a pellet at the bottom of the centrifuge tube which contained ∼20% of the enzymic activity. After 5 to 20 min' in vivo labeling with leucine-1-C14, radioactive amylase was solubilized from these three fractions by a combined DOC-spermine treatment and purified by precipitation with glycogen, according to Loyter and Schramm. In all cases, the amylase found in the pellet had five to ten times the specific activity (CPM/enzymic activity) of the amylase found in the light or heavy regions of the gradient. The specific radioactivity (CPM/mg protein) of the proteins or peptides not extracted by DOC-spermine was similar for all three fractions. Hypotonic treatment of the fractions solubilized ∼80% of the total amylase in the fraction from the heavy region of the gradient, but only ∼20% of the amylase in the monomer or pellet fraction. Electron microscope observation indicates that the monomer region of the gradient contained only ribosomes, that the heavy region of the gradient contained small vesicles with relatively few attached ribosomes, and that the pellet was composed mostly of intact or ruptured microsomes with ribosomes still attached to their membranes. It is concluded from the above, and from other evidence, that most of the amylase activity in the monomer region is due to old, adsorbed enzyme; in the heavy region mostly to enzyme already inside microsomal vesicles; and in the pellet to a mixture of newly synthesized and old amylase still attached to ribosomes. Furthermore, the ribosomes with nascent, finished protein still bound to them are more firmly attached to the membranes than are ribosomes devoid of nascent protein.

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Mechanism of delayed hepatic glycogen synthesis after an oral galactose load vs. an oral glucose load in adult rats

AJP Endocrinology and Metabolism ◽

10.1152/ajpendo.1992.263.1.e42 ◽

1992 ◽

Vol 263 (1) ◽

pp. E42-E49 ◽

Cited By ~ 3

Author(s):

C. B. Niewoehner ◽

B. Neil

Keyword(s):

Glucose Concentration ◽

Glycogen Synthesis ◽

Liver Glycogen ◽

Hepatic Glycogen ◽

Oral Glucose ◽

Glucose Load ◽

Adult Rats ◽

Glycogen Accumulation ◽

Glucose Administration

We have compared the effects of administration of oral galactose or glucose (1 g/kg) to 24-h fasted rats to examine the mechanism by which galactose regulates its own incorporation into liver glycogen in vivo. Liver glycogen increased to a maximum more slowly after galactose than after glucose administration (0.14 vs. 0.29 mumol.g liver-1.min-1). Glycogen accumulation after the galactose load was 70% of that after the glucose load (149 vs. 214 mumol), and the net increase in liver glycogen represented the same proportion (24 vs. 22%) of added carbohydrate after urinary loss of galactose was accounted for. Slower glycogen accumulation after galactose vs. glucose loading could not be explained by galactosuria, by differences in the active forms of synthase or phosphorylase, by end product (glycogen) inhibition of synthase phosphatase, or by different concentrations of the known allosteric effectors of synthase R plus I and phosphorylase a. Similar increases in glucose 6-phosphate were observed after both hexoses. AMP and ADP increased only transiently after galactose administration, and ATP, UTP, and Pi concentrations were unchanged. The UDP-glucose concentration decreased, whereas the UDP-galactose concentration increased two- to threefold after galactose but not glucose administration. The UDP-glucose pyrophosphorylase reaction is inhibited competitively by UDP-galactose. This could explain the decreased UDP-glucose concentration and the reduced rate of glycogen synthesis after galactose was given.

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Accelerated glycogenolysis in uremia and under sucrose feeding: role of phosphorylase alpha regulators

AJP Endocrinology and Metabolism ◽

10.1152/ajpendo.1997.273.1.e17 ◽

1997 ◽

Vol 273 (1) ◽

pp. E17-E27

Author(s):

Z. Bakkour ◽

D. Laouari ◽

S. Dautrey ◽

J. P. Yvert ◽

C. Kleinknecht

Keyword(s):

Hepatic Glucose Production ◽

Glycogen Synthesis ◽

Glucose Production ◽

Glycogen Storage ◽

Hepatic Insulin Resistance ◽

Hepatic Glycogen ◽

Glycogen Depletion ◽

Sucrose Feeding

To understand the mechanism of hepatic glycogen depletion found in uremia and under sucrose feeding, we examined net hepatic glycogenolysis-associated active enzymes and metabolites during fasting. Liver was taken 2, 7, and 18 h after food removal in uremic and pair-fed control rats fed either a sucrose or cornstarch diet for 21 days. Other uremic and control rats fasted for 18 h were refed a sucrose meal to measure glycogen increment. Glycogen storage in uremia was normal, suggesting effective glycogen synthesis. During a short fast, sucrose feeding and uremia enhanced net glycogenolysis through different but additive mechanisms. Under sucrose feeding, there were high phosphorylase alpha levels associated with hepatic insulin resistance. In uremia, phosphorylase alpha levels were low, but the enzyme was probably activated in vivo by a fall of inhibitors (ATP, alpha-glycerophosphate, fructose-1,6-diphosphate, and glucose) and a rise of Pi, as verified in vitro. Enhanced gluconeogenesis was also suggested, but excessive hepatic glucose production was unlikely in uremia. During fasting, hypoglycemia occurred in uremia due to reduced glycogenolysis, inefficient hepatic gluconeogenesis, and impaired renal gluconeogenesis. This may be relevant to poor fasting tolerance in uremia, which could be aggravated under excessive sucrose intake.

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Metabolic control analysis of hepatic glycogen synthesis in vivo

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.1921694117 ◽

2020 ◽

Vol 117 (14) ◽

pp. 8166-8176 ◽

Cited By ~ 4

Author(s):

Yuichi Nozaki ◽

Max C. Petersen ◽

Dongyan Zhang ◽

Daniel F. Vatner ◽

Rachel J. Perry ◽

...

Keyword(s):

Metabolic Control ◽

Glycogen Synthesis ◽

Metabolic Control Analysis ◽

Glucose Infusion ◽

Male Rats ◽

Hepatic Insulin Resistance ◽

Hepatic Glycogen ◽

Control Analysis ◽

Rate Controlling Step

Multiple insulin-regulated enzymes participate in hepatic glycogen synthesis, and the rate-controlling step responsible for insulin stimulation of glycogen synthesis is unknown. We demonstrate that glucokinase (GCK)-mediated glucose phosphorylation is the rate-controlling step in insulin-stimulated hepatic glycogen synthesis in vivo, by use of the somatostatin pancreatic clamp technique using [13C6]glucose with metabolic control analysis (MCA) in three rat models: 1) regular chow (RC)-fed male rats (control), 2) high fat diet (HFD)-fed rats, and 3) RC-fed rats with portal vein glucose delivery at a glucose infusion rate matched to the control. During hyperinsulinemia, hyperglycemia dose-dependently increased hepatic glycogen synthesis. At similar levels of hyperinsulinemia and hyperglycemia, HFD-fed rats exhibited a decrease and portal delivery rats exhibited an increase in hepatic glycogen synthesis via the direct pathway compared with controls. However, the strong correlation between liver glucose-6-phosphate concentration and net hepatic glycogen synthetic rate was nearly identical in these three groups, suggesting that the main difference between models is the activation of GCK. MCA yielded a high control coefficient for GCK in all three groups. We confirmed these findings in studies of hepatic GCK knockdown using an antisense oligonucleotide. Reduced liver glycogen synthesis in lipid-induced hepatic insulin resistance and increased glycogen synthesis during portal glucose infusion were explained by concordant changes in translocation of GCK. Taken together, these data indicate that the rate of insulin-stimulated hepatic glycogen synthesis is controlled chiefly through GCK translocation.

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A physiological increase in the hepatic glycogen level does not affect the response of net hepatic glucose uptake to insulin

AJP Endocrinology and Metabolism ◽

10.1152/ajpendo.00043.2009 ◽

2009 ◽

Vol 297 (2) ◽

pp. E358-E366 ◽

Cited By ~ 16

Author(s):

Jason J. Winnick ◽

Zhibo An ◽

Mary Courtney Moore ◽

Christopher J. Ramnanan ◽

Ben Farmer ◽

...

Keyword(s):

Glucose Uptake ◽

Glycogen Synthesis ◽

Control Period ◽

In Vivo Studies ◽

Hepatic Glycogen ◽

Glycogen Level ◽

Hepatic Glucose ◽

Glycogen Deposition ◽

Hepatic Glucose Uptake

To determine the effect of an acute increase in hepatic glycogen on net hepatic glucose uptake (NHGU) and disposition in response to insulin in vivo, studies were performed on two groups of dogs fasted 18 h. During the first 4 h of the study, somatostatin was infused peripherally, while insulin and glucagon were replaced intraportally in basal amounts. Hyperglycemia was brought about by glucose infusion, and either saline ( n = 7) or fructose ( n = 7; to stimulate NHGU and glycogen deposition) was infused intraportally. A 2-h control period then followed, during which the portal fructose and saline infusions were stopped, allowing NHGU and glycogen deposition in the fructose-infused animals to return to rates similar to those of the animals that received the saline infusion. This was followed by a 2-h experimental period, during which hyperglycemia was continued but insulin infusion was increased fourfold in both groups. During the initial 4-h glycogen loading period, NHGU averaged 1.18 ± 0.27 and 5.55 ± 0.53 mg·kg−1·min−1 and glycogen synthesis averaged 0.72 ± 0.24 and 3.98 ± 0.57 mg·kg−1·min−1 in the saline and fructose groups, respectively ( P < 0.05). During the 2-h hyperinsulinemic period, NHGU rose from 1.5 ± 0.4 and 0.9 ± 0.2 to 3.1 ± 0.6 and 2.5 ± 0.5 mg·kg−1·min−1 in the saline and fructose groups, respectively, a change of 1.6 mg·kg−1·min−1 in both groups despite a significantly greater liver glycogen level in the fructose-infused group. Likewise, the metabolic fate of the extracted glucose (glycogen, lactate, or carbon dioxide) was not different between groups. These data indicate that an acute physiological increase in the hepatic glycogen content does not alter liver glucose uptake and storage under hyperglycemic/hyperinsulinemic conditions in the dog.

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Glycogen synthesis in the perfused liver of the starved rat

Biochemical Journal ◽

10.1042/bj1290529 ◽

1972 ◽

Vol 129 (3) ◽

pp. 529-538 ◽

Cited By ~ 88

Author(s):

D. A. Hems ◽

P. D. Whitton ◽

E. A. Taylor

Keyword(s):

Time Course ◽

Sequential Sampling ◽

Glycogen Synthesis ◽

Lateral Lobe ◽

Hepatic Glycogen ◽

Perfused Liver ◽

Glycogen Deposition ◽

Glucose Dependence

1. In the isolated perfused liver from 48h-starved rats, glycogen synthesis was followed by sequential sampling of the two major lobes. 2. The fastest observed rates of glycogen deposition (0.68–0.82μmol of glucose/min per g fresh liver) were obtained in the left lateral lobe, when glucose in the medium was 25–30mm and when gluconeogenic substrates were present (pyruvate, glycerol and serine: each initially 5mm). In this situation there was no net disappearance of glucose from the perfusion medium, although 14C from [U-14C]glucose was incorporated into glycogen. There was no requirement for added hormones. 3. In the absence of gluconeogenic precursors, glycogen synthesis from glucose (30mm) was 0–0.4μmol/min per g. 4. When livers were perfused with gluconeogenic precursors alone, no glycogen was deposited. The total amount of glucose formed was similar to the amount converted into glycogen when 30mm-glucose was also present. 5. The time-course, maximal rates and glucose dependence of hepatic glycogen deposition in the perfused liver resembled those found in vivo in 48h-starved rats, during infusion of glucose. 6. In the perfused liver, added insulin or sodium oleate did not significantly affect glycogen synthesis in optimum conditions. In suboptimum conditions (i.e. glucose less than 25mm, or with gluconeogenic precursors absent) insulin caused a moderate acceleration of glycogen deposition. 7. These results suggest that on re-feeding after starvation in the rat, hepatic glycogen deposition could be initially the result of continued gluconeogenesis, even after the ingestion of glucose. This conclusion is discussed, particularly in connexion with the role of hepatic glucokinase, and the involvement of the liver in the glucose intolerance of starvation.

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The activity of glycogen synthase phosphatase limits hepatic glycogen deposition in the adrenalectomized starved rat

Biochemical Journal ◽

10.1042/bj2140539 ◽

1983 ◽

Vol 214 (2) ◽

pp. 539-545 ◽

Cited By ~ 12

Author(s):

M Bollen ◽

G Gevers ◽

W Stalmans

Keyword(s):

Phosphatase Activity ◽

Protein Phosphatase ◽

Glycogen Synthase ◽

Glycogen Synthesis ◽

Hepatic Glycogen ◽

Complete Inactivation ◽

Glycogen Deposition ◽

Initial Recovery ◽

No Activation

Hepatocytes from adrenalectomized 48 h-starved rats responded to increasing glucose concentrations with a progressively more complete inactivation of phosphorylase. Yet no activation of glycogen synthase occurred, even in a K+-rich medium. Protein phosphatase activities in crude liver preparations were assayed with purified substrates. Adrenalectomy plus starvation decreased synthase phosphatase activity by about 90%, but hardly affected phosphorylase phosphatase activity. Synthase b present in liver extracts from adrenalectomized starved rats was rapidly and completely converted into the a form on addition of liver extract from a normal fed rat. Glycogen synthesis can be slowly re-induced by administration of either glucose or cortisol to the deficient rats. In these conditions there was a close correspondence between the initial recovery of synthase phosphatase activity and the amount of synthase a present in the liver. The latter parameter was strictly correlated with the measured rate of glycogen synthesis in vivo. The decreased activity of synthase phosphatase emerges thus as the single factor that limits hepatic glycogen deposition in the adrenalectomized starved rat.

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Glycogen synthesis in the perfused liver of streptozotocin-diabetic rats

Biochemical Journal ◽

10.1042/bj1500153 ◽

1975 ◽

Vol 150 (2) ◽

pp. 153-165 ◽

Cited By ~ 85

Author(s):

P D Whitton ◽

D A Hems

Keyword(s):

Direct Action ◽

Glycogen Synthesis ◽

Diabetic Rats ◽

Hepatic Glycogen ◽

Perfused Liver ◽

Glycogen Accumulation ◽

Glycogen Synthetase ◽

Streptozotocin Diabetic Rats

1. Net glycogen accumulation was measured in sequentially removed samples during perfusion of the liver of starved streptozotocin-diabetic rats, and shown to be significantly impaired, compared with rates in normal (starved) rats. 2. In perfusions of normal livers with glucose plus C3 substrates, there was an increase in the proportion of glycogen synthetase ‘a’, compared with that in the absence of substrates. This response to substrates, followed in sequential synthesis and enzymic sensitivity in the perfused liver of diabetic rats were reversed by pretreatment in vivo with glucose plus fructose, or insulin. Glucose alone did not produce this effect. 4. Glucose, fructose, insulin or cortisol added to e perfusion medium (in the absence of pretreatment in vivo) did not stimulate glycogen synthesis in diabetic rats. 5. In intact diabetic rats, there was a decline in rates of net hepatic glycogen accumulation, and the response of glycogen synthetase to substrates. The most rapid rates of synthesis were obtained after fructose administration. 6. These results demonstrate that there is a marked inherent impairment in hepatic glycogen synthesis in starved diabetic rats, which can be rapidly reversed in vivo but no in perfusion. Thus hepatic glycogen synthesis does not appear to be sensitive to either the short-term direct action of insulin (added alone to perfusions) of to long-term insulin deprivation in vivo. The regulatory roles of substrates, insulin and glycogen synthetase in hepatic glycogen accumulation are discussed.

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