14 results on '"Damgaard SE"'
Search Results
2. Primary deuterium and tritium isotope effects upon V/K in the liver alcohol dehydrogenase reaction with ethanol.
- Author
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Damgaard SE
- Subjects
- Alcohol Dehydrogenase, Hydrogen-Ion Concentration, Kinetics, Mathematics, NAD metabolism, Alcohol Oxidoreductases metabolism, Deuterium metabolism, Ethanol metabolism, Liver enzymology, Tritium metabolism
- Abstract
The primary isotope effect upon V/K when ethanol stereospecifically labeled with deuterium or tritium is oxidized by liver alcohol dehydrogenase has been measured between pH 6 and 9. The deuterium isotope effect was obtained with high reproducibility by the use of two different radioactive tracers, viz. 14C and 3H, to follow the rate of acetaldehyde formation from deuterium-labeled ethanol and normal ethanol, respectively. Synthesis of the necessary labeled compounds is described in this and earlier work referred to. V/K isotope effects for both tritium and deuterium have been measured with three different coenzymes, NAD+, thio-NAD+, and acetyl-NAD+. With NAD+ at pH 7, D(V/K) was 3.0 and T(V/K) was 6.5. With increasing pH, these values decreased to 1.5 and 2.5 at pH 9. The intrinsic isotope effect evaluated by the method of Northrop [Northrop, D.B. (1977) in Isotope Effects on Enzyme-Catalyzed Reactions (Cleland, W. W., O'Leary, M, H., & Northrop, D. B., Eds.) pp 112-152, University Park Press, Baltimore] varies little with pH. It amounts to about 10 with NAD+ and about 5 with the coenzyme analogues. Commitment functions and their dependence upon pH calculated in this connection appear to be in agreement with known kinetic parameters of liver alcohol dehydrogenase. This assay method was also applied in vivo in the rat. Being a noninvasive method because only trace amounts of isotopes are needed, it may yield information about alternative routes of ethanol oxidation in vivo. In naive rats at low concentrations of ethanol, it confirms the discrete role of the non alcohol dehydrogenase systems.
- Published
- 1981
- Full Text
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3. Isotope effect in peroxidation of deuterium-labelled ethanol by liver catalase.
- Author
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Damgaard SE
- Subjects
- Animals, Carbon Radioisotopes, Female, Kinetics, Peroxides, Rats, Tritium, Catalase metabolism, Deuterium, Ethanol metabolism, Liver enzymology
- Abstract
The kinetic V/K isotope effect upon peroxidation of (1R)-[1-2H1]ethanol by liver catalase was studied by using a radiochemical assay with both 3H ad 14C as tracers. The value of 1.9 found is in agreement with the value of 2.52 for peroxidation of (1R)-[1-3H1]ethanol according to the 'Swain equation' [Swain, Stivers, Ruver & Schaad (1958) J. Am. Chem. Soc. 80, 5885-5893]. There was no isotope effect on V, the catalase haem up to 500 min-1. Even at rates 20-fold higher the isotope effect on V may not be different from 1. A detailed description of the synthesis of the 2H- and 3H-substituted ethanol compounds and the analysis of these has been deposited as Supplementary Publication SUP 50110 (5 pages) at the British Library Lending Division, Boston Spa, Wetherby, W. Yorkshire LS23 7BQ, U.K., from whom copies can be obtained on the terms indicated in Biochem. J. (1978) 169,5.
- Published
- 1980
- Full Text
- View/download PDF
4. Metabolism of palmitate in perfused rat liver. Effect of ethanol in livers from rats fed on a high-fat diet with or without ethanol.
- Author
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Kondrup J, Lundquist F, and Damgaard SE
- Subjects
- Animals, Female, Glycerides metabolism, Liver drug effects, Perfusion, Phospholipids metabolism, Rats, Subcellular Fractions metabolism, Triglycerides metabolism, Dietary Fats pharmacology, Ethanol pharmacology, Liver metabolism, Palmitates metabolism, Palmitic Acids metabolism
- Abstract
1. Rats were treated for 4 weeks with liquid diets that contained, on the basis of energy content, 35% fat, 18% protein and 47% carbohydrate (high-fat diet) or 35% fat, 18% protein, 11% carbohydrate and 36% ethanol (high-fat/ethanol diet). 2. The livers were perfused with 1mm-[1-(14)C]palmitate and with 0, 10mm- or 80mm-ethanol. The oxidation and esterification of palmitate was measured. Two subcellular pools of triacylglycerol were separated; one contained triacylglycerol from cytoplasmic lipid droplets and the other contained triacylglycerol from the endoplasmic reticulum and Golgi apparatus. 3. In the presence of ethanol, liver from rats fed on the high-fat diet esterified about 70% of the [1-(14)C]palmitate taken up compared with 90% in liver from rats fed chow (containing 11% fat on the basis of energy content). Compared with chow diet the high-fat diet did not potentiate the effect of ethanol on storage of [1-(14)C]palmitate in hepatic triacylglycerol. The relation between the fat content of the diet and the degree of fatty liver induced by by ethanol [Lieber & DeCarli (1970) Am. J. Clin. Nutr.23, 474-478] is discussed. 4. The ethanol-containing diet increased the hepatic content of triacylglycerol 4-fold and the increase was exclusively found in the fraction suggested to contain lipid from cytoplasmic lipid droplets. The ethanol-induced fatty liver, perfused with ethanol, esterified and oxidized palmitate at rates that were quite similar to the rates found in high-fat control livers perfused without ethanol. This suggests that the fatty liver had adapted to the presence of ethanol with respect to palmitate metabolism. 5. O(2) and ethanol uptake by the livers were not affected by the ethanol-containing diet.
- Published
- 1979
- Full Text
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5. Determination of acetaldehyde in human blood using thiourea to inhibit ethanol interference.
- Author
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Iversen HL and Damgaard SE
- Subjects
- Chromatography, Gas, Ethanol blood, Humans, Microchemistry, Tritium, Acetaldehyde blood, Thiourea
- Abstract
Determination of acetaldehyde in human blood by the semicarbazide method has been studied. An artefactual production of acetaldehyde from ethanol in blood and plasma of about 20 mumol/l was observed at concentrations of ethanol of about 60 mmol/l. This artefact was reduced to less than 1 mumol/l after addition of thiourea. The presumably non-enzymatic production of acetaldehyde from ethanol was demonstrated by the release of 3H from (1R)-[3H]ethanol added to the blood immediately after sampling. The results demonstrate that oxidation of ethanol is the major cause of the artefactual acetaldehyde formation. In human volunteers, metabolising ethanol, very low concentrations of acetaldehyde were found by the modified method, which includes thiourea.
- Published
- 1983
- Full Text
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6. Metabolism of palmitate in perfused rat liver. Computer models of subcellular triacylglycerol metabolism.
- Author
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Kondrup J, Damgaard SE, and Fleron P
- Subjects
- Animals, Computers, Diglycerides metabolism, Fatty Acids analysis, Female, Perfusion, Rats, Subcellular Fractions metabolism, Liver metabolism, Models, Biological, Palmitates metabolism, Palmitic Acids metabolism, Triglycerides metabolism
- Abstract
1. In the preceding paper [Kondrup (1979) Biochem. J.184, 63-71] the separation of two major fractions of hepatic triacylglycerol was described. One fraction contained triacylglycerol from the endoplasmic reticulum and from the Golgi apparatus. The other fraction contained triacylglycerol from the cytoplasmic lipid droplets. In the present paper possible precursor-product relationships between the two fractions were investigated by means of computer models. 2. The fatty acids present in di- and tri-acylglycerol in the fractions isolated in the time studies were analysed by gas chromatography. From this analysis the relative specific radioactivities, and contents, of palmitate in acylglycerols in the two fractions at the various time points were calculated. 3. A computer was used to predict relative specific radioactivities of pools in defined models of hepatic triacylglycerol metabolism. The acceptability of the models was evaluated by comparing predicted with measured relative specific radioactivities. 4. It is suggested that triacylglycerol in cytoplasmic lipid droplets does not originate (a) directly from triacylglycerol in the endoplasmic reticulum, (b) from a sub-pool of it or (c) directly from non-esterified fatty acids entering the cell. Rather, it is formed from diacylglycerol (and acyl-CoA) in the endoplasmic reticulum. Diacylglycerol, on the other hand, is furnished in part by hydrolysis of triacylglycerol in the endoplasmic reticulum. 5. This suggestion is discussed in relation to previous models of hepatic fatty acid metabolism.
- Published
- 1979
- Full Text
- View/download PDF
7. Ethanol metabolism in heavy drinkers after massive and moderate alcohol intake.
- Author
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Keiding S, Christensen NJ, Damgaard SE, Dejgård A, Iversen HL, Jacobsen A, Johansen S, Lundquist F, Rubinstein E, and Winkler K
- Subjects
- Epinephrine blood, Humans, Kinetics, Male, Norepinephrine blood, Alcohol Drinking physiology, Alcoholism metabolism, Ethanol metabolism
- Abstract
Some alcoholics have a regular daily alcohol consumption of more than 100 g. In preliminary observations we had the impression that the claimed alcohol intake in such 'heavy drinkers' was higher than could be accounted for by the ethanol elimination rate as measured routinely at 10 mmol/l (0.5 g/l). We therefore measured the ethanol elimination rate at very high blood ethanol concentrations of 40-80 mmol/l (2-4 g/l) found in eight alcoholics following heavy alcohol intake by measuring the falling blood ethanol concentrations until being less than 1 mmol/l. The elimination rate, on average 83 mumol/min per 1 blood, was about 49% higher than the elimination rate measured at 10 mmol/l in the same subject, being on average 58 mumol/min per 1/blood (paired t-test, P less than 0.05). The elimination rate following the high initial ethanol concentrations remained high until the concentration was below 5 mmol/l. Calculations of elimination rates are based on a number of assumptions concerning the physiologic and metabolic conditions. We examined specifically if the concentration-time curves could be adequately described by assuming metabolism according to a Michaelis-Menten pathway with a low Km value (simulating alcoholdehydrogenase with Km 0.2 mmol/l) or by assuming metabolism by two pathways with an alternative high-Km pathway with Km about 10 mmol/l. It was not necessary, in the statistical analysis, to include an alternative high-Km pathway. On the other hand, the data does give room for up to 50% elimination via such alternative pathways. The elimination rate at the high concentrations corresponded roughly to the claimed daily alcohol intake; furthermore the measured elimination rate at the lower concentrations were similar to values in non-alcoholics.
- Published
- 1983
- Full Text
- View/download PDF
8. Tritium effect in peroxidation of ehtanol by liver catalase.
- Author
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Damgaard SE
- Subjects
- Acetaldehyde metabolism, Animals, Catalysis, Cattle, Hydrogen Peroxide metabolism, Hydrogen-Ion Concentration, Kinetics, Pyrazoles, Rats, Spectrum Analysis, Catalase metabolism, Ethanol metabolism, Liver enzymology, Tritium
- Abstract
1. Simultaneous determination of the rate of appearance of 3H in water from [(1R)-1-3H1] ethanol and the rate of acetaldehyde formation in the presence of rat or ox liver catalase under conditions of steady-state generation of H2O2 allowed calculation of the 3H isotope effect. The mean value of 2.52 obtained for rat liver catalase at 37 degrees C and pH 6.3-7.7 was independent of both ethanol concentration and the rate of H2O2 generation over a wide range. At 25 degrees C a slightly lower mean value of 2.40 was obtained with the ox liver catalase. 2. Neither the product, acetaldehyde, nor 4-methylpyrazole influenced the two rates measured in the assay. 3. Relating the value obtained for the 3H isotope effect to a known value for the 2H isotope effect strongly supports the view that both values are close to the true isotope effect with the respective substituted compounds on the rate constant in the catalytic step involving scission of the C-H bond. 4. The constancy of the isotope effect under various conditions makes it possible to use it for interpretations in vivo. 5. It was established that beta-D-galactose dehydrogenase exhibits B-specificity towards the nicotinamide ring in NAD.
- Published
- 1977
- Full Text
- View/download PDF
9. Metabolism of palmitate in perfused rat liver. Effect of low and high ethanol concentrations at various concentrations of palmitate in the perfusion medium.
- Author
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Kondrup J, Lundquist F, and Damgaard SE
- Subjects
- Animals, Cytoplasm metabolism, Female, Glycerides metabolism, Liver drug effects, Oxygen metabolism, Perfusion, Phospholipids metabolism, Rats, Subcellular Fractions metabolism, Triglycerides metabolism, Ethanol pharmacology, Liver metabolism, Palmitates metabolism, Palmitic Acids metabolism
- Abstract
1. The effect of ethanol on the metabolism of [1-(14)C]palmitate in rat liver was investigated in a single-pass perfusion system at concentrations of 10mm- or 80mm-ethanol and 0.2mm- or 1mm-palmitate. 2. After the perfusion the hepatic lipid was isolated in subcellular fractions. The two major fractions contained triacylglycerol from cytoplasmic lipid droplets and from endoplasmic reticulum plus Golgi apparatus respectively. 3. In experiments with 0.2mm-palmitate perfusion with 10mm- or 80mm-ethanol did not measurably increase the esterification, and the oxidation was markedly decreased and the fatty acid uptake was not affected. 4. Perfusion with ethanol, at 1mm-palmitate, increased the fatty acid uptake, increased esterification and decreased oxidation. The effects of 10mm- and 80mm-ethanol were similar. The incorporation of [1-(14)C]palmitate into triacylglycerol in cytoplasmic lipid droplets was not affected statistically significantly by ethanol. Ethanol increased the incorporation of [1-(14)C]palmitate into di- and tri-acylglycerol in the membranous fraction. Estimated chemically, the contents of di- and tri-acylglycerol were only slightly affected by ethanol. These results suggest that the effect of ethanol was to increase the turnover of fatty acids in triacylglycerol rather than to increase its accumulation. 5. The results indicate that an increased concentration of fatty acids is more important for the formation of acute fatty liver in fed rats than are the direct effects of ethanol on hepatic fatty acid metabolism.
- Published
- 1979
- Full Text
- View/download PDF
10. Fructose and D-glyceraldehyde metabolism in the isolated perfused pig liver.
- Author
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Sestoft L, Tonnesen K, Hansen FV, and Damgaard SE
- Subjects
- Alcohol Oxidoreductases metabolism, Animals, Biotransformation, Female, Fructose-Bisphosphate Aldolase antagonists & inhibitors, Fructosephosphates metabolism, Glyceric Acids, Kinetics, Lactates biosynthesis, Liver enzymology, Manometry, Oxygen Consumption, Perfusion, Phosphotransferases metabolism, Swine, Fructose metabolism, Glyceraldehyde metabolism, Liver metabolism
- Published
- 1972
- Full Text
- View/download PDF
11. The interrelationship between fructose and ethanol metabolism in the isolated perfused pig liver.
- Author
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Damgaard SE, Sestoft L, Lundquist F, and Tygstrup N
- Subjects
- Acetates metabolism, Alcohol Oxidoreductases metabolism, Animals, Dinitrophenols pharmacology, Fructose pharmacology, Glyceraldehyde metabolism, Glyceraldehyde pharmacology, Liver drug effects, Liver enzymology, Malate Dehydrogenase metabolism, Mitochondria, Liver drug effects, Mitochondria, Liver metabolism, NAD metabolism, NADP metabolism, Oxidation-Reduction, Oxidative Phosphorylation, Oxygen Consumption, Perfusion, Pyrazoles pharmacology, Pyruvates pharmacology, Stimulation, Chemical, Swine, Ethanol metabolism, Fructose metabolism, Liver metabolism
- Published
- 1972
- Full Text
- View/download PDF
12. Utilization of acetate in the human forearm during exercise after ethanol ingestion.
- Author
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Lundquist F, Sestoft L, Damgaard SE, Clausen JP, and Trap-Jensen J
- Subjects
- Acetates blood, Adult, Blood Flow Velocity, Blood Glucose analysis, Ethanol blood, Fatty Acids blood, Glycerol blood, Humans, Lactates blood, Male, Acetates metabolism, Ethanol metabolism, Forearm metabolism, Muscles metabolism, Physical Exertion
- Abstract
The uptake of acetate in the human forearm was studied in five fasting (14 h) subjects during 10-min periods of ergometer work at 7 and 10 kilopond-meters per minute (kpm/min). A constant arterial acetate concentration was established by administration of a small quantity of alcohol (25 g) to the subjects after a control work period. Blood flow was measured by an indicator dilution technique. Acetate uptake varied linearly with the product of arterial acetate concentration and blood flow. Acetate metabolism was calculated to account for about 6.5% of the energy metabolism, assuming complete combustion to carbon dioxide and water. Oxygen uptake and blood flow did not change in the presence of acetate and ethanol. After administration of ethanol the arterial concentrations of FFA and glycerol decreased to about half, whereas the lactate concentration increased to about twice the control values, confirming other reports. Glucose utilization was increased and lactate output decreased during the ethanol periods, presumably a consequence of the changing arterial concentrations and increased insulin level. Measurements of the arterial and venous lactate/pyruvate concentration ratios indicate that the NAD-mediated cytoplasmic redox state in the muscle is not changed in the presence of acetate and ethanol.
- Published
- 1973
- Full Text
- View/download PDF
13. Metabolism of ethanol and fructose in the isolated perfused pig liver.
- Author
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Damgaard SE, Lundquist F, Tonnesen K, Hansen FV, and Sestoft L
- Subjects
- Acetates metabolism, Animals, Cytosol metabolism, Ethanol pharmacology, Glyceraldehyde pharmacology, Glycerophosphates metabolism, Ketone Bodies metabolism, Lactates metabolism, Liver drug effects, NAD, Oxidation-Reduction, Perfusion, Pyruvates metabolism, Sorbitol metabolism, Stimulation, Chemical, Swine, Ethanol metabolism, Fructose pharmacology, Liver metabolism
- Published
- 1973
- Full Text
- View/download PDF
14. Effect of fructose and glyceraldehyde on ethanol metabolism in human liver and in rat liver.
- Author
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Thieden HI, Grunnet N, Damgaard SE, and Sestoft L
- Subjects
- Acetaldehyde, Alcohol Oxidoreductases, Aldehyde Oxidoreductases, Animals, Ethanolamines, Female, Fructose-Bisphosphate Aldolase, Glyceric Acids, Humans, Kinetics, Liver drug effects, Malate Dehydrogenase metabolism, NAD, NADP, Oxaloacetates metabolism, Phosphotransferases, Pyruvates pharmacology, Rats, Sorbitol, Trioses, Ethanol metabolism, Fructose pharmacology, Glyceraldehyde pharmacology, Liver enzymology
- Published
- 1972
- Full Text
- View/download PDF
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