Departments of 1 Medicine and 2 Physiology and Pharmacology, University of Rochester School of Medicine, Rochester, New York 14642
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ABSTRACT |
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Recent studies indicate a role for the kidney in postabsorptive glucose homeostasis. The present studies were undertaken to evaluate the role of the kidney in postprandial glucose homeostasis and to compare its contribution to that of liver and skeletal muscle. Accordingly, we used the double isotope technique along with forearm and renal balance measurements to assess systemic, renal, and hepatic glucose release as well as glucose uptake by kidney, skeletal muscle, and splanchnic tissues in 10 normal volunteers after ingestion of 75 g of glucose. We found that, during the 4.5-h postprandial period, 22 ± 2 g (30 ± 3% of the ingested glucose) were initially extracted by splanchnic tissues. Of the remaining 53 ± 2 g that entered the systemic circulation, 19 ± 3 g were calculated to have been taken up by skeletal muscle and 7.5 ± 1.7 g by the kidney (26 ± 3 and 10 ± 2%, respectively, of the ingested glucose). Endogenous glucose release during the postprandial period (16 ± 2 g), calculated as the difference between overall systemic glucose appearance and the appearance of ingested glucose in the systemic circulation, was suppressed 61 ± 3%. Surprisingly, renal glucose release increased twofold (10.6 ± 2.5 g) and accounted for ~60% of postprandial endogenous glucose release. Hepatic glucose release (6.7 ± 2.2 g), the difference between endogenous and renal glucose release, was suppressed 82 ± 6%. These results demonstrate a hitherto unappreciated contribution of the kidney to postprandial glucose homeostasis and indicate that postprandial suppression of hepatic glucose release is nearly twofold greater than had been calculated in previous studies (42 ± 4%), which had assumed that there was no renal glucose release. We postulate that increases in postprandial renal glucose release may play a role in facilitating efficient liver glycogen repletion by permitting substantial suppression of hepatic glucose release.
gluconeogenesis; glycogenolysis; glucose disposal
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INTRODUCTION |
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CONSIDERABLE INFORMATION has recently accumulated regarding postprandial glucose homeostasis. It appears that about one-third of ingested carbohydrate is immediately taken up by splanchnic tissues (5, 22, 33-35, 37, 38, 44, 60). Of the remaining two-thirds of the ingested carbohydrate that enters the systemic circulation, some is extracted by the liver (23), but most is taken up by peripheral tissues. Limb balance measurements indicate that skeletal muscle is the predominant site for this peripheral glucose disposal, being responsible for about one-fourth of the ingested carbohydrate (5, 26, 33-35, 37, 38, 44). The fate of the remaining 40% of the ingested carbohydrate is less clear.
In addition to tissue uptake of ingested carbohydrate, another important factor for postprandial glucose homeostasis is suppression of the release of glucose endogenously produced by gluconeogenesis and breakdown of stored glycogen (18, 33, 44). Until recently, this was thought to occur almost exclusively in the liver (51). Most (7, 8, 39-42, 45, 49, 50, 52) but not all (21) recent studies indicate that, in postabsorptive normal volunteers, the kidney may account for 15-25% of all glucose released into the circulation. However, it should be pointed out that bias in the handling of data in some of these studies (39-42, 45, 49, 50, 52) may have led to an overestimation of renal glucose release (28). Recent studies also indicate that renal release of glucose, like that of the liver, is regulated by insulin (9, 40) and counterregulatory hormones (10, 39, 49). These findings suggest that the kidney may also be involved in postprandial glucose homeostasis.
Changes in renal glucose metabolism after carbohydrate ingestion have not, to our knowledge, been previously investigated. Certain considerations, however, indicate that the kidney may play a role. Normally, renal glucose fractional extraction in the postabsorptive state is 1-2% (7, 8, 21, 39-42, 49, 50, 52). Should this persist postprandially, the kidney could be a site of considerable glucose disposal. Moreover, previous studies have estimated postprandial hepatic glucose release merely as the difference between total systemic glucose appearance and the appearance of ingested glucose in the systemic circulation, ignoring the potential contribution of the kidney (5, 22, 26, 33-35, 37, 38, 44). Consequently, postprandial hepatic glucose release has been overestimated, and the importance of its suppression may also have been overestimated if there were concomitant suppression of renal glucose release.
The present studies were therefore undertaken to quantitate the contribution of the kidney to postprandial glucose homeostasis and to reassess the magnitude of postprandial suppression of hepatic glucose release. Moreover, we also simultaneously evaluated muscle glucose uptake and its net release of potential gluconeogenic precursors so as to obtain a more complete view of postprandial glucose homeostasis.
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METHODS |
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Subjects.
Informed written consent was obtained from 10 healthy volunteers after
the protocol had been approved by The University of Rochester
Institutional Review Board. The subjects (5 men, 5 women 49 ± 2 yr of age) had normal physical examinations, routine laboratory tests,
and glucose tolerance (World Health Organization criteria) (59), as well as no family history of diabetes mellitus.
For 3 days before the study, all had been on a weight-maintaining diet
containing 200 g carbohydrate and had abstained from alcohol.
Protocol. Subjects were admitted to the University of Rochester General Clinical Research Center between 6:00 and 7:00 PM the evening before experiments, consumed a standard meal between 6:30 and 8:00 PM, and fasted thereafter.
At ~5:30 AM, an antecubital vein was cannulated, and primed continuous infusions of [6-3H]glucose (~75 µCi, ~0.75 µCi/min; Amersham Biosciences, Arlington Heights, IL) was started. At ~8:00 AM, an infusion of p-aminohippuric acid (12 mg/min) was started for determination of renal blood flow (RBF). In addition, five subjects also received an infusion of [9,10-3H]palmitate; their baseline data have been previously reported (41). Between 8:00 and 9:00 AM, a renal vein was catheterized under fluoroscopy and the position of the catheter tip ascertained by injecting a small amount of iodinated contrast material. At ~9:00 AM, a dorsal hand vein was cannulated and kept in a thermoregulated Plexiglas box at 65°C for sampling arterialized venous blood, and a large antecubital vein was cannulated retrogradely in the contralateral arm for sampling of the deep venous system of the forearm, as previously described (34). About 1 h later, simultaneous blood sampling was started from the dorsal hand vein, the renal vein, and the antecubital vein at 30-min intervals for the next 5.5 h. After the 60-min baseline period, each subject ingested 75 g of glucose as an oral glucose solution (Dextrol, American Scientific Products, McGaw Park, IL) containing 3 g of [6,6-2H2]glucose for determination of the rate of appearance of the ingested glucose in the systemic circulation.Analytical procedures. Blood samples were collected for glucose, lactate, alanine, and glycerol concentrations, [6-3H]glucose specific activities, and [6,6-2H2]glucose enrichments in oxalate-fluoride tubes for free fatty acid (FFA) concentrations in EDTA tubes and for insulin and glucagon concentrations in EDTA tubes containing a protease inhibitor. Whole blood glucose was immediately determined in triplicate with a glucose analyzer (Yellow Springs Instrument, Yellow Springs, OH) with a coefficient of variation (CV) of 0.9%. For other determinations, samples were placed immediately in a 4°C ice bath, and plasma was separated within 30 min by centrifugation at 4°C. [6-3H]glucose specific activities were determined using 4 ml of plasma in duplicate by HPLC (46) with a CV of 0.5%. Plasma [6,6-2H2]glucose enrichments were determined by gas chromatography-mass spectroscopy (GC-MS) as previously described (14). Plasma lactate, alanine, glycerol, and FFA concentrations were determined by standard microfluorometric assays (36, 43, 56). Plasma insulin and glucagon were determined by standard radioimmunoassays, as previously described (53). Plasma p-aminohippuric acid concentrations were determined by a colorimetric method (4). Forearm blood flow (FBF) was determined at each blood sampling at baseline and at 1-h intervals after oral glucose ingestion (30, 90, 150, 210 and 270 min) by means of electrocapacitance plethysmography (34) after the procedure described by Jackson et al. (31).
Calculations. Systemic release and uptake of glucose were determined with steady-state equations under basal conditions (58) and subsequently after glucose ingestion with the non-steady-state equations of DeBodo et al. (16) and Finegood et al. (25), with a pool fraction of 0.65 and a volume of distribution of 200 ml/kg. The rate of appearance of the oral glucose in the systemic circulation was calculated from [6,6-2H2]glucose data with the equation of Chiasson et al. (13). Endogenous glucose release was calculated as the difference between the overall rate of glucose appearance and the rate of appearance of exogenous glucose. Hepatic glucose release was calculated as the difference between endogenous glucose release and renal glucose release (RGR).
Initial splanchnic glucose uptake of the ingested glucose was calculated as the difference between the amount of glucose ingested and the total appearance of the ingested glucose in the systemic circulation during the 4.5-h postprandial period, on the assumption that absorption of the ingested glucose had been completed as has been reported by Radziuk et al. (48). Renal plasma flow (RPF) was determined by p-aminohippuric acid clearance technique (4), and RBF was calculated as RPF/(1Statistical analysis. Unless stated otherwise, data are expressed as means ± SE. Paired two-tailed Student's t-tests were used to compare the mean baseline data with the mean data obtained after oral glucose ingestion. A P value <0.05 was considered statistically significant.
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RESULTS |
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Arterial glucose, insulin, and glucagon concentrations.
Postabsorptive arterial glucose, insulin, and glucagon
concentrations averaged 4.7 ± 0.1 mM, 56 ± 5 pM, and
69 ± 5 ng/l, respectively (Fig. 1).
After glucose ingestion, arterial glucose increased to peak values
(7.8 ± 0.3 mM) at 90 min and returned to postabsorptive levels
(4.7 ± 0.2 mM) by 240 min. Arterial insulin followed a similar
pattern, reaching a peak concentration (325 ± 45 pM) at 90 min
and returning to postabsorptive values (50 ± 8 pM) by 270 min.
Plasma glucagon decreased to a nadir (48 ± 4 ng/l) at 120 min and
returned to postabsorptive values (63 ± 6 ng/l) at 270 min.
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Overall systemic glucose appearance and disappearance.
Arterial glucose concentrations, [6-3H]glucose specific
activity and radioactivity, 6,6-dideuteroglucose enrichments, and
arterial-renal vein differences are given in Table
1.
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Systemic appearance of ingested glucose and renal and hepatic
glucose release.
Postprandial systemic glucose appearance consists of the appearance of
endogenous glucose released from liver and kidney and the appearance of
ingested glucose. The appearance of ingested glucose into the systemic
circulation was evident by 30 min and peaked at 90 min (15.6 ± 1.5 µmol · kg1 · min
1)
(Fig. 3). Over the 4.5-h postprandial
period, 53.0 ± 2.2 g of the 75 g ingested glucose
appeared in the systemic circulation. The ingested glucose accounted
for an average of 77.7 ± 2.4% of the circulating glucose during
this interval, a value similar to the ~75% found by Kelley et al.
(34) and Féry et al. (24) under
comparable experimental conditions. Although the rate of appearance of
the ingested glucose was still above zero at 270 min, this probably
represented ingested glucose initially incorporated into hepatic
glycogen (54) rather than ongoing intestinal absorption (33, 34). Therefore, with the assumption of complete
absorption of the ingested glucose, net splanchnic sequestration would
have amounted to 22.0 ± 2.2 g (29.3 ± 2.9% of the
ingested load).
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RGU and other substrate net balances.
RBF and renal FX both increased transiently, reaching peak values at
150 min and 210 min, respectively (P = 0.02 and
P = 0.05, respectively) (Fig.
4).
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Muscle glucose uptake and other substrate net balances.
Muscle glucose uptake averaged 1.91 ± 0.23 µmol · kg1 · min
1 before
glucose ingestion and accounted for 22.0 ± 3.7% of systemic glucose disposal. After glucose ingestion, muscle blood flow increased about 10% (P = 0.03) (Fig. 4). Muscle glucose FX also
increased, reaching a peak threefold greater than baseline (9.7 ± 1.9 vs. 3.1 ± 0.4%, P < 0.001) at 60 min before
returning to baseline at 210 min. During the initial 2 h after
glucose ingestion, muscle glucose uptake increased approximately
fivefold. Over the 4.5-h postprandial period, it averaged 5.72 ± 0.79 µmol · kg
1 · min
1
and accounted for 38.3 ± 5.0% of systemic glucose disposal
(25.9 ± 3.5 g) and 25.9 ± 3.4% of the disposal of the
ingested glucose (19.4 ± 2.6 g).
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DISCUSSION |
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Our study attempted to quantitate the fate of an ingested glucose load. Before the results of our experiments are discussed, certain limitations of the methods employed need to be taken into consideration to understand the precision with which such quantification can be made (45). First, splanchnic, muscle, and renal net balance measurements depend on detection of relatively small differences in arteriovenous concentrations and variability in blood flow calculations. The precision of these measurements depends on the inherent variability of the analytical procedures as well as on the reproducibility of the results of the people making these measurements. In our hands, the CVs for glucose concentrations and skeletal/renal blood flow measurements are ~1.5 and 5%, respectively. Second, there is analytic imprecision in specific activity measurements. In our hands, the CV for glucose specific activity measured by HPLC is ~0.5%.
Another source of variation is the use of the "hot hand" procedure to obtain arterialized blood as opposed to the use of arterial blood, because there may be venous contamination. In our studies, O2 saturation in samples exceeded 90%, thus indicating little or no contamination. With hepatic and renal venous sampling, one assumes that sampling from one kidney or one hepatic vein is representative of both kidneys and the whole liver, respectively. However, there can be considerable variation between simultaneously sampled hepatic veins (3), and there can be contamination of renal vein sampling. In our studies, monitoring of para-aminohippuric acid levels indicating >90% clearance suggests that there was little or no contamination. There are several other sources for imprecision such as using plasma values for substrates corrected to whole blood values based on hematocrit (45); these have been discussed in detail previously (45).
Regardless of the foregoing discussion of methods, our data provide clear-cut evidence for a hitherto unappreciated contribution of the kidney to postprandial glucose homeostasis and indicate that there is considerably greater postprandial suppression of hepatic glucose release than was previously thought.
In the present study, the kidney accounted for ~10% of the disposal of a 75-g ingested glucose load. To put this into perspective, the uptake of glucose by skeletal muscle, based on simultaneously measured forearm glucose uptake, was estimated to account for ~25% of the ingested glucose load. Although extrapolations to total body skeletal muscle from regional measurements should be viewed with caution, the value that we obtained is similar to the average (27 ± 2%) found in eight previous studies whose data permitted this calculation (5, 26, 33-35, 37, 38, 44).
Renal uptake of glucose has been previously shown to increase during hyperglycemia (6, 19) and to be stimulated by insulin (9, 40). In the present study, increases in renal glucose fractional extraction and renal blood flow both contributed to the increased postprandial renal glucose uptake. These changes may have resulted, at least in part, from postprandial hyperinsulinemia, because insulin has been shown to increase renal blood flow and glucose fractional extraction in normal postabsorptive humans (7, 40). Had these changes in blood flow and fractional extraction not occurred, the observed renal glucose uptake would have been reduced by ~50%. Thus the mass action effects of hyperglycemia and changes in blood flow and fractional extraction contributed similarly to the postprandial renal glucose uptake.
The magnitude of the postprandial renal glucose uptake may seem surprising beause the kidney, in contrast to liver and muscle, does not normally store appreciable glycogen (2). However, all of the glucose taken up by the kidney could be accounted for by its being released as lactate and its being oxidized, as a substitute for FFA.
Lipid is normally the major oxidative fuel of the kidney (57). In the present study, postprandial renal FFA net uptake was reduced by 65% (i.e., by 48 µmol/min). Substitution of glucose for these FFA to provide equivalent ATP via oxidation would have required 163 µmol/min, or 7.9 g, over the 4.5-h postprandial period. This would account for 79% of the glucose taken up by the kidney postprandially (10.0 g). These considerations provide further, albeit indirect, evidence in favor of a renal glucose-fatty acid cycle, as has been recently postulated (41) and analogous to the situation for skeletal muscle postulated by Taylor et al. (54). These investigators observed no net glycogen accumulation in skeletal muscle for nearly 2 h after ingestion of a meal containing 290 g of carbohydrate. Because muscle glucose uptake would have increased substantially during this period, as demonstrated in the present and other studies (5, 26, 33-35, 37, 38, 44, 47), it was postulated that the glucose taken up was oxidized in place of FFA.
Not only did the kidney play a role in the disposal of the ingested glucose, it also influenced postprandial glucose homeostasis by increasing its release of glucose. Thus, in contrast to liver, whose postprandial release of glucose was markedly decreased, there was a more than twofold increase in renal glucose release, so that it on average actually exceeded that of the liver during the 4.5-h postprandial period. This finding was surprising, because hyperglycemia and hyperinsulinemia would have been expected to suppress renal glucose release (6, 19, 40).
Several factors could explain the reciprocal changes in hepatic and renal glucose release. First of all, the liver is exposed to higher (i.e., portal) insulin concentrations than is the kidney. Second, suppression of hepatic glycogenolysis, which we postulate to have largely accounted for the suppression of hepatic glucose release, is known to be more sensitive to insulin than is hepatic gluconeogenesis (12). Third, suppression of glucagon secretion may have played a role, because glucagon supports hepatic glucose release (11) but has no effect on renal glucose release (50). Fourth, glucose ingestion increases sympathetic nervous system activity (55), which may have preferentially augmented renal glucose release. In support of this view is the observation that infusion of epinephrine causes a sustained increase in renal glucose release while increasing hepatic glucose release transiently and to a lesser extent (49).
From a teleological point of view, this increased postprandial release of glucose by the kidney would permit greater suppression of hepatic glycogenolysis so that there could be more efficient glycogen replenishment. Because the kidney increases its release of glucose, calculation of postprandial hepatic glucose release as the difference between the overall appearance of glucose in the systemic circulation and the appearance of the ingested glucose substantially underestimates the suppression of hepatic glucose release. In nine previous studies in which hepatic glucose release was calculated in this manner, the mean value for its postprandial suppression was 42 ± 4% (5, 22, 26, 33-35, 37, 38, 44). In the present studies, calculation of hepatic glucose release as the difference between overall systemic glucose release and the sum of ingested and renal glucose release indicated a suppression of 82 ± 6%. To put this into perspective, 82% suppression of hepatic glucose release would amount to ~30 g less glucose entering the circulation during the 4.5-h postprandial period. A suppression of 42% would have led to only ~10 g less glucose entering the circulation.
It is worth noting that the initial net splanchnic sequestration (presumably representing hepatic glucose uptake) found in the present study (~22 g) accounted for 30 ± 3% of the ingested glucose load. This is remarkably similar to the mean of 33 ± 4% found in the nine previous reports (5, 22, 26, 33-35, 37, 38, 44, 60). Although this in itself is substantial, it underestimates total postprandial hepatic glucose uptake, since the liver also extracts glucose from the systemic circulation (23). Nevertheless, taking into consideration only the initial net hepatic uptake of ingested glucose (22 g) and the glucose conserved via suppression of hepatic glucose release (30 g), one can assign to the liver management of ~50 g of postprandial "glucose traffic." Muscle, the next most important tissue for postprandial glucose disposal (see below), was responsible for uptake of 26 g (~20 g ingested glucose + 6 g endogenous glucose). These considerations suggest that the liver is the more important organ for postprandial glucose homeostasis and that hepatic abnormalities would be expected to have a substantial impact on postprandial glucose metabolism, as has been demonstrated in people with impaired glucose tolerance and those with type 2 diabetes (18, 27).
Quantification of postprandial renal glucose uptake and release in the present study not only refines our appreciation of the contribution of the liver but also provides a more complete view of postprandial glucose disposal than has been previously available. According to the results of the present and previous studies (5, 22, 26, 33-35, 37, 38, 44, 60), ~25-35% of an ingested 100-g carbohydrate load would be initially extracted by the liver. Of the remaining 65-75% of the ingested glucose that enters the systemic circulation, ~40% would be taken up by skeletal muscle (5, 26, 33-35, 37, 38, 44) and ~10% would be taken up by the kidney and liver. These three tissues could thus account for ~75-85% of the disposal of the ingested glucose. Brain glucose uptake in postabsorptive volunteers has been reported to be ~80 mg/min (17, 20, 29). On the assumption that this rate would remain constant postprandially and that ingested glucose represented 75% of circulating glucose, as was found in the present and previous studies (24, 34), it can be calculated that brain would take up ~15-20% of the ingested glucose. Therefore, uptake of glucose by liver, muscle, brain, and kidney could account for at least 90% of the disposal of an ingested glucose load.
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ACKNOWLEDGEMENTS |
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We thank Mary Little for excellent editorial assistance and the nursing and laboratory staff of the General Clinical Research Center (GCRC) for superb help.
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FOOTNOTES |
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The present work was supported in part by Division of Research Resources-GCRC Grant 5M01 RR-00044 and the National Institute of Diabetes and Digestive and Kidney Diseases Grant DK-20411.
Address for reprint requests and other correspondence: J. E. Gerich, Univ. of Rochester School of Medicine, 601 Elmwood Ave., Box MED/CRC, Rochester, NY 14642 (E-mail: Johngerich{at}compuserve.com).
The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
10.1152/ajpendo.00032.2001
Received 25 January 2001; accepted in final form 3 October 2001.
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REFERENCES |
---|
![]() ![]() ![]() ![]() ![]() ![]() ![]() |
---|
1.
Andres, R,
Cader G,
and
Zierler K.
The quantitatively minor role of carbohydrate in oxidative metabolism by skeletal muscle in intact man in the basal state. Measurements of oxygen and glucose uptake and carbon dioxide and lactate production in the forearm.
J Clin Invest
35:
671-682,
1956[ISI].
2.
Biava, C,
Grossman A,
and
West M.
Ultrastructural observations on renal glycogen in normal and pathologic human kidneys.
Lab Invest
15:
330-356,
1966[ISI][Medline].
3.
Bradley, S,
Ingelfinger F,
Bradley G,
and
Curry J.
The estimation of hepatic blood flow in man.
J Clin Invest
24:
890-897,
1945[ISI].
4.
Brun, C.
A rapid method for the determination of para-aminohippuric acid in kidney function tests.
J Lab Clin Med
37:
955-958,
1951[ISI].
5.
Butler, P,
Kryshak E,
and
Rizza R.
Mechanism of growth hormone-induced postprandial carbohydrate intolerance in humans.
Am J Physiol Endocrinol Metab
260:
E513-E520,
1991
6.
Cersosimo, E,
Ajmal M,
Naukam R,
Molina P,
and
Abumrad N.
Role of the kidney in plasma glucose regulation during hyperglycemia.
Am J Physiol Endocrinol Metab
272:
E756-E761,
1997
7.
Cersosimo, E,
Garlick P,
and
Ferretti J.
Insulin regulation of renal glucose metabolism in humans.
Am J Physiol Endocrinol Metab
276:
E78-E84,
1999
8.
Cersosimo, E,
Garlick P,
and
Ferretti J.
Renal glucose production during insulin-induced hypoglycemia in humans.
Diabetes
48:
261-266,
1999
9.
Cersosimo, E,
Judd R,
and
Miles J.
Insulin regulation of renal glucose metabolism in conscious dogs.
J Clin Invest
93:
2584-2589,
1994[ISI][Medline].
10.
Cersosimo, E,
Molina A,
and
Abumrad N.
Renal glucose production during insulin-induced hypoglycemia.
Diabetes
46:
643-646,
1997[Abstract].
11.
Chiasson, J,
and
Cherrington A.
Glucagon and liver glucose output in vivo.
In: Glucagon I, edited by Lefebvre P. New York: Springer-Verlag, 1983, p. 361-382.
12.
Chiasson, J,
Liljenquist J,
Finger F,
and
Lacy W.
Differential sensitivity of glycogenolysis and gluconeogenesis to insulin infusions in dogs.
Diabetes
25:
283-291,
1976[Abstract].
13.
Chiasson, J,
Liljenquist J,
Lacy W,
Jennings A,
and
Cherrington A.
Gluconeogenesis: methodological approaches in vivo.
Fed Proc
36:
229-235,
1977[ISI][Medline].
14.
Consoli, A,
Nurjhan N,
Reilly J,
Bier D,
and
Gerich J.
Mechanism of increased gluconeogenesis in noninsulin dependent diabetes mellitus: role of alterations in systemic, hepatic and muscle lactate and alanine metabolism.
J Clin Invest
86:
2038-2045,
1990[ISI][Medline].
15.
Cooper, K,
Edholm O,
and
Moltram R.
The blood flow in skin and muscle of the human forearm.
J Physiol (Lond)
128:
258-267,
1955[ISI].
16.
DeBodo, R,
Steele R,
Dunn A,
and
Bishop J.
On the hormonal regulation of carbohydrate metabolism: studies with 14C glucose.
Recent Prog Horm Res
19:
445-448,
1963[ISI].
17.
DellaPorta, P,
Maiolo A,
Negri V,
and
Rossella E.
Cerebral blood flow and metabolism in therapeutic insulin coma.
Metabolism
13:
131-140,
1964[ISI].
18.
Dinneen, S,
Gerich J,
and
Rizza R.
Carbohydrate metabolism in noninsulin-dependent diabetes mellitus.
N Engl J Med
327:
707-713,
1992[ISI][Medline].
19.
Dzurik, R,
and
Chorvathova V.
Relation between the uptake of glucose and fatty acids by the rat kidney in vivo.
Physiol Bohemoslov
21:
361-365,
1972[ISI][Medline].
20.
Eisenberg, S,
and
Seltzer H.
The cerebral metabolic effect of acutely induced hypoglycemia in normal subjects.
Metabolism
11:
1162-1168,
1962[ISI].
21.
Ekberg, K,
Landau B,
Wajngot A,
Chandramouli V,
Efendic S,
Brunengraber H,
and
Wahren J.
Contributions by kidney and liver to glucose production in the postabsorptive state and after 60 h of fasting.
Diabetes
48:
292-298,
1999
22.
Ferrannini, E,
Bjorkman O,
Reichard G,
Pilo A,
Olsson M,
Wahren J,
and
DeFronzo R.
The disposal of an oral glucose load in healthy subjects: a quantitative study.
Diabetes
34:
580-588,
1985[Abstract].
23.
Ferrannini, E,
Wahren J,
Felig P,
and
DeFronzo R.
The role of fractional glucose extraction in the regulation of splanchnic glucose metabolism in normal and diabetic man.
Metabolism
29:
28-35,
1980[ISI][Medline].
24.
Féry, F,
Plat L,
and
Balasse E.
Mechanisms of whole-body glycogen deposition after oral glucose in normal subjects. Influence of the nutritional status.
J Clin Endocrinol Metab
83:
2810-2816,
1998
25.
Finegood, D,
Bergman R,
and
Vranic M.
Estimation of endogenous glucose production during hyperinsulinemic-euglycemic glucose clamps. Comparison of unlabeled and labeled exogenous glucose infusates.
Diabetes
36:
914-924,
1987[Abstract].
26.
Firth, R,
Bell P,
Marsh H,
Hansen I,
and
Rizza R.
Postprandial hyperglycemia in patients with noninsulin-dependent diabetes mellitus. Role of hepatic and extrahepatic tissues.
J Clin Invest
77:
1525-1532,
1986[ISI][Medline].
27.
Gerich, J.
Metabolic abnormalities in impaired glucose tolerance.
Metabolism
46:
40-43,
1997[ISI][Medline].
28.
Gerich, J.
Measurements of renal glucose release.
Diabetes
50:
905,
2001
29.
Gottstein, U,
Muller W,
Berghoff W,
Gartner H,
and
Held K.
Zur utilisation von nicht-veresterten fettsauern and ketonkorpen in gehirn des Menschen.
Klin Wschr
49:
406-411,
1971[Medline].
30.
Heymsfield, S,
McManus C,
Stevens V,
and
Smith J.
Muscle mass: reliable indicator of protein-energy malnutrition severity and outcome.
Am J Clin Nutr
35:
1192-1199,
1982[ISI][Medline].
31.
Jackson, R,
Blix P,
Matthews J,
Morgan L,
Rubenstein A,
and
Nabarro J.
Comparison of peripheral glucose uptake after oral glucose loading and a mixed meal.
Metabolism
32:
706-710,
1983[ISI][Medline].
32.
Jackson, R,
Peters N,
Advani V,
Perry G,
Rogers J,
Brough W,
and
Pilkington T.
Forearm glucose uptake during the oral glucose tolerance test in normal subjects.
Diabetes
22:
442-458,
1973[ISI][Medline].
33.
Jackson, R,
Roshania R,
Hawa M,
Sim B,
and
DiSilvio L.
Impact of glucose ingestion on hepatic and peripheral glucose metabolism in man: an analysis based on simultaneous use of the forearm and double isotope techniques.
J Clin Endocrinol Metab
63:
541-549,
1986[Abstract].
34.
Kelley, D,
Mitrakou A,
Marsh H,
Schwenk F,
Benn J,
Sonnenberg G,
Archangeli M,
Aoki T,
Sorensen J,
Berger M,
Sonksen P,
and
Gerich J.
Skeletal muscle glycolysis, oxidation, and storage of an oral glucose load.
J Clin Invest
81:
1563-1571,
1988[ISI][Medline].
35.
Kelley, D,
Mokan M,
and
Veneman T.
Impaired postprandial glucose utilization in non-insulin-dependent diabetes mellitus.
Metabolism
43:
1549-1557,
1994[ISI][Medline].
36.
Lowry, O,
and
Passonneau J.
Typical fluorimetric procedures for metabolic assays.
In: A Flexible System for Enzymatic Analysis, edited by Lowry O,
and Passonneau J. New York: Academic, 1972, p. 194-199.
37.
McMahon, M,
Marsh H,
and
Rizza R.
Comparison of the pattern of postprandial carbohydrate metabolism after ingestion of a glucose drink or a mixed meal.
J Clin Endocrinol Metab
68:
647-653,
1989[Abstract].
38.
McMahon, M,
Marsh H,
and
Rizza R.
Effects of basal insulin supplementation on disposition of a mixed meal in obese patients with NIDDM.
Diabetes
38:
291-303,
1989[Abstract].
39.
Meyer, C,
Dostou J,
and
Gerich J.
Role of the human kidney in glucose counterregulation.
Diabetes
48:
943-948,
1999[Abstract].
40.
Meyer, C,
Dostou J,
Nadkarni V,
and
Gerich J.
Effects of physiological hyperinsulinemia on systemic, renal, and hepatic substrate metabolism.
Am J Physiol Renal Physiol
275:
F915-F921,
1998
41.
Meyer, C,
Nadkarni V,
Stumvoll M,
and
Gerich J.
Human kidney free fatty acid and glucose uptake: evidence for a renal glucose-fatty acid cycle.
Am J Physiol Endocrinol Metab
273:
E650-E654,
1997
42.
Meyer, C,
Stumvoll M,
Nadkarni V,
Dostou J,
Mitrakou A,
and
Gerich J.
Abnormal renal and hepatic glucose metabolism in type 2 diabetes mellitus.
J Clin Invest
102:
619-624,
1998
43.
Miles, J,
Glassock R,
Aikens J,
Gerich J,
and
Haymond M.
A microfluorimetric method for the determination of free fatty acids on plasma.
J Lipid Res
24:
96-99,
1983[Abstract].
44.
Mitrakou, A,
Kelley D,
Mokan M,
Veneman T,
Pangburn T,
Reilly J,
and
Gerich J.
Role of reduced suppression of glucose production and diminished early insulin release in impaired glucose tolerance.
N Engl J Med
326:
22-29,
1992[Abstract].
45.
Moller, N,
Rizza R,
Ford G,
and
Nair K.
Assessment of postabsorptive renal glucose metabolism in humans with multiple glucose tracers.
Diabetes
50:
747-751,
2001
46.
Nurjhan, N,
Kennedy F,
Consoli A,
Martin C,
Miles J,
and
Gerich J.
Quantification of the glycolytic origin of plasma glycerol: implications for the use of the rate of appearance of plasma glycerol as an index of lipolysis in vivo.
Metabolism
37:
386-389,
1988[ISI][Medline].
47.
Radziuk, J,
and
Inculet R.
The effects of ingested and intravenous glucose on forearm uptake of glucose and glucogenic substrate in normal man.
Diabetes
32:
977-981,
1983[Abstract].
48.
Radziuk, J,
McDonald T,
Rubenstein D,
and
Dupre J.
Initial splanchnic extraction of ingested glucose in normal man.
Metabolism
27:
657-669,
1978[ISI][Medline].
49.
Stumvoll, M,
Chintalapudi U,
Perriello G,
Welle S,
Gutierrez O,
and
Gerich J.
Uptake and release of glucose by the human kidney: postabsorptive rates and responses to epinephrine.
J Clin Invest
96:
2528-2533,
1995[ISI][Medline].
50.
Stumvoll, M,
Meyer C,
Kreider M,
Perriello G,
and
Gerich J.
Effects of glucagon on renal and hepatic glutamine gluconeogenesis in normal postabsorptive humans.
Metabolism
47:
1227-1232,
1998[ISI][Medline].
51.
Stumvoll, M,
Meyer C,
Mitrakou A,
Nadkarni V,
and
Gerich J.
Renal glucose production and utilization: new aspects in humans.
Diabetologia
40:
749-757,
1997[ISI][Medline].
52.
Stumvoll, M,
Meyer C,
Perriello G,
Kreider M,
Welle S,
and
Gerich J.
Human kidney and liver gluconeogenesis: evidence for organ substrate selectivity.
Am J Physiol Endocrinol Metab
274:
E817-E826,
1998
53.
Stumvoll, M,
Perriello G,
Nurjhan N,
Bucci A,
Welle S,
Jansson P-A,
Dailey G,
Bier D,
Jenssen T,
and
Gerich J.
Glutamine and alanine metabolism in NIDDM.
Diabetes
45:
863-868,
1996[Abstract].
54.
Taylor, R,
Price T,
Katz L,
Shulman R,
and
Shulman G.
Direct measurement of change in muscle glycogen concentration after a mixed meal in normal subjects.
Am J Physiol Endocrinol Metab
265:
E224-E229,
1993
55.
Welle, S,
Lilavivathana U,
and
Campbell R.
Increased plasma norepinephrine concentrations and metabolic rates following glucose ingestion in man.
Metabolism
29:
806-809,
1980[ISI][Medline].
56.
Wieland, O.
Glycerol UV method.
In: Methods of Enzymatic Analysis, edited by Bergmeyer U. New York: Academic, 1974, vol. 3, p. 1404-1414.
57.
Wirthensohn, G,
and
Guder W.
Renal substrate metabolism.
Physiol Rev
66:
469-497,
1986
58.
Wolfe, R.
Radioactive and Stable Isotope Tracers in Biomedicine: Principles and Practice of Kinetic Analysis. New York: Wiley-Liss, 1992.
59.
World Health Organization Expert Committee.
Diabetes mellitus: a second report. Geneva, Switzerland: WHO, 1980, p. 1-80. (Tech. Rep. Ser. 646)
60.
Yki-Järvinen, H,
Helve E,
Sane T,
Nurjhan N,
and
Taskinen MR.
Insulin inhibition of overnight glucose production and gluconeogenesis from lactate in NIDDM.
Am J Physiol Endocrinol Metab
256:
E732-E739,
1989