This Article Abstract Full Text (PDF) All Versions of this Article: 111/16/2066    most recent 01.CIR.0000162466.06150.D4v1 Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Request Permissions Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Wang, P. Articles by Chatham, J. C. Search for Related Content PubMed PubMed Citation Articles by Wang, P. Articles by Chatham, J. C. Related Collections Contractile function Biochemistry and metabolism Animal models of human disease Energy metabolism

(Circulation. 2005;111:2066-2072.)
© 2005 American Heart Association, Inc.

Heart Failure

Impact of High Glucose/High Insulin and Dichloroacetate Treatment on Carbohydrate Oxidation and Functional Recovery After Low-Flow Ischemia and Reperfusion in the Isolated Perfused Rat Heart

Peipei Wang, MD, PhD; Steven G. Lloyd, MD, PhD; John C. Chatham, DPhil

From the Division of Cardiovascular Disease, Department of Medicine (P.W., S.G.L., J.C.C.) and Department of Physiology and Biophysics, Department of Cell Biology (J.C.C.), The Comprehensive Cancer Center, The Clinical Nutrition Research Center (J.C.C.), University of Alabama, Birmingham.

Correspondence to John C. Chatham, University of Alabama at Birmingham, McCallum Bldg, Room 684, 1530 3rd Ave S, Birmingham, AL 35294-0005. E-mail jchatham{at}uab.edu

Received September 21, 2004; revision received November 23, 2004; accepted December 21, 2004.

	Abstract

Top Abstract Introduction Methods Results Discussion References

 
Background— It is believed that increasing cardiac glucose metabolism in the setting of ischemia and reperfusion is protective because of the resulting decrease in fatty acid oxidation, which improves cardiac efficiency and increases glucose oxidation relative to glycolysis; however, these conclusions are based primarily on studies in which glucose is the only carbohydrate provided. The goal of this study was to examine the effect of stimulating myocardial carbohydrate use either by increasing glucose and insulin levels or by using dichloroacetate on the response to ischemia and reperfusion in hearts perfused with physiological concentrations of lactate and pyruvate plus glucose and fatty acids.

Methods and Results— Metabolic fluxes were determined in hearts from male Sprague-Dawley rats perfused with ¹³C-labeled substrates using ¹³C/¹H-NMR isotopomer analysis after 30 minutes of low-flow ischemia (0.3 mL/min) and 60 minutes of reperfusion. Measurements were made under control conditions: 5 mmol/L glucose, 1 mmol/L lactate, 0.1 mmol/L pyruvate, 0.3 mmol/L palmitate, and 50 µU/mL insulin plus dichloroacetate 5 mmol/L or glucose and insulin increased to 30 mmol/L and 1000 µU/mL, respectively. Dichloroacetate increased carbohydrate oxidation and the ratio of glucose oxidation to glycolysis but did not improve functional recovery or cardiac efficiency; however, elevated glucose and insulin levels improved functional recovery and cardiac efficiency but did not increase carbohydrate oxidation or the ratio of glucose oxidation to glycolysis.

Conclusions— These data support the notion that increasing myocardial glucose use is beneficial in the setting of ischemia and reperfusion; however, the protective effect appears not to be mediated by shifting the balance between carbohydrate and fatty acid oxidation.

Key Words: fatty acids • glucose • ischemia • metabolism • reperfusion

	Introduction

Top Abstract Introduction Methods Results Discussion References

 
Modulation of cardiac metabolism as a therapeutic approach for treating ischemic heart disease has been the subject of investigation for >40 years and generally is predicated on increasing cardiac glucose use while decreasing fatty acid use. In this context, glucose-insulin-potassium (GIK) therapy is one of the most widely investigated approaches used in a clinical setting; it was first reported in 1962,¹ with results from new trials continuing to be published.^2,3 Although in general GIK therapy is found to improve outcome after acute myocardial infarction,^4,5 this is not a uniform observation.³ The discrepancies could be due in part to the relatively large fluid volumes administered with this protocol, which may adversely affect some patient groups more than others.² An alternative approach that avoids these complications is direct pharmacological modulation of cardiac fatty acid and carbohydrate metabolism.⁶ This has been the focus of many studies, leading to the development of putative fatty acid oxidation inhibitors such as trimetazidine and ranolazine for the treatment of ischemic disease.^7,8 Their protective effects are typically attributed to increased glucose oxidation and decreased fatty acid oxidation.^6–8

Despite the continuing interest in GIK therapy and the apparent efficacy of trimetazidine and ranolazine, there is no consensus about the mechanisms underlying their beneficial effects. One of the most frequently proposed mechanisms is that decreasing fatty acid oxidation and increasing glucose oxidation improve efficiency by decreasing the amount of oxygen required for ATP synthesis.⁶ Theoretically, there is an 12% decrease in oxygen required for ATP synthesis in shifting from 100% palmitate oxidation to 100% glucose oxidation⁹; however, such extreme metabolic shifts are unlikely to occur under physiological conditions. Another explanation for the beneficial consequences of increasing glucose oxidation is that it improves the "coupling" between glucose oxidation and glycolysis, decreasing proton production and thus reducing intracellular acidosis.^10,11 It is noteworthy that both of these mechanisms are based on the premise that glucose and palmitate are the primary substrates for cardiac energy production despite the fact that lactate is more readily oxidized than glucose in the heart.^12–14 We found that when lactate and pyruvate, as well as glucose and palmitate, are available for oxidation, decreasing fatty acid oxidation from 60% to 5% of total energy production did not alter the efficiency of ATP production.¹²

Given the broad acceptance of the notion that increasing glucose use is beneficial, relatively few studies have examined the impact of these interventions on the regulation of carbohydrate and fatty acid metabolism after ischemia and reperfusion, particularly in the presence of substrates other than glucose and fatty acids. Therefore, the aim of this study was to compare the effect of stimulating cardiac glucose use by increasing glucose and insulin concentrations with direct activation of carbohydrate oxidation using dichloroacetate (DCA) on the metabolic and functional responses to ischemia and reperfusion in hearts perfused with physiological concentrations of lactate and pyruvate, as well as glucose and palmitate. The results demonstrated that increasing glucose and insulin improved functional recovery compared with DCA treatment, whereas DCA had a greater impact on increasing carbohydrate oxidation. We also found that the protection associated with increased glucose and insulin levels was not related to changes in cardiac efficiency or to the coupling of glucose oxidation to glycolysis.

	Methods

Top Abstract Introduction Methods Results Discussion References

 
Animals
Animal experiments were approved by the Institutional Animal Care and Use Committee at the University of Alabama at Birmingham and followed the Guidelines for the Care and Use of Laboratory Animals (National Academy of Sciences, 1996). Male Sprague-Dawley rats (Charles Rivers Laboratories) weighing 300 to 325 g were used throughout.

Isolated Heart Preparation
Hearts were isolated and perfused as previously described¹² with a Krebs-Henseleit buffer containing 3% BSA (essentially fatty acid free, Intergen Corp), 0.32 mmol/L sodium palmitate, 1.0 mmol/L sodium lactate, 0.1 mmol/L sodium pyruvate, 5 mmol/L glucose, and 50 µU/mL insulin unless stated otherwise. Cardiac function was monitored via a fluid-filled balloon placed in the left ventricle and connected to a pressure transducer. End-diastolic pressure was set to 5 mm Hg by adjusting balloon volume. Hearts were perfused under constant perfusion pressure of 75 mm Hg and paced at 320 bpm throughout the experiments.

Experimental Protocol
Hearts were assigned to 1 of 3 groups: (1) control, 5 mmol/L glucose and 50 µU/mL insulin; (2) high glucose and high insulin (HG/HI), 30 mmol/L glucose and 1000 µU/mL insulin; or (3) DCA (5 mmol/L), 5 mmol/L glucose and 50 µU/mL insulin. Hearts from all groups were equilibrated for 30 minutes under normal-flow perfusion and subjected to low-flow ischemia (LFI; 0.3 mL/min) for 30 minutes followed by 60 minutes of reperfusion, during which time flow was restored to achieve a perfusion pressure of 75 mm Hg as described previously.¹⁵ Hearts from the control and HG/HI groups were also perfused under normal-flow conditions for 60 minutes. In some experiments, at the onset of LFI, unlabeled lactate was replaced with [3-¹³C]lactate to permit the rates of exogenous lactate uptake and glycolytic lactate efflux to be determined as previously described.¹³ During the last 30 minutes of each protocol, hearts were perfused with [U-¹³C]palmitate, [2-¹³C]pyruvate, [3-¹³C]lactate, and unlabeled glucose at the same concentrations used during preceding perfusion period.

Coronary effluent samples were collected immediately before ischemia, every 5 minutes during ischemia, every 1 minute during the first 5 minutes of reperfusion, and at the end of reperfusion in the LFI protocol and at the end of the experiments in the normal-flow experiments. Oxygen consumption was determined as previously described.¹³ At the end of each protocol, hearts were freeze-clamped.

As described previously,¹² tissue and coronary effluent samples were acid extracted, freeze-dried, and redissolved in a potassium phosphate buffer (pH 7.5, 50 mmol/L) with ²H₂O solvent (99.9%; Cambridge Isotope Laboratories) before ¹³C- and ¹H-nuclear magnetic resonance (NMR) analysis.

¹³C-NMR Glutamate Isotopomer Analysis and Determination of Substrate Oxidation Rates
¹³C-NMR spectra of heart extracts were collected and ¹³C-glutamate isotopomer analysis was performed^12,13 to determine the fraction of total acetyl-CoA entering the tricarboxylic acid cycle originating from unlabeled, [1,2-¹³C]-, [2-¹³C]-, and [1-¹³C]acetyl-CoA resulting from oxidation of unlabeled glucose, [U-¹³C]-palmitate, [3-¹³C]-lactate, and [2-¹³C]-pyruvate, respectively. Combined with measurements of tissue oxygen consumption, the absolute oxidation rates of each substrate were determined.¹³ Theoretical oxidative ATP production was calculated from the oxidation rates of each substrate multiplied by the oxidative component of the calculated ATP yield for each substrate as described by Opie⁹ using the corrections for loss of energy during oxidative phosphorylation as reported by Hinkle et al.¹⁶

Determination of Lactate Efflux and Uptake Rates
¹H-NMR spectroscopy was used to determine the fraction of unlabeled lactate formed by metabolism of exogenous glucose or glycogen and [3-¹³C] lactate added to the perfusate. These data, multiplied by the total lactate concentration in the effluent determined by enzymatic colorimetric methods and the coronary flow rates, were used to determine the rates of exogenous [3-¹³C] lactate uptake and unlabeled glycolytic lactate efflux.

Statistical Analysis
All data are presented as mean±SEM. One-way ANOVA and repeated-measures ANOVA were used when appropriate, combined with Scheffé post hoc test (Statview, Abacus Concepts, Inc). A value of P<0.05 was considered significant.

	Results

Top Abstract Introduction Methods Results Discussion References

 
Baseline cardiac function was not significantly different between the 3 groups (Figure 1A). The onset of LFI led to a rapid cessation of contractile function and a gradual increase in end-diastolic pressure characteristic of the development of contracture (Figure 1B); this increase in contracture was completely abolished in the HG/HI group. The time to maximum contracture was more rapid in the DCA group than the control group (15.0±1.6 versus 22.3±1.4 minutes, respectively; P<0.05). During reperfusion, contractile function recovered more rapidly in the HG/HI group than in either the control or DCA group. For example, the rate of recovery of the rate-pressure product (RPP; maximum RPP in reperfusion divided by time to maximum RPP) in the HG/HI group was 2932±656 mm Hg · min^–1 · min^–1 compared with 1206±249 and 926±235 mm Hg · min^–1 · min^–1 in the control and DCA groups, respectively (Figure 1C). In the HG/HI group, RPP was 87% of baseline at the end of reperfusion, which was significantly higher than in the control group (74%; P<0.05). An important contributing factor to the improved function in the HG/HI group was a significantly lower end-diastolic pressure (Figure 1C).

View larger version (33K): [in this window] [in a new window]   Figure 1. Cardiac function during baseline (A), LFI (B), and reperfusion conditions (C) in control (Cont; open symbols and bars), DCA (gray symbols and bars), and HG/HI (solid symbols and bars) groups. EDP indicates end-diastolic pressure. *P<0.05 vs control.

As summarized in Figure 2A, DCA significantly increased total carbohydrate oxidation rate by >2-fold with an 5-fold decrease in palmitate oxidation. Surprisingly, there were no significant differences in carbohydrate and fatty acid oxidation rates between the control and HG/HI groups. As shown in Figure 2B, lactate represented the predominant source of total carbohydrate oxidation. Interestingly, although DCA increased total carbohydrate oxidation, it did not change the relative contributions of lactate, pyruvate, and glucose. Although total carbohydrate oxidation was not increased in the HG/HI group, the contribution of glucose to total carbohydrate oxidation was significantly increased and the contribution from lactate was decreased compared with the control group.

View larger version (27K): [in this window] [in a new window]   Figure 2. A, Substrate oxidation rates in control (open bars), DCA (gray bars), and HG/HI (solid bars) groups at end of reperfusion. B, Percent contribution of lactate, pyruvate, and glucose to total carbohydrate oxidation (CHO). *P<0.05 vs control; P<0.05 vs HG/HI.

During LFI, glycolytic lactate efflux was increased 2-fold in the HG/HI group compared with the other 2 groups, whereas there was no significant difference in lactate uptake between groups (Figure 3A). During reperfusion, the rate of glycolytic lactate efflux remained higher in the HG/HI group; the rate of exogenous lactate uptake was also increased in the HG/HI group compared with the control group (Figure 3B).

View larger version (19K): [in this window] [in a new window]   Figure 3. A, Lactate efflux and uptake during LFI. B, Lactate efflux and uptake at end of reperfusion in control (Cont; open bars), DCA (gray bars), and HG/HI (solid bars) groups. *P<0.05 vs control; P<0.05 vs HG/HI.

From the lactate efflux rates and the substrate oxidation rates, we determined oxidative, glycolytic, and total ATP synthesis rates during reperfusion (Table 1). There were no differences in total ATP synthesis rates between the groups; however, in the HG/HI group, there was a significant decrease in oxidative ATP production and an increase in the contribution of glycolytic ATP production to total ATP production. The rates of oxidative ATP synthesis from the individual substrates are shown in Table 2. These data reinforce the results in Figure 2, demonstrating that DCA increases the contributions of lactate, pyruvate, and glucose to oxidative ATP synthesis relative to both the control and HG/HI groups. In the HG/HI group, the contribution to oxidative ATP synthesis from pyruvate is decreased by >50% and that from palmitate is decreased by 30%.

View this table: [in this window] [in a new window]   TABLE 1. Total, Oxidative, and Glycolytic ATP Production Rates at the End of Reperfusion

View this table: [in this window] [in a new window]   TABLE 2. Rates of Oxidative ATP Production From Individual Substrates During Reperfusion

To evaluate the impact of DCA and HG/HI treatment on the coupling of glucose oxidation to glycolysis, we calculated the ratio of the rate of glycolytically derived pyruvate oxidation to the total rate of glycolysis (defined as the sum of the rates of glycolytically derived pyruvate oxidation plus glycolytically derived lactate efflux) (Table 3). DCA increased this ratio, ie, improved the coupling of glucose oxidation to glycolysis, compared with the HG/HI group, consistent with their effects on both lactate efflux (Figure 3) and glucose oxidation (Figure 2). To estimate the efficiency of converting oxygen consumption to contractile work, we calculated the ratio of RPP to oxygen consumption (MVO₂). This ratio was significantly higher in the HG/HI group compared with the control and DCA groups, demonstrating that the HG/HI group consumed less oxygen to perform the same level of contractile work. Thus, the HG/HI group showed improved recovery of function and cardiac efficiency compared with the DCA group, despite a decrease in the coupling of glucose oxidation to glycolysis and increased contribution of fatty acids to energy production.

View this table: [in this window] [in a new window]   TABLE 3. Ratio of Glucose Oxidation to Glycolysis, O2max, and Cardiac Efficiency at the End of Reperfusion

The lack of effect of HG/HI on carbohydrate oxidation compared with control conditions during reperfusion was surprising. Therefore, we determined the rates of substrate oxidation and lactate uptake and efflux in these 2 groups during normal-flow conditions (Figure 4). In contrast to our findings during reperfusion, in normal flow, there was a significant increase in total carbohydrate oxidation in the HG/HI group compared with the control group. Interestingly, this increase was a result of increased lactate and glucose oxidation. Furthermore, whereas glycolytic lactate efflux was increased during reperfusion in the HG/HI group, there was no difference during normal perfusion. Nevertheless, lactate uptake was increased with HG/HI in accordance with the increase in lactate oxidation; this is consistent with previous reports of insulin stimulating lactate uptake.¹⁷ A larger increase in carbohydrate oxidation might have been anticipated with 30 mmol/L glucose and 1000 µU/mL insulin; however, these data are consistent with our earlier report in which we found that the greatest increase in carbohydrate oxidation was between 0 and 100 µU/mL insulin,¹² whereas increasing insulin from 100 to 1000 µU/mL increased total carbohydrate oxidation by only 20%.

View larger version (17K): [in this window] [in a new window]   Figure 4. Substrate oxidation rates (A) and lactate efflux and uptake rates (B) under baseline perfusion conditions in control (Cont; open bars) and HG/HI (solid bars) groups. *P<0.05 vs control. CHO indicates total carbohydrate oxidation.

To gain further insight into the effects of HG/HI on glycolysis and lactate metabolism, we calculated the ratio of lactate oxidation to lactate uptake and the ratio of lactate efflux to lactate uptake (Table 3). Previous reports have shown that 70% of lactate extracted by the heart is subsequently oxidized.^18,19 In contrast, during reperfusion in the control and DCA groups, only 30% of lactate taken up was subsequently oxidized; in the HG/HI group, this was reduced to 12%. Here, we show that, in both the control and DCA groups, the rate of lactate uptake exceeds lactate efflux rates (Table 4); in the HG/HI group, however, these rates are approximately equal.

View this table: [in this window] [in a new window]   TABLE 4. Ratios of Lactate Oxidation to Lactate Uptake and Lactate Efflux to Lactate Uptake During Reperfusion

	Discussion

Top Abstract Introduction Methods Results Discussion References

 
The most frequently cited mechanisms underlying the protection associated with increased myocardial glucose use are that it improves efficiency by decreasing oxygen consumption²⁰ and improves the coupling between glucose oxidation and glycolysis, thereby reducing intracellular acidosis.^10,11 Surprisingly, however, given the considerable interest in this area, remarkably few studies have directly evaluated these mechanisms, particularly under conditions in which, in addition to glucose, other exogenous sources of pyruvate such as lactate and pyruvate were present at physiologically relevant concentrations. We report here, for the first time, a comparison between the effect of direct activation of carbohydrate oxidation using DCA with stimulation of cardiac glucose use by increasing glucose and insulin concentrations (HG/HI) on cardiac efficiency and the relationship between glucose oxidation and glycolysis after ischemia and reperfusion. The results demonstrated that HG/HI significantly improved the rate of functional recovery and markedly increased efficiency compared with the control and DCA groups; however, this was not accompanied by a reduction in fatty acid oxidation or an increase in the ratio of glucose oxidation to glycolysis. Conversely, although DCA decreased fatty acid oxidation and increased the ratio of glucose oxidation to glycolysis, this result had no beneficial effect on the response to ischemia and reperfusion. Consequently, although these data clearly support the notion that increasing myocardial glucose use is beneficial in the setting of ischemia and reperfusion, this protective effect does not appear to be mediated by the mechanisms typically associated with this phenomenon.

The relationship between improved efficiency and decreased fatty acid oxidation is usually attributed to the fact that the amount of ATP produced per unit of oxygen consumed is 12% greater when glucose compared with palmitate is the sole energy source⁹; however, the amount of ATP produced per oxygen consumed by lactate or pyruvate oxidation falls midway between that for glucose and palmitate. Because lactate and pyruvate contribute appreciably to oxidative energy metabolism both under normal conditions^12–14 and during reperfusion (Figure 2), it seems unlikely that physiologically relevant shifts in substrate oxidation would greatly affect myocardial oxygen consumption. Furthermore, even though DCA decreased fatty acid oxidation by 5-fold after reperfusion, it did not reduce oxygen consumption. Although increased levels of exogenous fatty acids significantly increase basal myocardial oxygen requirements, the increase in oxygen consumption is too large to be accounted for by differences in efficiency of ATP production.²¹ This suggests that if exogenous fatty acid concentrations are constant, as was the case here, shifts in the contribution of fatty acids to oxidative energy metabolism do not lead to measurable changes in oxygen consumed per unit work, whereas elevated exogenous fatty acids could impair cardiac efficiency via mechanisms independent of changes in substrate oxidation. Thus, strategies designed to reduced circulating levels of fatty acids may well be of greater benefit in the treatment of myocardial ischemia than those targeting the regulation of cardiac substrate oxidation.

The detrimental effects of increased fatty acid oxidation in a range of pathological conditions, including cardiac ischemia, have also been attributed to the "uncoupling" of glucose oxidation from glycolysis.^10,11 Improving this relationship has been one of the proposed mechanisms underlying the efficacy of fatty acid oxidation inhibitors such as trimetazidine and ranolazine in protecting against ischemic injury^6–8; however, this proposed mechanism is based almost exclusively on studies in which glucose is considered to be the primary, if not the only, source for pyruvate oxidation. Clearly, this is not the case in vivo where resting lactate levels are 1 mmol/L and can easily reach 5 mmol/L in response to exercise, trauma, or stress.^22,23 As shown in Table 2, both lactate and pyruvate contribute significantly to oxidative ATP production. It is noteworthy that even though lactate is present at a 5-fold-lower concentration than glucose in the control group, its contribution to ATP production is >3-fold higher. Furthermore, despite the fact that pyruvate is present at a 50-fold-lower concentration than glucose, its contribution to ATP production is similar to that from glucose. This is consistent with other reports that examine glucose, lactate, and pyruvate oxidation.^12–14 Here, we found that although DCA increased the ratio of glucose oxidation to glycolysis by 5-fold compared with the HG/HI group, functional recovery was not improved; indeed, we found that an increase in glycolytic flux relative to glucose oxidation was associated with improved functional recovery. Thus, at least in this setting, increasing glucose oxidation rates relative to glycolysis rates was not protective. It is possible that this mechanism is applicable when glucose is the only exogenous source of pyruvate.

Contrary to the concept of decreasing glycolytic flux relative to glucose oxidation, the primary metabolic difference between the HG/HI group and the other 2 groups was an increase in glycolytic lactate efflux during both ischemia and reperfusion. The latter resulted in a significant increase in total ATP production coming from glycolysis during reperfusion. The increase in glycolytic lactate efflux during LFI in the HG/HI group could be a result of increased glucose entry into the cell or increased mobilization of glycogen, possibly resulting from higher glycogen levels in this group before ischemia. This could lead to higher ATP levels at the end of ischemia and on reperfusion, which may be an important contributing factor to the improved cardiac efficiency and functional recovery in the HG/HI group; however, the relationship between bioenergetic status and cardiac efficiency remains to be determined.

The importance of glycolytic ATP production in improving recovery from ischemia has been demonstrated by a number of investigators. Cross et al²⁴ showed that, in the presence of residual flow, increasing glycolysis during ischemia was protective. Others have shown that inhibition of glycolysis during reperfusion markedly impaired recovery,²⁵ supporting the concept that glycolytic ATP was critical in maintaining cardiomyocyte function. Furthermore, several studies have demonstrated a direct link between glycolytic ATP production and membrane ion transport, which may reflect compartmentation of glycolytic ATP production in the vicinity of sarcolemmal or sarcoplasmic reticulum ion pumping ATPases.^26–28 Thus, improved glycolytic ATP production could account for both the improved ischemic and postischemic diastolic function observed in the HG/HI group.

Ischemic contracture, typically associated with increased severity of ischemic injury,²⁹ can be attenuated by increasing glycolysis.²⁴ The reduction in contracture in the HG/HI group associated with increased glycolytic lactate efflux and improved recovery of function is certainly consistent with this concept. Surprisingly, in the DCA group, the development of contracture was accelerated relative to the control group, although functional recovery ultimately was not significantly different. A dissociation between the severity of ischemic contracture and functional recovery has been previously reported by Kolocassides et al,³⁰ who found that the onset of contracture was associated with ATP depletion whereas the improved recovery of function was associated with less severe acidosis. It is worth noting that although DCA is a well-established activator of pyruvate oxidation, it has been reported to inhibit glycolysis,³¹ which could account for the accelerated development of contracture. Further studies are needed to better understand the impact of DCA on ATP hydrolysis, intracellular acidosis, and development of ischemic contracture.

It is also possible that insulin may exert a direct protective effect independent of its effects on metabolism; however, the development of acidosis during no-flow ischemia has been shown to inhibit insulin receptor tyrosine kinase signaling, thereby preventing activation of downstream targets.³² Thus, it is possible that the insulin effects are mediated primarily at the time of reperfusion. For example, Jonassen et al³³ reported that increased levels of insulin administered at the time of reperfusion afforded significant protection that was mediated independently of effects of glucose metabolism and was associated with activation of cell survival signaling pathways. This could also account, at least in part, for the improved recovery of function seen here in the HG/HI group. Interestingly, we found that under normal perfusion conditions, there was a significant increase in carbohydrate oxidation in the HG/HI group that was absent during reperfusion. This suggests that, after ischemia and reperfusion, the effect of insulin on stimulating carbohydrate oxidation was blunted and could account for the increased contribution of fatty acids to oxidative energy metabolism after ischemia and reperfusion compared with normoxic perfusion. It was also intriguing that HG/HI treatment also significantly affected the ratio of lactate oxidation to uptake and the ratio of lactate efflux to uptake (Table 3). The mechanisms underlying these changes and the relationship to the improved recovery of function remain to be determined; however, hyperinsulinemia has been reported to increase lactate extraction in vivo,¹⁷ and it has been proposed that changes in the ratio of lactate efflux to uptake may reflect alterations in cytosolic redox state.¹⁹ At the very least, these data demonstrate that the impact of HG/HI treatment on cardiac metabolism go beyond simply altering the relationship between glucose and fatty acid oxidation.

An important distinction between this report and many of those that have examined the impact of altered substrate use in mediating ischemic injury is that we used a model of LFI rather than zero-flow ischemia. Cross et al²⁴ reported that increased glycolytic flux resulting from glycogen loading was beneficial during LFI but was detrimental in a zero-flow ischemia model. Furthermore, whereas oxidative energy production is minimal during zero-flow ischemia, we have recently shown that oxidative energy metabolism contributes 30% to 50% of ATP production during the LFI protocol used here.¹³ Interestingly, King et al³⁴ showed that the provision of additional oxidizable substrates such as long-chain fatty acids improved functional recovery after a similar LFI protocol compared with situations when glucose was the only available substrate. We believe that using an LFI protocol is relevant because, in both large animal studies and patients, there is considerable residual flow in the infarct zone.^35,36 Furthermore, areas of reduced flow represent regions that could be accessible to therapeutic interventions before reperfusion. Although, much of the focus on development of agents designed to improve recovery from ischemic injury has emphasized treatment at the time of reperfusion, it is noteworthy that treatment was started before revascularization began in many GIK trials. Furthermore, interventions before the onset of ischemia are possible in the context of perioperative myocardial infarction, which affects 3% to 6% of patients undergoing coronary artery bypass³⁷ and is considered one of the most important potentially reversible risk factors for mortality after noncardiac surgery.³⁸

In conclusion, we compared the effect of stimulating cardiac glucose use by increasing glucose and insulin concentrations with direct activation of carbohydrate oxidation (with DCA) on the metabolic and functional response to ischemia and reperfusion under conditions in which physiological concentrations of lactate, pyruvate, glucose, and palmitate were provided. We found that the combination of increased glucose and insulin improved functional recovery compared with DCA treatment despite the fact that DCA treatment had a greater impact on increasing carbohydrate oxidation. Furthermore, the primary metabolic difference between the HG/HI group and the other 2 groups was an increase in glycolytic lactate efflux during both ischemia and reperfusion, which is contrary to the concept that decreasing glycolytic flux relative to glucose oxidation is beneficial. This dissociation between functional recovery and increased carbohydrate oxidation suggests that the mechanisms underlying the protection associated with increased myocardial glucose use are not related to changes in cardiac efficiency or the coupling of glucose oxidation to glycolysis.

	Acknowledgments

 
This work was supported in part by grants from the National Heart, Lung and Blood Institute (HL-67464 and HL-48789 to Dr Chatham). All NMR studies were performed at the UAB NMR Core Facility funded by NCI Cancer Center support grant CA-13148. We thank Charlye Brocks and Clarence Forrest for technical assistance.

	References

Top Abstract Introduction Methods Results Discussion References

 

1. Sodi-Pallares D, Testelli M, Fishleder F. Effects of intravenous infusion of a potassium-insulin-glucose solution on the electrographic signs of myocardial infarction. Am J Cardiol. 1962; 9: 166–181.[CrossRef][Medline] [Order article via Infotrieve]
   
2. van der Horst IC, Zijlstra F, van’t Hof AW, Doggen CJ, de Boer MJ, Suryapranata H, Hoorntje JC, Dambrink JH, Gans RO, Bilo HJ. Glucose-insulin-potassium infusion inpatients treated with primary angioplasty for acute myocardial infarction: the Glucose-Insulin-Potassium Study: a randomized trial. J Am Coll Cardiol. 2003; 42: 784–791.[Abstract/Free Full Text]
   
3. Pache J, Kastrati A, Mehilli J, Bollwein H, Ndrepepa G, Schuhlen H, Martinoff S, Seyfarth M, Nekolla S, Dirschinger J, Schwaiger M, Schomig A. A randomized evaluation of the effects of glucose-insulin-potassium infusion on myocardial salvage in patients with acute myocardial infarction treated with reperfusion therapy. Am Heart J. 2004; 148: e3.[Medline] [Order article via Infotrieve]
   
4. Fath-Ordoubadi F, Beatt KJ. Glucose-insulin-potassium therapy for treatment of acute myocardial infarction: an overview of randomized placebo-controlled trials. Circulation. 1997; 96: 1152–1156.[Abstract/Free Full Text]
   
5. Diaz R, Paolasso EA, Piegas LS, Tajer CD, Moreno MG, Corvalan R, Isea JE, Romero G. Metabolic modulation of acute myocardial infarction: the ECLA (Estudios Cardiologicos Latinoamerica) Collaborative Group. Circulation. 1998; 98: 2227–2234.[Abstract/Free Full Text]
   
6. Stanley WC, Lopaschuk GD, Hall JL, McCormack JG. Regulation of myocardial carbohydrate metabolism under normal and ischaemic conditions: potential for pharmacological interventions. Cardiovasc Res. 1997; 33: 243–257.[Free Full Text]
   
7. Chaitman BR, Pepine CJ, Parker JO, Skopal J, Chumakova G, Kuch J, Wang W, Skettino SL, Wolff AA. Effects of ranolazine with atenolol, amlodipine, or diltiazem on exercise tolerance and angina frequency in patients with severe chronic angina: a randomized controlled trial. JAMA. 2004; 291: 309–316.[Abstract/Free Full Text]
   
8. Fragasso G, Piatti PM, Monti L, Palloshi A, Lu C, Valsecchi G, Setola E, Calori G, Pozza G, Margonato A, Chierchia S. Acute effects of heparin administration on the ischemic threshold of patients with coronary artery disease: evaluation of the protective role of the metabolic modulator trimetazidine. J Am Coll Cardiol. 2002; 39: 413–419.[Abstract/Free Full Text]
   
9. Opie LH. Heart: Physiology: From Cell to Circulation. 4th ed. Philadelphia, Pa: Lippincott, Williams and Wilkins; 2004.
   
10. Lopaschuk GD, Wambolt RB, Barr RL. An imbalance between glycolysis and glucose oxidation is a possible explanation for the detrimental effects of high levels of fatty acids during aerobic reperfusion of ischemic hearts. J Pharmacol Exp Ther. 1993; 264: 135–144.[Abstract/Free Full Text]
    
11. Liu Q, Docherty JC, Rendell JC, Clanachan AS, Lopaschuk GD. High levels of fatty acids delay the recovery of intracellular pH and cardiac efficiency in post-ischemic hearts by inhibiting glucose oxidation. J Am Coll Cardiol. 2002; 39: 718–725.[Abstract/Free Full Text]
    
12. Lloyd S, Brocks C, Chatham JC. Differential modulation of glucose, lactate and pyruvate oxidation by insulin and dichloroacetate in the isolated perfused rat heart. Am J Physiol Heart Circ Physiol. 2003; 285: H163–H172.[Abstract/Free Full Text]
    
13. Lloyd SG, Wang PP, Zeng H, Chatham JC. The impact of low flow ischemia on substrate oxidation and glycolysis in the isolated perfused rat heart. Am J Physiol Heart Circ Physiol. 2004; 287: 351–362.
    
14. Vincent G, Khairallah M, Bouchard B, Des Rosiers C. Metabolic phenotyping of the diseased rat heart using ¹³C-substrates and ex vivo perfusion in the working mode. Mol Cell Biochem. 2003; 242: 89–99.[CrossRef][Medline] [Order article via Infotrieve]
    
15. Wang P, Chatham JC. The onset of diabetes in Zucker diabetic fatty (ZDF) rats leads to improved recovery of function following ischemia in the isolated perfused heart. Am J Physiol Endocrinol Metab. 2004; 286: E725–E736.[Abstract/Free Full Text]
    
16. Hinkle PC, Kumar MA, Resetar A, Harris DL. Mechanistic stoichiometry of mitochondrial oxidative phosphorylation. Biochemistry. 1991; 30: 3576–3582.[CrossRef][Medline] [Order article via Infotrieve]
    
17. Young LH, Zaret BL, Barrett EJ. Physiologic hyperinsulinemia stimulates lactate extraction by heart muscle in the conscious dog. Metabolism. 1989; 38: 1115–1119.[CrossRef][Medline] [Order article via Infotrieve]
    
18. Bartelds B, Knoester H, Beaufort-Krol GCM, Smid GB, Takens J, Zijlstra WG, Heymans HSA, Kuipers JRG. Myocardial lactate metabolism in fetal and newborn lambs. Circulation. 1999; 99: 1892–1897.[Abstract/Free Full Text]
    
19. Chatham JC, Des Rosiers C, Forder JR. Evidence of separate pathways for lactate uptake and release by the perfused rat heart. Am J Physiol Endocrinol Metab. 2001; 281: E794–E802.[Abstract/Free Full Text]
    
20. Stanley WC, Hall JL, Hacker TA, Hernandez LA, Whitesell LF. Decreased myocardial glucose uptake during ischemia in diabetic swine. Metabolism. 1997; 46: 168–172.[CrossRef][Medline] [Order article via Infotrieve]
    
21. Burkhoff D, Weiss RG, Schulman SP, Kalil-Filho R, Wannenburg T, Gerstenblith G. Influence of metabolic substrate on rat heart function and metabolism at different coronary flows. Am J Physiol. 1991; 261: H741–H750.[Medline] [Order article via Infotrieve]
    
22. Hatherill M, McIntyre AG, Wattie M, Murdoch IA. Early hyperlactataemia in critically ill children. Intensive Care Med. 2000; 26: 314–318.[CrossRef][Medline] [Order article via Infotrieve]
    
23. Kemppainen J, Fujimoto T, Kalliokoski KK, Viljanen T, Nuutila P, Knuuti J. Myocardial and skeletal muscle glucose uptake during exercise. J Physiol. 2002; 542: 403–412.[Abstract/Free Full Text]
    
24. Cross HR, Opie LH, Radda GK, Clarke K. Is a high glycogen content beneficial or detrimental to the ischemic rat heart? A controversy resolved. Circ Res. 1996; 78: 482–491.[Abstract/Free Full Text]
    
25. Jeremy RW, Ambrosio G, Pike MM, Jacobus WE, Becker LC. The functional recovery of post-ischemic myocardium requires glycolysis during early reperfusion. J Mol Cell Cardiol. 1993; 25: 261–276.[CrossRef][Medline] [Order article via Infotrieve]
    
26. Dizon J, Burkhoff D, Tauskela J, Whang J, Cannon P, Katz J. Metabolic inhibition in the perfused rat heart: evidence for glycolytic requirement for normal sodium homeostasis. Am J Physiol. 1998; 274: H1082–H1089.[Medline] [Order article via Infotrieve]
    
27. Weiss J, Hiltbrand B. Functional compartmentation of glycolytic versus oxidative metabolism in isolated rabbit heart. J Clin Invest. 1985; 75: 436–447.[Medline] [Order article via Infotrieve]
    
28. Xu KY, Zweier JL, Becker LC. Functional coupling between glycolysis and sarcoplasmic reticulum Ca²⁺ transport. Circ Res. 1995; 77: 88–97.[Abstract/Free Full Text]
    
29. Kingsley PB, Sako EY, Yang MQ, Zimmer SD, Ugurbil K, Foker JE, From AH. Ischemic contracture begins when anaerobic glycolysis stops: a ³¹P-NMR study of isolated rat hearts. Am J Physiol Heart Circ Physiol. 1991; 261: H469–H478.[Abstract/Free Full Text]
    
30. Kolocassides KG, Seymour AM, Galinanes M, Hearse DJ. Paradoxical effect of ischemic preconditioning on ischemic contracture? NMR studies of energy metabolism and intracellular pH in the rat heart. J Mol Cell Cardiol. 1996; 28: 1045–1057.[CrossRef][Medline] [Order article via Infotrieve]
    
31. Stacpoole PW. The pharmacology of dichloroacetate. Metabolism. 1989; 38: 1124–1144.[CrossRef][Medline] [Order article via Infotrieve]
    
32. Beauloye C, Bertrand L, Krause U, Marsin AS, Dresselaers T, Vanstapel F, Vanoverschelde JL, Hue L. No-flow ischemia inhibits insulin signaling in heart by decreasing intracellular pH. Circ Res. 2001; 88: 513–519.[Abstract/Free Full Text]
    
33. Jonassen AK, Sack MN, Mjos OD, Yellon DM. Myocardial protection by insulin at reperfusion requires early administration and is mediated via Akt and p70s6 kinase cell-survival signaling. Circ Res. 2001; 89: 1191–1198.[Abstract/Free Full Text]
    
34. King LM, Sidell RJ, Wilding JR, Radda GK, Clarke K. Free fatty acids, but not ketone bodies, protect diabetic rat hearts during low-flow ischemia. Am J Physiol Heart Circ Physiol. 2001; 280: H1173–H1181.[Abstract/Free Full Text]
    
35. Sabia PJ, Powers ER, Ragosta M, Sarembock IJ, Burwell LR, Kaul S. An association between collateral blood flow and myocardial viability in patients with recent myocardial infarction. N Engl J Med. 1992; 327: 1825–1831.[Abstract]
    
36. Christian TF, O’Connor MK, Schwartz RS, Gibbons RJ, Ritman EL. Technetium-99m MIBI to assess coronary collateral flow during acute myocardial infarction in two closed-chest animal models. J Nucl Med. 1997; 38: 1840–1846.[Abstract/Free Full Text]
    
37. Force T, Hibberd P, Weeks G, Kemper AJ, Bloomfield P, Tow D, Josa M, Khuri S, Parisi AF. Perioperative myocardial infarction after coronary artery bypass surgery: clinical significance and approach to risk stratification. Circulation. 1990; 82: 903–912.[Abstract/Free Full Text]
    
38. Mangano DT, Layug EL, Wallace A, Tateo I. Effect of atenolol on mortality and cardiovascular morbidity after noncardiac surgery: Multicenter Study of Perioperative Ischemia Research Group. N Engl J Med. 1996; 335: 1713–1720.[Abstract/Free Full Text]
    

This article has been cited by other articles:

				M. Gandhi, B. A. Finegan, and A. S. Clanachan Role of glucose metabolism in the recovery of postischemic LV mechanical function: effects of insulin and other metabolic modulators Am J Physiol Heart Circ Physiol, June 1, 2008; 294(6): H2576 - H2586. [Abstract] [Full Text] [PDF]

				S. W. Zarich and R. W. Nesto Implications and Treatment of Acute Hyperglycemia in the Setting of Acute Myocardial Infarction Circulation, May 8, 2007; 115(18): e436 - e439. [Full Text] [PDF]

				A. D. Hafstad, A. M. Khalid, O.-J. How, T. S. Larsen, and E. Aasum Glucose and insulin improve cardiac efficiency and postischemic functional recovery in perfused hearts from type 2 diabetic (db/db) mice Am J Physiol Endocrinol Metab, May 1, 2007; 292(5): E1288 - E1294. [Abstract] [Full Text] [PDF]

				N. Fulop, Z. Zhang, R. B. Marchase, and J. C. Chatham Glucosamine cardioprotection in perfused rat hearts associated with increased O-linked N-acetylglucosamine protein modification and altered p38 activation Am J Physiol Heart Circ Physiol, May 1, 2007; 292(5): H2227 - H2236. [Abstract] [Full Text] [PDF]

				K. A. B. Davey, P. B. Garlick, A. Warley, and R. Southworth Immunogold labeling study of the distribution of GLUT-1 and GLUT-4 in cardiac tissue following stimulation by insulin or ischemia Am J Physiol Heart Circ Physiol, April 1, 2007; 292(4): H2009 - H2019. [Abstract] [Full Text] [PDF]

				H. B. van Wezel, C. J. Zuurbier, E. de Jonge, E. W. C. M. van Dam, J. van Dijk, E. Endert, B. A. de Mol, and E. Fliers Differential Effects of a Perioperative Hyperinsulinemic Normoglycemic Clamp on the Neurohumoral Stress Response during Coronary Artery Surgery J. Clin. Endocrinol. Metab., October 1, 2006; 91(10): 4144 - 4153. [Abstract] [Full Text] [PDF]

				B. Ellger, Y. Debaveye, I. Vanhorebeek, L. Langouche, A. Giulietti, E. Van Etten, P. Herijgers, C. Mathieu, and G. Van den Berghe Survival benefits of intensive insulin therapy in critical illness: impact of maintaining normoglycemia versus glycemia-independent actions of insulin. Diabetes, April 1, 2006; 55(4): 1096 - 1105. [Abstract] [Full Text] [PDF]

This Article Abstract Full Text (PDF) All Versions of this Article: 111/16/2066    most recent 01.CIR.0000162466.06150.D4v1 Alert me when this article is cited Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Request Permissions Citing Articles Citing Articles via HighWire Citing Articles via Google Scholar Google Scholar Articles by Wang, P. Articles by Chatham, J. C. Search for Related Content PubMed PubMed Citation Articles by Wang, P. Articles by Chatham, J. C. Related Collections Contractile function Biochemistry and metabolism Animal models of human disease Energy metabolism