Lumped constant for deoxyglucose is decreased when myocardial glucose uptake is enhanced

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Lumped constant for deoxyglucose is decreased when myocardial glucose uptake is enhanced

Katsuji Hashimoto¹, Tsunehiko Nishimura¹, Ken-Ichi Imahashi¹, Hitoshi Yamaguchi¹, Masatsugu Hori², and Hideo Kusuoka¹

¹ Division of Tracer Kinetics, Biomedical Research Center, and ² First Department of Medicine, Osaka University Medical School, Suita, Osaka 565-0871, Japan

ABSTRACT

Top
Abstract
Introduction
Methods
Results
Discussion
References

Quantification of myocardial glucose uptake by positron emission tomography with [¹⁸F]fluorodeoxyglucose (FDG) requires the "lumped constant" (LC),which corrects the difference of affinity between glucose andFDG to glucose transporters and phosphorylating system. SinceLC was introduced, it has been considered to be constant. However,this has recently been questioned. To elucidate the constancyof LC by other than radioisotope techniques, the accumulationrate of sugar phosphates (d[SP]/dt) was measured in isolated,perfused rat hearts by ³¹P NMR spectroscopy with 2-deoxyglucose (DG). We postulate $alpha$ asthe affinity of DG to transporters and the phosphorylating systemrelative to that of glucose. Theoretically, $alpha$ is equivalent toLC. We determined $alpha$ by measuring d[SP]/dt at DG concentration([DG]) = 10, 7, 5, and 3 mmol/l, keeping the total of glucoseconcentration ([glucose]) and [DG] to 10 mmol/l. When the glucoseuptake was enhanced by insulin (10 mU/ml) or stunning, calculated $alpha$ was reduced (insulin stimulated, 0.15; stunning, 0.19) comparedwith the control (0.59). These results indicate that LC can beevaluated by methods without radiolabeled tracers and is smallerwhen glucose uptake isaugmented.

insulin; myocardial stunning; nuclear magnetic resonance spectroscopy

	INTRODUCTION

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THE TRACER [¹⁸F]fluorodeoxyglucose (FDG) has been used widely with positron emission tomography (PET) to estimate glucose utilizationin myocardium (2, 13, 17-19). To quantify the myocardial glucoseuptake with FDG, it is necessary to introduce the "lumped constant"(LC) because the affinity of FDG for glucose transporters andphosphorylation enzymes is different from that of glucose. LCwas initially defined by Sokoloff (21) using 2-deoxyglucose(DG) as follows

lumped constant = &lgr;<IT>V</IT>*m<IT>K</IT>m/&PHgr;<IT>V</IT>m<IT>K</IT>*m (1)

where $lambda$ is the ratio of distribution volumes of DG and glucose, $Phi$ is glucose-6-phosphatase activity, V_m and K_m are the maximalvelocity and Michaelis-Menten constant of hexokinase to glucose,respectively, and <IT>V</IT>*m and are V_mand K_m to DG. Because LC was introduced on the basis of experimentsusing radioactive tracers, some conceptual parameters such asdistribution volumes are required to describe and determine LC(21). Whether LC can be determined by methods other than radioisotopetechnique has not beenelucidated.

Since LC was introduced, it has been supposed to be constant. Actually, it has been reported that LC did not change underphysiological conditions (8, 9, 15). Therefore, only onevalue (i.e., 0.6) has been used in quantifying the glucose uptakein myocardium using FDG PET. However, recent studies gave doubtabout the constancy of LC (1, 5, 12, 16). This studyaims to elucidate whether LC can be determined by a method withoutradioactive tracers and whether LC is changeable when myocardialglucose uptake isenhanced.

	METHODS

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The whole heart preparation was described previously (6). Briefly, hearts were excised from male rats (Sprague-Dawley,body wt 400-450 g) anesthetized with pentobarbital sodium (50mg/kg ip; Abbott Laboratories, North Chicago, IL) and heparinized.After excision, the aorta was cannulated, and the hearts wereretrogradely perfused with a modified HEPES buffer (standard perfusate;in mmol/l: 108 NaCl, 5 KCl, 1 MgCl₂, 1.5 CaCl₂, 5 HEPES, 10 glucose,and 20 Na-acetate) bubbled with 100% O₂ at 37°C. Heart rate wasmaintained at 300 beats/min by right ventricular pacing. A latexballoon tied to the end of a polyethylene tube was passed intothe left ventricle (LV) through the mitral valve and connectedto a pressure transducer (SPB-101, San-ei Electric, Tokyo, Japan).The balloon was filled with 25 mmol/l magnesium trimetaphosphatesolution as a standard for ³¹P NMR spectroscopy (10). LV end-diastolic pressure was set at5-10 mmHg by adjusting the balloon volume, and then the balloonwas kept isovolumic throughout the experiment. Aortic pressurewas monitored at the cannulation point of the aorta. LV pressureand aortic pressure were recorded with a direct-writing recorder.Aortic pressure was adjusted to 70-80 mmHg by controlling theflow rate of the perfusion, and flow rate was kept constant throughoutthe experiment except during ischemia. The experiments reportedherein were approved by the Animal Care and Use Committee of OsakaUniversity MedicalSchool.

Determination of DG uptake rate in myocardium. The uptake rate of DG in myocardium was determined as the accumulation rate of sugar phosphates (SP) when glucose in the perfusatewas substituted by DG (6). Acetate (20 mmol/l) was always presentin the perfusate. The signal of phosphorylated DG appears at ~6parts per million in the spectrum as SP (see Fig. 1). The accumulationrate of SP in myocardium (d[SP]/dt, where [SP] is SP concentration)was calculated from the slope of the regression line obtainedfrom the data over 20 min after the substitution of glucose byDG and is expressed in micromoles per gram of wet weight per minute.If SP peak saturated within the initial 20 min, d[SP]/dt was calculatedduring the initial 15min.

The method to determine myocardial DG uptake rate using ³¹P NMR was described previously (6). Briefly, the preparation wasput into a 20-mm-diameter tube and placed into the superconductingmagnet at 9.4 T. ³¹P NMR spectra were obtained on an NMR spectrometer (AMX-400wb,Bruker), for which the resonance frequency for ³¹P equals 161.98 MHz. The free induction decays from the heartusing 60-degree pulses delivered at 2-s intervals were accumulatedand processed. Each spectrum was obtained with 144 pulses, resultingin a total acquisition time of 5min.

Intramyocardial amounts of metabolites were quantified as reported previously (10). Briefly, the amounts of phosphorus compoundsin the myocardium were obtained by planimetry of the area underthe corresponding peak. The tissue contents were normalized bythe peak for the magnesium trimetaphosphate standard in the LVballoon. The calculated amount was divided by the measured weightof each heart to yield concentrations in micromoles per gram ofwetweight.

Calculation of parameter. Glucose and DG have different affinities to the glucose transporter (GLUT)-hexokinase system. Therefore, it has been consideredthat myocardial DG uptake is modified when glucose and DG arepresent simultaneously in the perfusate and that these two substratesare in competition to this system (21). To investigate the relativerelation between glucose and DG to the GLUT-hexokinase system,the effect of coexisting glucose on myocardial DG uptake was evaluatedin perfused hearts. Hearts were perfused with the standard solution,and then glucose in the perfusate was completely or partiallyreplaced by DG but the total of glucose concentration ([glucose])and DG concentration ([DG]) was kept to 10 mmol/l. d[SP]/dt wasmeasured in the hearts perfused with solutions of the following[DG] and [glucose]: 3:7, 5:5, 7:3, and 10:0 mmol/l.

To evaluate the relative relation between glucose and DG to the GLUT-hexokinase system quantitatively, we introduced the followingmodel. In this model, myocardial uptake of glucose and DG is consideredto be determined by two factors: one is [glucose] and [DG], andthe other is the relative affinity of glucose and DG to the GLUT-phosphorylationsystem. When [DG] in the perfusate is supposed to be x mmol/l,[glucose] in the perfusate is (10 $-$ x) mmol/l because the totalof [DG] and [glucose] is kept to 10 mmol/l in our experiments.If affinity of DG to transporter and phosphorylation system relativeto that of glucose is postulated as $alpha$ , the ratio of myocardialDG uptake to that of glucose is equal to $alpha$ x:(10 $-$ x). The accumulationof SP is mainly caused by the accumulation of deoxyglucose-6-phosphate.Therefore, d[SP]/dt normalized by its maximal value is expressedas

&agr;<IT>x</IT>/[(10 − <IT>x</IT>) + &agr;<IT>x</IT>]

(2)

The value of $alpha$ was determined by fitting data sets obtained with changing [DG] to Eq. 2.

Statistical analysis. Data are presented as means ± SE. Multiple comparison was performed using ANOVA with Scheffé's test. A P value <0.05 wasconsidered as significant. Curve fitting was performed with SigmaPlotversion 2.01 (Jandel ScientificSoftware).

	RESULTS

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$alpha$ In control hearts. Hearts were first perfused with the standard perfusate and allowed to stabilize. Afterward, NMR spectra and mechanical functionwere measured for 20 min as an initial control. Glucose in a perfusatewas then totally or partially replaced by DG. Figure 1 illustratesthe changes in P NMR spectra before and after the exposure toDG. SP was accumulated after the perfusate was switched. Figure2 summarizes the changes of [SP] in different [DG]. When [DG]was reduced from 10 to 3 mmol/l, keeping the total concentrationof DG and glucose to 10 mmol/l, the accumulation of SP becameslower and d[SP]/dt was decreased (Table 1).

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Fig. 1. Changes in sugar phosphate (SP) peak in ³¹P NMR spectra after substitution of glucose (10 mmol/l) with 2-deoxyglucose (DG, 10 mmol/l). A: spectrum obtained during control perfusion, i.e., without DG. B: spectrum obtained 10-15 min after switching from standard perfusate to solution containing DG (10 mmol/l). 1, SP; 2, inorganic phosphate; 3, phosphocreatine; 4-6, 3 phosphates of ATP ( $gamma$ , $alpha$ , and $beta$ , respectively); 7, magnesium trimetaphosphate (standard in left ventricular balloon).

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Fig. 2. Changes in myocardial SP concentration ([SP]) in control hearts perfused with solution containing different concentrations of DG and glucose. Symbols represent hearts perfused with solution containing following composition of DG and glucose (in mmol/l): $bullet$ , 10:0; $open circle$ , 7:3;

, 5:5;

, 3:7. * P < 0.05, ** P < 0.01 vs. DG = 10 mmol/l.

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Table 1. d[SP]/dt at different DG and glucose concentrations in control, insulin-stimulated, and stunned myocardium

d[SP]/dt of the hearts perfused with the solution in which glucose was totally replaced by DG gave the maximal rate of themyocardial sugar uptake because there was no competition betweenDG and glucose. Thus d[SP]/dt at different [DG] was normalizedby d[SP]/dt at [DG] = 10 mmol/l and fitted to Eq. 2. The bestfit was obtained when $alpha$ = 0.59 (Fig. 3).

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Fig. 3. SP accumulation rate (d[SP]/dt) normalized by d[SP]/dt at [DG] = 10 mmol/l. $open circle$ , control hearts; $bullet$ , insulin-stimulated hearts; $triangle$ , stunned myocardium. Solid line, dashed line, and dotted line indicate relation best fitted to equation y = $alpha$ x /[(10 $-$ x) + $alpha$ x], where $alpha$ is affinity of DG to transporters and phosphorylation system relative to that of glucose, in control, insulin-stimulated, and stunned groups, respectively. * P < 0.05, ** P < 0.01 vs. control hearts.

$alpha$ In hearts enhanced in glucose uptake. We also investigated the change in $alpha$ when glucose uptake was enhanced. To enhance myocardial glucose uptake, we first addedinsulin to the perfusate. In this group, the standard perfusatewas switched to that containing DG 10 min after the administrationof insulin (regular insulin, 10 mU/ml; Shimizu Pharmacy, Shizuoka,Japan). When compared in the control hearts, insulin augmentedd[SP]/dt at higher concentrations of DG but not significantlyat lower concentrations of DG (Table 1). These results suggestthat $alpha$ in insulin-stimulated hearts is not equal to that in controlhearts. The fitting revealed that $alpha$ was equal to 0.15 (Fig. 3).We also used stunning to enhance myocardial glucose uptake. Aspreviously reported, d[SP]/dt significantly increases in stunnedmyocardium (6). To stun myocardium, we reperfused hearts after15-min global ischemia at 37°C. Hearts were perfused with thestandard solution before ischemia and reperfused with the solutioncontaining DG. In stunned hearts, d[SP]/dt was significantly increasedat higher [DG] but not at lower [DG] as was observed in insulin-stimulatedhearts (Table 1). The fitting revealed that $alpha$ was equal to 0.19(Fig. 3).

	DISCUSSION

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Relation between $alpha$ and LC. The LC was introduced by Sokoloff et al. (21) based on the three-compartment model describing the dynamics of glucose andDG (Fig. 4). On the basis of this model, the glucose utilizationrate, R_i, is described by Eq. 3, when substrate concentrationsand rate constants are defined as in Fig. 4 (7, 14)

R<IT>i</IT> = 1/(LC)<IT>k</IT>*1<IT>k</IT>*3/(<IT>k</IT>*2 + <IT>k</IT>*3)CP (3)

According to the assumption of a steady state in myocardial sugar uptake and metabolism, i.e., dC*E /dt = 0

<IT>k</IT>*1C*P = (<IT>k</IT>*2 + <IT>k</IT>*3)C*E (4)

Therefore

R<IT>i</IT> = 1/(LC) CP/C*P<IT>k</IT>*3C*E (5)

LC = (<IT>k</IT>*3C*E/C*P)/(R<IT>i</IT>/CP) (6)

This equation indicates that LC is equal to the ratio of the unit utilization rate of DG (/)to that of glucose (R_i/C_P). The definition of LC in this manneris completely equivalent to the definition of $alpha$ in our model.Actually, the estimated value of $alpha$ in control hearts in our experimentswas equal to 0.59 and agrees well with the LC currently used forFDG (0.6) (8, 9, 15) or that measured with DG in rat (5).Thus these results indicate that our method is a new method todetermine LC without radioactive tracers.

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Fig. 4. Three-compartment model for kinetics of glucose and DG. Left compartment represents extracellular space for glucose and DG. Middle compartment represents intracellular space for free glucose and free DG. Right compartment represents intracellular space for glucose-6-phosphate and deoxyglucose-6-phosphate. k and C are rate constant and concentration, respectively, where subscripts P, E, M indicate extracellular, intracellular free, and intracellular phosphorylated, respectively. Quantities for DG and glucose are denoted by symbols with and without asterisk, respectively. Modified from Sokoloff et al. (21).

Radioactive tracer has a lot of advantages in measuring metabolic states. However, as shown by the original definition ofLC (21), many assumptions with compartmental models are necessaryto quantify metabolic parameters. Recent studies adopted the directcomparison of metabolic rates of FDG/DG and glucose (4, 5),and these methods are close to our new method measuring DG accumulationdirectly. Our method is equivalent to those with radioactive tracersand is preferable to perform in those countries, including Japan,where the use of radioisotopes in whole animals in vivo is difficultbecause of major restriction by legalregulations.

Change in LC at enhanced glucose uptake rate. Coupled with the previous discussion, our results indicate that LC decreases when glucose uptake is enhanced. Ng et al. (12)reported that 10 mU/ml insulin decreased LC from 0.94 to 0.33when [glucose] was kept to 5 mmol/l. Recently, it is reportedthat myocardial glucose uptake measured with DG underestimatestrue uptake in insulin-stimulated myocardium (5). The variabilityof LC, depending on the condition to which hearts are exposed,is proposed as the mechanism for the underestimation of glucoseuptake. Changes in LC measured by FDG PET were also reported (1);LC showed biphasic change, that is, increased at lower serum levelof insulin and decreased at higher serum level ofinsulin.

Changes in LC were also suggested in reperfused myocardium. Doenst et al. (3) showed that FDG retention in reperfused heartswas blunted compared with that before ischemia and then graduallyincreased during the reperfusion period. These results also suggesta change in LC. Actually, the decrease in LC was reported in heartsreperfused after low-flow ischemia (4). Glucose uptake ratein stunned myocardium is enhanced just after reperfusion and graduallydecreases during reperfusion (6). Therefore, the time-dependentchange in the FDG retention pattern may be caused by the changein LC parallel to the withdrawal of glucose uptake in reperfusedmyocardium.

Mechanism of changes in LC. The mechanism for the change in LC has not been clarified. Ng et al. (12) suggested that LC may be sensitive to [glucose]in the perfusate and that LC rises with increase in [glucose]because glycolysis comes to be rate limiting. In fact, low [glucose]increased LC in their experiments. This may be caused by the limitationin the transport of glucose via GLUT, because the influx of glucoseis determined by the concentration gradient. In contrast, thetotal sugar concentration in our experiments was kept to 10 mmol/l,which may be enough to saturate the GLUT. Thus the transport stepwould not be the rate-limiting step in our experiments. Russellet al. (16) reported that insulin increased hexokinase activityassociated with the mitochondrial fraction. Hexokinase bound tomitochondria exhibited an 8.5-fold increase in K_m for DG comparedwith that of hexokinase in the cytosol (16). Therefore, insulin-dependentchange in the relative affinity to hexokinase between DG and glucosemay play an important role in the change ofLC.

GLUT4 and GLUT1 are the primary forms expressed in adult mammalian heart muscle (22). Insulin increases the number of GLUT4on the cell surface (20, 23). Ischemia also translocates GLUT4and GLUT 1 to the cell surface (23, 24). Therefore, the changesin the population of GLUT on the cell surface may also be amechanism.

Recently, Doenst and Taegtmeyer (4) showed a significant increase of intracellular free glucose during reperfusion thataccompanied the decrease in LC, supporting the hypothesis thatglucose influx exceeds the ability ofphosphorylation.

Limitations. In this study, we determined the relative affinity of DG to glucose in the GLUT-hexokinase system using NMR, not radioisotope.NMR cannot detect the concentration of tracer. However, P NMRdetects only the phosphorylated form of DG within the cell. Therefore,we need not discriminate C*E and C*M by compartment analysis.Nevertheless, LC in control hearts determined by the NMR methodwas equal to the value previously reported with the radioactivetracer technique (8, 9, 15). Thus both methods can beconsidered to be equivalent to measureLC.

Hexokinase phosphorylates DG and glucose with different preferences (4, 16), suggesting that our estimation for myocardialaccumulation of phosphorylated DG may overestimate the actualvalue even though glucose-6-phosphate is metabolized further.However, we used the accumulation rate of SP rather than the absoluteamount of SP. Furthermore, $alpha$ is postulated as the total affinityof DG to both the transporter and phosphorylation system relativeto that of glucose. Thus the contamination of the signals fromthe metabolites of glucose little affects the determination of $alpha$ .

It is well known that a high [DG] has deteriorating effects on myocardial energy metabolism. As addressed previously (6),we carefully used only the initial part of the NMR data afterswitching glucose to DG in the perfusate to determine the myocardialaccumulation rate of DG. A similar concept is used to measureenzyme activity, although the time span is different. The dataused in the analysis were obtained during the phase when the interventioninduced minimal changes inmetabolism.

It might be possible that LC for FDG is different from that for DG. It has been reported that LC in brain metabolism is notdifferent between FDG and DG. Recently, LC for FDG was reportedto be higher than that for DG in rabbit hearts (11). Nevertheless,the same report observed that insulin decreased LC for FDG andDG in a parallel manner (11). Thus the absolute value of LCmay be different between LC and FDG, but our conclusion aboutthe effect of insulin on LC is consistent for both FDG andDG.

In conclusion, the lumped constant can be evaluated by methods other than those using radiolabeled tracers. Our data indicatethat the lumped constant is smaller in insulin-stimulated heartsor in stunned myocardium compared with the control condition.These results suggest that the lumped constant is changed dependingon the metabolic state, and careful quantification is necessaryto estimate of myocardial glucose utilization using FDG PET whenmyocardial glucose uptake isenhanced.

	ACKNOWLEDGEMENTS

This work was partly supported by Grants-in-Aid for Scientific Research (no. B 08457208 and University-to-University CooperativeResearch no. 07045051 to H. Kusuoka) of the Ministry of Education,Science and Culture ofJapan.

	FOOTNOTES

The costs of publication of this article were defrayed in part by the payment of page charges. The article must thereforebe hereby marked "advertisement" in accordance with 18 U.S.C.§1734 solely to indicate thisfact.

Address for reprint requests: H. Kusuoka, Inst. for Clinical Research, Osaka National Hosp. 2-1-14 Hoenzaka, Chuo Osaka 540-0006 Japan (E-mail: kusuoka{at}onh.go.jp).

Received 4 May 1998; accepted in final form 10 September 1998.

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