Department of Medicine, University of Pittsburgh School of Medicine, Pittsburgh, Pennsylvania
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ABSTRACT |
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INTRODUCTION |
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The hormonal regulation of hexokinase II expression suggests a specific role in glucose metabolism. Binding of hexokinase isozymes to mitochondria and other subcellular structures has been considered as a potential mechanism for the regulation of enzyme activity and is therefore potentially important for the regulation of glucose metabolism (3,1415161718). Most studies on hexokinase in skeletal muscle have been performed using rodent models. Studies of hexokinase isozymes in human skeletal muscle are limited. The results that are available suggest that insulin can regulate hexokinase II expression (19,20). A recent study addressed hexokinase isozyme cellular distribution and found a high level of hexokinase II binding to mitochondria (21). However, these results are controversial (21,22). The estimation of activity of hexokinase isozymes in human skeletal muscle was questioned by Wilson (23). His studies indicated that methods previously used to estimate the content of hexokinase I and II isozymes in muscle (21,24), namely thermal inactivation and electrophoresis, may not be reliable (23) for distinguishing hexokinase I and II isozymes, especially in relation to mitochondrial binding. Therefore, the goal of the current study was to examine the cellular distribution and activities of hexokinase I and II in human skeletal muscle in healthy volunteers. To accomplish this aim, we explored the application of ion-exchange chromatography, thermal inactivation, and a highly sensitive high-performance liquid chromatography (HPLC)-based hexokinase assay for measuring the activity and distribution of hexokinase isozymes among subcellular fractions in human skeletal muscle.
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RESEARCH DESIGN AND METHODS |
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Sampling.
Volunteers (11 healthy lean individuals: 5 men and 6 women; BMI 23.5 ± 0.5 kg/m2) were recruited and medically screened. Written consent was obtained.
Tissue material from the vastus lateralis portion of quadriceps femoris muscle was obtained after an overnight fast using the percutaneous biopsy technique of Bergstrom (25). Samples were frozen in liquid nitrogen and kept at -75°C before analysis.
Preparation of homogenate and separation of soluble and particulate hexokinase
Preparation of homogenate.
The homogenization medium contained 100 mmol/l mannitol, 80 mmol/l potassium gluconate, 20 mmol/l KF, 10 mmol/l glucose, 1 mmol/l MgCl2, 5.0 mg/ml bovine serum albumin (BSA), 100 µmol/l deferoxamine mesylate, 0.2 mmol/l EGTA, 10 mmol/l histidine, 20 µmol/l leupeptin, 100 µmol/l phenylmethylsulfonyl fluoride, and 10 mmol/l triethanolamine (TEA)3-[N-morpholino]-2-hydroxypropanesulfonic acid (MOPSO) buffer, pH 7.6, at 21°C. We used potassium gluconate to keep the K+ concentration in the homogenization and the reaction media close to physiological levels and to avoid high concentrations of chloride because these things can affect hexokinase binding (26).
Samples of tissue (10 mg) were incubated for 5 min at 4°C in 400 µl homogenization medium to wash out any blood. The washes were mixed with an equal volume of 50% glycerol in albumin-free homogenization medium and saved for subsequent analysis. The tissue was then transferred into 400 µl fresh homogenization medium and homogenized for 10 s at full speed (
25,000 RPM) by a Polytron 1200CL handheld homogenizer with a 5-mm shaft. For optimal results, the piece of tissue was placed directly into the homogenizer tip, and the tip was washed by running for 23 s in 400 µl albumin-free homogenization medium. The homogenate and the wash were combined.
Separation of soluble and particulate hexokinase.
The homogenate, without delay, was centrifuged for 20 min at 4°C at 22,000 RPM (45,000g) in a Heraeus Stratos Biofuge (Hanau, Germany). The supernatant was mixed with an equal volume of 50% glycerol in an albumin-free homogenization medium, separated into 200-µl aliquots, and saved for subsequent analysis. The pellet was suspended in 500 µl storage medium (homogenization medium with 0.1 mg/ml BSA, 20 µmol/l leupeptin, and 25% glycerol). Samples were kept at -80°C before estimation of enzyme activities.
Unmasking of enzyme activities in the particulate fraction and preparation of samples for thermal inactivation and chromatography.
To eliminate latency in enzyme activities, we used procedures based on the destruction of the myofibrillar matrix by 0.6 mol/l KCl (2,27). To an aliquot of the particulate fraction suspended in 25% buffered glycerol, 4 mol/l KCl solution was added to a final concentration 0.60 mol/l. The detergent Triton X-100 (0.5%) and diethylenetriaminepentaacetic acid (DTPA) (2 mmol/l) were added to samples along with KCl to facilitate penetration of KCl into muscle fiber fragments and to solubilize cell membranes. The mixture was sonicated at 4°C under nitrogen in the horn probe of a Torbeo Ultrasonic cell disrupter (Cole-Parmer Instrument, Vernon Hills, IL) at an output of 17 W for 5 min, kept on ice for 1 h, and then sonicated again for 5 min. The sonicated suspension was centrifuged at 45,000g for 20 min in a Heraeus Stratos Biofuge. The pellet was discarded, and the supernatant, containing >90% of total hexokinase activity, was saved for subsequent analysis. This treatment increased the activity of hexokinase by two to three times in the particulate fraction but did not affect the activity of hexokinase in the soluble fraction. For experiments on thermal inactivation and chromatography, the samples were subjected to gel filtration. An aliquot of extract from the sonicated particulate fraction (100200 µl) or an aliquot of the soluble fraction (400 µl) was mixed with 100 or 200 µl of H2O, respectively. The mixture was applied to a G-25 column 0.7 x 3 cm (bed volume, 3 ml) equilibrated with 10 mmol/l imidazole buffer (pH 7.1) containing 15% glycerol, 20 mmol/l KCl, 3 mmol/l KF, 0.1 mmol/l DTPA, 0.1 mmol/l deferoxamine, 5 mmol/l glucose, 1 mg/ml Triton X-100, and 4 mmol/l DTT (buffer A). The column was eluted by buffer A. Three 1-ml fractions were collected. The second fraction contained 90% of applied hexokinase activity and was used in experiments on thermal inactivation and for separation of hexokinase isozymes by ion-exchange chromatography.
Separation of hexokinase isozymes by ion-exchange chromatography.
The aliquot obtained by gel filtration was applied on a DEAE-Trisacryl or a DEAE-Agarose column (0.7 x 15 cm, 6-ml bed volume) or on a Mono-Q HR 5/5 (1-ml bed volume) column (Pharmacia, Uppsala, Sweden) that had been equilibrated with buffer A (10 mmol/l imidazole buffer [pH 7.1] containing 15% glycerol, 20 mmol/l KCl, 3 mmol/l KF, 0.1 mmol/l DTPA, 0.1 mmol/l deferoxamine, 5 mmol/l glucose, 1 mg/ml Triton X-100, and 4 mmol/l DTT) or buffer B (10 mmol/l K-phosphate buffer [pH 7.1] containing 15% glycerol, 5 mmol/l EDTA-Na4, 5 mmol/l glucose, 1 mg/ml Triton X-100, and 4 mmol/l DTT) to a final pH of 7.1. Columns were washed by 37 ml of buffer and then eluted with 25 ml of a linear gradient of KCl from 20 to 520 mmol/l (buffer A) or from 0 to 500 mmol/l (buffer B) at a flow rate of 0.250.5 ml/min. The gradient was formed using a fast protein, peptide, and polynucleotide liquid chromatography (FPLC) system equipped with two P-500 pumps, a LCC-500 controller, and a FRAC-100 fraction collector (Pharmacia). Fractions (0.5 ml) were collected starting from the time the sample was applied.
Enzyme assays
Hexokinase.
Activity of hexokinase was determined by HPLC detection of NADPH generated in a coupled enzymatic reaction with Glc-6-P DH. A fluorescence detector at an excitation of 340 nm and an emission of 460 nm monitored fluorescence of NADPH in eluates. The reaction medium contained 100 mmol/l potassium gluconate, 50 mmol/l mannitol, 10 mmol/l glucose, 5 mmol/l ATP, 10 mmol/l phosphocreatine, 10 mmol/l MgCl2, 0.2 mmol/l EGTA, 0.1 mmol/l deferoxamine, 10 mmol/l 3-[(3-cholamidopropyl)-dimethylammonio]-1-propanesulfonate (CHAPS), 0.2 mg/ml BSA, 0.5 mmol/l NADP, 0.1 U/ml Glc-6-P DH, 0.1 U/ml CrK, and 10 mmol/l TEA-MOPSO (pH 7.6 at 21°C). Aliquots of the soluble fraction or extract from the sonicated particulate fraction (10 µl) were combined with 190 µl of the diluent mixture (100 mmol/l potassium gluconate, 50 mmol/l mannitol, 0.2 mmol/l EGTA, 0.1 mmol/l deferoxamine, and 10 mmol/l TEA-MOPSO, pH 7.6). For analysis of chromatographic fractions, aliquots of chromatographic fractions (10 µl) were combined with 40 µl of the diluent mixture. Diluted samples were kept on ice before assay. The reaction was started by adding 50 µl diluted sample to 50 µl reaction mixture and was incubated at 30°C for 40 min. For a blank test, the diluted samples were heated at 65°C for 5 min before mixing with reagents. The reaction was terminated by the addition of 120 µl of 10 mmol/l hydrazine plus 30 mmol/l 2-amino-2-methyl-1-propanol in methanol. Samples were kept at 80°C before HPLC analysis. Freezing the samples facilitated aggregation of denaturated protein. Thawed samples were centrifuged at 45,000g for 5 min in a Heraeus Stratos Biofuge. Aliquots of supernatant (10 µl) were injected onto a C-18 reverse-phase column (Hewlett Packard Hypersil, 5 µm, 100 x 4.6 mm). The column was eluted by a mobile phase composed of 0.2 mol/l KH2PO4 (pH 6.0), 2 mmol/l tetrabutylammonium-OH as an ion-paring reagent, and 14% methanol. The flow rate was 1 ml/min. A Shimadzu LC-100AT vp HPLC equipped with a fluorescence detector (model RF-10Axl) and an autosampler (model SIL-10AD vp) were used. In experiments on hexokinase latency, a Waters HPLC system (Shimadzu, Kyoto, Japan) equipped with an ultraviolet detector was used (Fig. 1). Chromatograms were processed and stored in digital form with Class-VP software. A calibration curve was obtained by plotting the peak areas against amounts of NADPH (Fig. 2B).
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CrK.
Activity of CrK was measured at 30°C by spectrophotometric monitoring of the generation of NADPH at 340 nm in a coupled enzymatic reaction (hexokinase/Glc-6-P DH) (28). The reaction was initiated with the addition of 25 mmol/l phosphocreatine to 2.5 ml of reaction mixture composed of 100 mmol/l potassium gluconate, 10 mmol/l Mg-acetate, 1 mmol/l ADP, 0.05 mmol/l P1,P5-di(adenosine-5')pentaphosphate, 0.1 mmol/l deferoxamine, 0.2 mmol/l EGTA, 2 mmol/l DTT, 0.2 mg/ml BSA, 2.5 mmol/l glucose, 1 mmol/l NADP, 3 U/ml yeast hexokinase, 2 U/ml Glc-6-P DH, and 25 mmol/l imidazole-acetate buffer (pH 6.8) after a 2-min preincubation with the sample (2 µl of the soluble fraction or 10 µl of the extract from the particulate fraction).
Phosphoglucose isomerase.
Activity of phosphoglucose isomerase (PGI) was measured at 30°C with fructose-6-phosphate as the substrate (reverse reaction) (29). The generation of glucose-6-phosphate was measured by spectrophotometric monitoring of the reduction of NADP at 340 nm in the presence of Glc-6-P DH. The reaction was initiated with the addition of 5 mmol/l fructose-6-phosphate to 2.5 ml reaction mixture, the latter composed of 100 mmol/l potassium gluconate, 50 mmol/l mannitol, 0.2 mmol/l EGTA, 0.1 mmol/l deferoxamine, 0.5 mg/ml BSA, 1 mmol/l NADP, 1.0 U/ml Glc-6-P DH, and 10 mmol/l TEA-MOPSO (pH 8.0 at 21°C) after a 1-min preincubation with the sample (50 µl of the soluble fraction or the extract from the particulate fraction).
Statistics.
All enzyme activities were run in triplicate. The mean and SD are presented in the tables and figures. For all 11 biopsies, specific hexokinase activity was measured twice, before and after gel filtration, in the thermal inactivation assay. These data are shown in Table 1, Table 2, and Fig. 3. The estimated hexokinase activities from both measurements were very close (±5%). The chromatograms were used to calculate total hexokinase activity and the activities of hexokinase isozymes (Table 2) and were based on data from three biopsies.
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RESULTS |
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We use a high concentration of methanol (60%, vol/vol) to denature enzymes and stop the reaction. Then, 10 mmol/l hydrazine was added to the methanol to destroy NADP after termination of the reaction (30), and 30 mmol/l 2-amino-2-methyl-1-propanol was added to protect generated NADPH from destruction by hydrazine and to provide alkaline conditions that stabilize NADPH (30). During an HPLC analysis of 70 samples taking 8 h, the concentration of NADPH in samples was stable despite the ambient temperature (2125oC) of the sample tray. Also, we did not find a significant difference in peak areas for NADPH standards separated by HPLC at pH 6.0 or pH 7.5 in the mobile phase. We used a mobile phase adjusted to pH 6.0 in most experiments because separation at pH 6.0 provides better peak symmetry. Introduction to the mobile phase of 2 mmol/l ascorbate plus 0.1 mmol/l deferoxamine mesylate to prevent possible oxidation of reduced pyridine nucleotides during separation did not affect peak area of NADPH.
Proportionality of hexokinase reaction with time and amount of sample.
It was found that except for an initial short lag period (90 s), the hexokinase reaction is absolutely linear for at least 50 min of incubation. To reduce the possible error due to an initial lag period, a time count for a 40-min reaction was started after a 30-s warm-up of the reaction tube in a water bath.
To prevent possible interference by sample components in the hexokinase assay, samples used in the reaction mixture were diluted to the limits imposed by the sensitivity of the assay. In experiments on hexokinase activity in homogenate fractions, it was found that velocity of the reaction depends, in a linear manner, on the final tissue dilution in the reaction mixture across a range from 1:2,000 to 1:5,000. In experiments on hexokinase activity in chromatographic fractions, it was found that velocity of the reaction depends linearly on the volume of the fraction aliquot that is added to the reaction mixture, in a range from 5 to 25 µl.
Total, soluble, and particulate-bound hexokinase activity of human skeletal muscle homogenate
The latency of hexokinase activity.
We compared the effect of 0.6 mol/l KCl on hexokinase activity of whole muscle homogenate and on hexokinase activity of soluble and particulate fractions. Data on the effect of 0.6 mol/l KCl on hexokinase activity are presented in Fig. 1.
As shown in Fig. 1, addition of 0.6 mol/l KCl to samples of human skeletal muscle homogenate and a subsequent triple cycle of freezing and thawing with liquid nitrogen and a 30°C water bath increases hexokinase activity of muscle homogenate by 24 fold. The freezing-thawing cycle in the absence of KCl, but in the presence of the detergent CHAPS, did not significantly affect hexokinase activity. Treatment of the particulate fraction with 0.6 mol/l KCl increased hexokinase activity by severalfold (Fig. 1). The increase of homogenate hexokinase activity by KCl that was observed was due to this effect on the particulate fraction because KCl did not affect hexokinase activity in the soluble fraction.
Distribution of hexokinase activity between soluble and particulate fractions.
We compared the distribution of total hexokinase activity between soluble and particulate fractions in skeletal muscle from 11 healthy lean research volunteers. The results are shown in Fig. 3. Sonication was used in the presence of KCl/Triton X-100 to convert hexokinase activity in the particulate fraction to a soluble form. Hexokinase activity was 2.78 ± 0.6 U/g wet wt tissue in the particulate fraction and 0.31 ± 0.1 U/g wet wt tissue in the soluble fraction.
To estimate the amount of hexokinase in the particulate fraction that is bound to subcellular structures versus the amount that is mechanically trapped within the myofibrillar matrix, we compared the distribution of hexokinase activity between soluble and particular fractions with the distribution of the activity of CrK and PGI. CrK has some affinity to myofibrils and mitochondria (32,33), whereas PGI is considered as a truly cytosolic enzyme (34). For correct estimation of hexokinase, CrK and PGI enzyme activities were measured not only in the soluble and particulate fractions, but also in the solution that was left after brief washing of tissue samples to remove any blood. The results of these experiments are presented in Fig. 3. As can be seen in Fig. 3, the incubation of a 10-mg piece of tissue for 5 min on ice resulted in the release of 30% of CrK,
30% of PGI, and only traces of hexokinase activities. The different compartmentalization of hexokinase and the other two enzymes can be seen from the distribution of activities between the soluble and particulate fractions. The soluble fraction contains >90% of CrK and PGI and only 10% of total hexokinase activity (Fig. 3). From these results, we estimate that not more than 10% of skeletal muscle hexokinase is mechanically trapped within the myofibrillar matrix. Therefore, the great majority of the activity of hexokinase in the particulate fraction can be explained by binding to subcellular structures, most probably to mitochondria, rather than trapping of hexokinase, as has also been established for hexokinase distribution in transformed cell cultures and neuronal tissue (16,18).
In Fig. 3, hexokinase activity is expressed as activity per gram of actual wet weight of tissue. Because of the small weight of tissue specimens used in these experiments, the inclusions of collagen, fat, or blood could significantly affect this estimation of specific hexokinase activity. It has been shown that the activity of CrK in human muscle does not depend on muscle fiber type, sex, or physical training and therefore can be used as a reliable criterion for an estimation of the amount of functionally active muscle fibers in biopsy samples (35). In Table 1, hexokinase activities are expressed per unit of total CrK activity in tissue samples and per gram of tissue wet weight. The wet weight of tissue samples has been normalized on the basis of CrK activity, assuming that the tissue sample with the highest CrK activity indicates the true wet weight of viable muscle fibers (35). As can be seen from Table 1, the total hexokinase activity in human skeletal muscle is 4 U/g wet wt or 0.7 U/mU CrK.
Hexokinase isozymes in the soluble and particulate fractions of human skeletal muscle homogenate
Ion-exchange chromatography.
To estimate the activities of hexokinase isozymes I and II in preparations from human skeletal muscle, we used analytical ion-exchange chromatography on DEAE-Agarose, DEAE-Tricacryl, and Mono Q sorbents. Aliquots of samples obtained from the Sephadex column were applied to ion-exchange columns. These results are presented in Figs. 4A and B. The amount of soluble fraction that was applied to the column was twice the amount of the particulate fraction on the basis of tissue wet weight. Three well-defined peaks (peak S, I, and II) were found in chromatograms of the soluble extract prepared from particulate fractions (Figs. 4A and B). More than 90% of the hexokinase activity applied to the column was recovered as the sum of these three peaks. For chromatograms of the particulate fraction, the activity that was recovered in peak I represented 7080% of total activity. For the soluble fraction, peak I represents
30% of total activity. The comparison of the chromatograms of the particulate and soluble fractions show that most hexokinase activity (8090%) in human muscle resides in the particulate fraction, and this is in agreement with data of direct analysis (Fig. 3).
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These empirically derived conditions for thermal inactivation were then applied to samples from human muscle. Presented in Fig. 6A is a chromatographic profile of hexokinase activity in the particulate fraction from human skeletal muscle before and after heating the chromatographic fractions at 45°C for 45 min. As can be seen in Fig. 6A, heating destroyed peaks S and II but did not affect hexokinase activity in peak I. These data clearly indicate that the particulate fraction from human skeletal muscle contains substantial activity of the hexokinase I isozyme.
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Kinetic analysis of thermal inactivation of hexokinase activity in particulate and soluble fractions from human skeletal muscle.
In preliminary experiments, we found that incubation of particulate fractions from human muscle at 45°C for 60 min destroyed >80% of total hexokinase activity. These results clearly contradicted chromatographic data showing that 80% of total hexokinase activity in the particulate fraction corresponds to thermally stable hexokinase I isozyme. However, after ion-exchange chromatography of the particulate fraction, heating of chromatographic fractions did allow easy differentiation of hexokinase I and hexokinase II isozymes (Fig. 6A). The reason for rapid thermal inactivation of hexokinase I isozyme bound within the particulate fraction probably originates from the destabilizing effects of surrounding lipids or proteins on the structure of bound hexokinase I. The conversion of particulate bound hexokinase to a soluble form by KCl/Triton X-100 extraction, as described in RESEARCH DESIGN AND METHODS, followed by subsequent gel filtration of the extract and then introduction to a thermal inactivation medium including 5 mmol/l CHAPS to reduce protein and lipid interactions, prevents rapid thermal inactivation of hexokinase I at 45°C. Using the described procedure for sample preparation for thermal inactivation, we found only a 25% decline in hexokinase activity in the particulate fraction in the first 5 min (Fig. 7), and the rest of the activity, belonging to hexokinase I isozyme, showed little loss during the next 55 min of heating. The soluble fraction treated by the same methods (excepting sonication) showed an identical two-phase kinetic pattern of thermal inactivation. During the rapid phase of decline of activity, likely corresponding to inactivation of type II isozyme, there was an 60% loss of hexokinase activity in the soluble fraction (Fig. 7).
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DISCUSSION |
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Hexokinase isoforms in human skeletal muscle.
Hexokinase isozymes I and II are expressed in skeletal muscle (3). Rat skeletal muscle contains mostly type II enzyme (1,5), whereas human muscle contains approximately equal amounts of type II and type I isoforms (19,21,40). Our data (based on two approachesion-exchange chromatography and a modified method of thermal inactivation) reveal that in human skeletal muscle, 7075% of hexokinase activity corresponds to the type I isoform, and 2530% of activity belongs to the thermally labile type II isozyme (Table 2). Thermally labile hexokinase II exists in human skeletal muscle as two chromatographically distinct forms: peak S and peak II (Figs. 4 and 6). The same forms were also found in rat skeletal muscle (Fig. 5) but were not found in extracts from rat brain that contain solely the hexokinase I isoform (Fig. 5A). The reason for partial elution of type II hexokinase without retention on the column will require future studies.
Subcellular distribution of hexokinase isoforms in human skeletal muscle.
Hexokinase activity in a particulate cellular fraction, denoting, but not specifically proving mitochondrial binding, has been reported in many mammalian cells cultures and tissues. A relatively small amount of particulate-bound hexokinase was found in rat skeletal muscle (5,34) in contrast to brain tissue, where >80% of hexokinase is found within the particulate fraction (41). As can be seen in Fig. 3 and Table 1, in human skeletal muscle, 90% of total hexokinase activity is bound within the particulate fraction.
Using chromatography and thermal inactivation methods, we found distinct differences in the distribution of hexokinase I and II among the soluble and particulate fractions of human muscle homogenate. As shown in Table 2, 95% of type I hexokinase activity was found in the particulate fraction. Type II hexokinase activity was largely bound to mitochondria (72%), but 28% was found within the cytosolic fraction. Thus, within the particulate fraction, the relative contributions of hexokinase I and II were 81 and 19%, respectively, whereas within the soluble fraction, the relative contributions for hexokinase I and II were 37 and 63%, respectively (Table 2). In the soluble fraction, approximately the same ratio between these two hexokinase isoforms was found, as was previously reported by Vogt et al. (21), in which the thermal inactivation method was used to identify hexokinase I and II. However, our results on hexokinase isoforms in the particulate fraction differ substantially from the data of Vogt et al. (21). They found that 90% of hexokinase in the particulate fraction was due to a thermally labile enzyme and interpreted this thermal lability to represent solely hexokinase II. This difference, from our data, can be explained by differences in the conditions of thermal inactivation used in the two studies. In our preliminary experiments, it was found that most of the hexokinase activity bound in the particulate fraction is highly temperature sensitive. This finding appeared to be in sharp contrast with data from chromatographic analyses that showed that 80% of hexokinase activity, in the particulate fraction, belonged to the thermally stable isoform type I (Table 2). However, after conversion of bound hexokinase to a soluble form and inclusion of the detergent CHAPS in the thermal inactivation mixture to reduce nonspecific lipid-protein and protein-protein interactions, we found excellent agreement between chromatography and thermal inactivation data (Table 2). Our data confirm that heating of untreated particulate fractions cannot be used for the estimation of hexokinase isozyme composition in these fractions, as has been recently pointed out by Wilson (23). However, our data showed that with certain preparation of the sample and proper conditions, thermal inactivation is a reliable and valuable tool for the study of hexokinase isoforms.
There are no definitive data on the localization of bound hexokinase within human muscle. The association of hexokinase with mitochondria was shown in brain tissue and transformed cells (15161718). In mitochondria, hexokinase is bound on the outer mitochondria membrane at contact sites, probably as part of the permeability transition pore, which includes the adenine nucleotide translocator, porin, and other proteins (424344). Porin is considered to be a "hexokinase binding protein" (42) .The proximity of bound hexokinase to the adenine nucleotide translocator establishes a "privileged access" of the enzyme to ATP generated by oxidative phosphorylation. This is one reason for the high level of mitochondria-bound hexokinase in some lines of rapidly growing transformed cells (16). The decreased sensitivity of bound hexokinase to inhibition by glucose-6-phosphate might additionally contribute to a high glycolytic rate in transformed cells (45). The "privileged access" of hexokinase to ATP obviously makes cellular bioenergetics more protected and reliable, and a detailed consideration of the functional significance of this binding of hexokinase is presented in a review by Wilson (3). The high level of hexokinase binding in human skeletal muscle (Fig. 3) in comparison with rat muscle (34) probably reflects better protection of human muscle bioenergetics in the situation of intense physical activity.
The existence and role of nonmitochondrial binding sites for hexokinase have been previously considered in connection with a potential role of hexokinase in mediating the transport of glucose (3,46). It was shown that stimulation of macrophages by phorbol ester activates hexose transport and induces the translocation of hexokinase to the cell surface. Cytochalasin D, an inhibitor of actin microfilament polymerization, prevents phorbol-induced translocation of hexokinase and activation of hexose transport (47). These data indirectly indicate binding of hexokinase with microfilaments. A model for participation of hexokinase in glucose transport ("loose-coupling" model) suggests binding of enzyme in the vicinity of the transporter and that this may decrease exit of glucose from the cell (48). A similar model was used to explain insulin-induced activation of glucose transport in adipocytes (49). A very tight coordination between appearance of insulin sensitivity and expression of hexokinase II and GLUT4 type transporter during ontogenesis of rat skeletal muscle has been reported (50). This coordination can reflect a specific function of the hexokinase II isozyme in muscle insulin-regulated glucose transport.
Hexokinase II has a lesser affinity to mitochondria than hexokinase I (39). Our data show enrichment of the soluble fraction by hexokinase II in comparison with the particulate fraction (Table 2). For that reason, potentially, hexokinase II might be more easily translocated to the vicinity of the glucose transporter in plasma membrane under stimulation by insulin. In addition, the sensitivity of hexokinase II expression to exercise and hormones make hexokinase II an ideal tool for fine-tuning glucose transport in relation to the demands of muscle bioenergetics.
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ACKNOWLEDGMENTS |
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We gratefully acknowledge the participation of our research volunteers and the excellent nursing care provided by the staff of the University of Pittsburgh General Clinical Research Center (5MO1RR00056). Sue Andreko, MS, Janice Beattie, RN, and Carol Kelley, RN, provided expert technical and analytic support.
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FOOTNOTES |
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Received for publication 18 July 2000 and accepted in revised form 20 February 2001.
BSA, bovine serum albumin; CHAPS, 3-[(3-cholamidopropyl)-dimethylammonio]-1-propanesulfonate; CrK, creatine kinase; DTPA, diethylenetriaminepentaacetic acid; DTT, dithiothreitol; FPLC, fast protein, peptide, and polynucleotide liquid chromatography; Glc-6-P DH, glucose-6-phosphate dehydrogenase; HPLC, high-performance liquid chromatography; MOPSO, 3-[N-morpholino]-2-hydroxypropanesulfonic acid; PGI, phosphoglucose isomerase; TEA, triethanolamine.
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REFERENCES |
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