(Received for publication, February 13, 1997, and in revised form, March 11, 1997)
From the Institute of General Pathology, University
of Siena, 53100 Siena, Italy and the ¶ Department of Obstetrics
and Gynaecology, Ninewells Hospital and Medical School, University of
Dundee, Dundee, DD1 9SY, Scotland
Glucose-6-phosphate transport was investigated in rat or human liver microsomal vesicles using rapid filtration and light-scattering methods. Upon addition of glucose-6-phosphate, rat liver microsomes accumulated the radioactive tracer, reaching a steady-state level of uptake. In this phase, the majority of the accumulated tracer was glucose, but a significant intraluminal glucose-6-phosphate pool could also be observed. The extent of the intravesicular glucose pool was proportional with glucose-6-phosphatase activity. The relative size of the intravesicular glucose-6-phosphate pool (irrespective of the concentration of the extravesicular concentration of added glucose-6-phosphate) expressed as the apparent intravesicular space of the hexose phosphate was inversely dependent on glucose-6-phosphatase activity. The increase of hydrolysis by elevating the extravesicular glucose-6-phosphate concentration or temperature resulted in lower apparent intravesicular glucose-6-phosphate spaces and, thus, in a higher transmembrane gradient of glucose-6-phosphate concentrations. In contrast, inhibition of glucose-6-phosphate hydrolysis by vanadate, inactivation of glucose-6-phosphatase by acidic pH, or genetically determined low or absent glucose-6-phosphatase activity in human hepatic microsomes of patients suffering from glycogen storage disease type 1a led to relatively high intravesicular glucose-6-phosphate levels. Glucose-6-phosphate transport investigated by light-scattering technique resulted in similar traces in control and vanadate-treated rat microsomes as well as in microsomes from human patients with glycogen storage disease type 1a. It is concluded that liver microsomes take up glucose-6-phosphate, constituting a pool directly accessible to intraluminal glucose-6-phosphatase activity. In addition, normal glucose-6-phosphate uptake can take place in the absence of the glucose-6-phosphatase enzyme protein, confirming the existence of separate transport proteins.
Liver plays a major role in regulation of blood glucose levels. In response to stress or low blood glucose levels, it releases glucose for use by other tissues. The terminal step of both glycogenolysis and gluconeogenesis, the two glucose producing pathways, is catalyzed by glucose-6-phosphatase (EC 3.1.3.9) (1). The importance of this enzyme in the regulation of blood glucose levels is clear from the debilitating effects in the absence of enzyme activity in glycogen storage disease (GSD)1 type 1 (2). The enzyme activity was originally recovered with the microsomal subcellular fraction in the 1950s, e.g. de Duve et al. (3), which mainly derives from the endoplasmic reticulum (ER) membranes (4). The latency of its activity, discovered in early studies (5, 6), together with histochemical studies (7) indicated the compartmentation of the enzyme in the ER lumen. Consistent with this, more recent sequence information (8, 9) revealed that mammalian glucose-6-phosphatases contain the carboxyl-terminal two-lysine retention motif by which transmembrane proteins are retained in the ER by retrieval from the Golgi (10, 11). They are also very hydrophobic proteins (12), and a variety of topological studies indicate that the active site of the enzyme is located in the lumen of microsomes (13, 14).
There is no consensus of opinion to date, however, concerning the catalytic mechanism of the enzyme. Presently there are essentially two models to explain it. According to the "translocase-catalytic unit" or "substrate transport" model (15-18), the catalytic site of the glucose-6-phosphatase enzyme, situated inside the lumen of the ER (16), acts in concert with at least three putative ER transport proteins for the substrate glucose-6-phosphate and for the products phosphate and glucose, which have been named T1, T2, and T3 (2, 12, 16, 18), respectively. In the "combined conformational flexibility-substrate transport model" (19-21), there is no T1 transport protein. Instead, glucose-6-phosphatase enzyme traverses the microsomal membrane forming a water-filled space around the catalytic site in the ER membranes. The catalytic site is thus accessible from the cytosol, and the latency would be caused by the interactions between the enzyme and its membrane environment.
The substrate transport model was suggested more than two decades ago after comparing the enzyme kinetic behavior of native microsomes, which exhibit enzyme latency, and that of detergent-disrupted microsomes, i.e. after removal of the microsomal membrane barrier (15, 16). It was subsequently observed that various GSD 1 patients lack the enzyme activity in native but not in disrupted microsomes (2) and, most importantly, that the enzyme activities of these patients behave as predicted by the original substrate transport model (22-24). In other words, certain cases of GSD can be explained assuming the inherited deficiency of the putative transporter T1 (GSD 1b), T2 (GSD 1c), or T3 (GSD 1d) (2). Liver glucose-6-phosphatase enzyme cDNAs have been cloned in humans, rats, and mice (8, 9, 25, 26), and a number of point mutations of the gene have been shown to underlie GSD 1a (27). In contrast, no mutations of this gene have been found in patients with deficiencies of microsomal glucose-6-phosphate transport (28). This indicates that the enzyme protein does not have transport function and that other loci (and proteins) are also needed for glucose-6-phosphate hydrolysis in native (intact) microsomes (2, 12, 16). Very recent evidence also indicates that the human chromosome 17 (which contains the glucose-6-phosphatase enzyme gene) is not the site of the defect in GSD 1b (29). Light-scattering transport experiments showed that liver microsomal vesicles are permeable to glucose-6-phosphate, but not to its isomers mannose-6-phosphate and glucose-1-phosphate (30), which supports a selective ER transport for the substrate of the glucose-6-phosphatase enzyme.
Despite the increasing genetic and other evidence of the existence of T1, there is still controversy. The main recent argument for the nonexistence of a T1 transport protein in the conformational model is based on the putative absence of accumulation of glucose-6-phosphate in liver microsomes incubated with the 14C-labeled hexose phosphate (6, 31). In fact, it was observed that liver microsomes accumulate more 14C than could be explained by the facilitative transport/passive equilibrium of added extravesicular [14C]glucose-6-phosphate, and this was interpreted as a microsomal accumulation of the enzyme product 14C-labeled glucose, assuming that the latter exits the microsomal lumen slowly (6, 31). In other kinetic studies (31, 32), the enzyme activity showed an initial burst phase, which was attributed to a tight coupling between glucose-6-phosphate transport and hydrolysis and thus to an extravesicular substrate pool. In addition, neither glucose-6-phosphate nor glucose uptake and accumulation have been observed in liver microsomes obtained from a GSD 1a patient (33). Very recently, knockout mice for the glucose-6-phosphatase enzyme gene have been produced (34), and it was observed that the addition of [14C]glucose-6-phosphate resulted in lower uptake of 14C in microsomes isolated from livers of knockout mice compared with the control, which was discussed as glucose-6-phosphatase-dependent substrate transport (34).
In contrast to this background, we have investigated the nature of the hepatic microsomal intravesicular pools deriving from the transport of glucose-6-phosphate. To this end, we have measured both [14C]glucose-6-phosphate uptake and [14C]glucose accumulation in rat hepatic microsomal vesicles as well as in liver microsomal preparations derived from two GSD 1a cases. Here we show that glucose-6-phosphate crosses the microsomal membrane and forms an intraluminal metabolically active pool allowing the formation of an intraluminal glucose pool whose extents were directly dependent on glucose-6-phosphatase activity. The present results confirm previous genetic evidence that the glucose-6-phosphatase enzyme is not responsible for endoplasmic reticulum glucose-6-phosphate transport and that a different T1 protein/gene is responsible for the ER transport of glucose-6-phosphate. In addition, the results provide an alternative explanation for kinetic data that were previously considered to support the conformational model.
24 h-fasted male Sprague-Dawley rats (180-230 g) were used. Liver microsomes were prepared as reported (35). Microsomal fractions were resuspended in a buffer (buffer A) containing (in mM): KCl, 100; NaCl, 20; MgCl2, 1; and Mops, 20, pH 7.2. The suspensions were rapidly frozen and maintained under liquid N2 until used. Intactness of microsomal vesicles checked by measuring the latency of mannose-6-phosphatase activity (36) was greater than 90% in all the preparations employed. Microsomal protein concentrations were determined by biuret reaction using bovine serum albumin as a standard. In some experiments, microsomal glucose-6-phosphatase was inactivated by mild acidic treatment according to (37). To measure microsomal water space, microsomes were diluted (10 mg protein/ml) in buffer A containing [3H]H2O (0.2 µCi/ml) or [3H(C)]inulin (0.17 µCi/ml) and centrifuged (100,000 × g, 60 min), and the radioactivity associated with pellets was measured to enable calculation of extravesicular and intravesicular water spaces (38, 39).
Preparation of Human Liver MicrosomesBoth GSD type 1a patients were initially diagnosed by kinetic analysis of the glucose-6-phosphatase system in microsomes isolated from liver biopsy samples. Case 1 had mild symptoms until adulthood, elevated hepatic glycogen levels, abnormally low glucose-6-phosphatase enzyme activity levels (20% of age-matched control levels), and low levels of abnormally sized glucose-6-phosphatase enzyme protein as judged by immunoblot analysis.2 Case 2 had a much more severe form of type 1a GSD with virtually all the signs and symptoms described for the disorder (2), elevated hepatic glycogen levels, virtually no glucose-6-phosphatase enzyme activity (~1% of age-matched control values), and no immunodetectable glucose-6-phosphatase enzyme protein by immunoblot analysis. Portions of liver biopsy samples from the two patients were histologically examined to check for the presence of adenoma or hepatoma cells. The need to do this is illustrated by case 2. Histology demonstrated that a first needle biopsy sample from the patient was partially adenoma and was not used for the present study (or diagnosis). In contrast, a second liver sample was found to contain only (nontransformed) liver cells and thus was used to prepare the microsomes investigated here. Human liver microsomes were prepared in 0.25 M sucrose containing 5 mM Hepes (pH 7.4) by differential centrifugation as described previously (40). The intactness of the two type 1 GSD microsomal preparations, based on the latency of p-nitrophenol UDP-glucuronosyltransferase activity (41), was greater than 90%. Protein concentrations were estimated by the method of Lowry as modified by Peterson (42). The study of the glucose-6-phosphatase system in human liver samples was approved by the Ethics Committee of Tayside Health Board.
Uptake MeasurementsLiver microsomes (1 mg protein/ml) were
incubated in buffer A containing 0.2, 0.5, 1, 5, 10, or 30 mM glucose-6-phosphate plus
D-[14C(U)]glucose-6-phosphate (2-3 µCi/ml)
at 22 °C. At the indicated time intervals, samples (0.1 ml) were
rapidly filtered through cellulose acetate/nitrate filter membranes
(pore size 0.22 µm), and filters were washed with 4 ml of Hepes (20 mM) buffer (pH 7.2) containing 250 mM sucrose
and 0.5 mM 4,4-diisothiocyanostilbene-2,2
-disulfonic acid. This latter compound was added to reduce eventual efflux of
vesicular glucose-6-phosphate during the washing procedure (30). The
time required to execute filtration and washing was 15-20 s.
Filtration of samples of media containing no microsomes, and washing of
filters as above, resulted in negligible amounts of radioactivity
retained by filters. The total 14C associated to microsomes
retained by filters was measured by liquid scintillation counting.
Parallel filters were treated with ZnSO4-Ba(OH)2 to separate [14C]glucose from [14C]glucose-6-phosphate, and labeled glucose-6-phosphate and glucose were recovered, respectively, in the pellet and supernatant, after centrifugation (43). Briefly, washed filters were transferred into tubes containing 0.3 ml of 0.2 M ZnSO4 and were pushed to the bottom. After mixing, 0.6 ml of a saturated solution of Ba(OH)2 was added. Tubes were centrifuged to remove the white precipitate and filters. A 0.45-ml portion of the clear supernatant was used to measure [14C]glucose produced from [14C]glucose-6-phosphate by liquid scintillation spectroscopy. Routinely, the amount of [14C]glucose-6-phosphate was calculated by subtracting [14C]glucose from the total 14C associated to microsomes measured in parallel samples (see above). In preliminary experiments, we verified i) that more than 97% of standard [14C]glucose and of standard [14C]glucose-6-phosphate applied on filters were recovered in the clear supernatant and in the precipitate, respectively, and ii) that direct measurements of precipitated [14C]glucose-6-phosphate (after resuspending barium precipitates and filters with ZnSO4-Ba(OH)2 solutions and centrifuging to remove [14C]glucose carry-over) gave essentially similar results.
In each experiment, alamethicin (0.05 mg/ml) was added to the parallel
incubates to distinguish the intravesicular and the bound radioactivity
(41, 44). The alamethicin-permeabilized microsomes were recovered on
filters and washed as above. More than 95% of the microsomal protein
was retained by filters, indicating that the alamethicin treatment did
not affect the vesicular structure of microsomes as already reported
(41). The alamethicin-permeabilized microsomes retained amounts of
radioactivity 20% of that associated to untreated microsomes.
Intravesicular radioactive compounds were bona fide lost
during the washing procedure since the alamethicin nonreleasable
portion did not further decrease even after extensive washing of
filters (and microsomes). This allowed us to regard the alamethicin
releasable portion of radioactivity as intravesicular.
To unequivocally identify the intraluminal material precipitated with barium as glucose-6-phosphate, some microsomal samples were incubated for 5 min in the presence of (30 mM) glucose-6-phosphate and in the presence or in the absence of alamethicin as described above. Samples (1 mg of protein) were filtered, and, after washing, the filters were treated with perchloric acid (3%, 1 ml). Samples were neutralized with KHCO3, tubes were centrifuged to remove the precipitate and filters, and the glucose-6-phosphate content of the neutralized supernatants was measured enzymatically. To this end, 0.5 ml of the supernatant was mixed with an equal volume of buffer A containing 2 mM NADP+, and NADPH formation was detected fluorimetrically (excitation and emission wavelengths were 360 and 470 nm, respectively) upon the addition of glucose-6-phosphate dehydrogenase (0.7 IU/ml). Pulse additions of standard glucose-6-phosphate (1 to 5 nmol) to the reaction mixture allowed the quantitation of microsomal glucose-6-phosphate.
Where indicated, the microsomal passive equilibration of intra- and extravesicular glucose-6-phosphate was calculated according to the formula: apparent intravesicular glucose-6-phosphate space (µl/mg of protein) = glucose-6-phosphate accumulated by microsomes (nmol/mg of protein)/concentration of added glucose-6-phosphate (nmol/µl) (30, 45).
Assay of Glucose-6-phosphataseGlucose-6-phosphatase activity was measured after 5 min of incubation in buffer A at 22 °C on the basis of D-[14C(U)]glucose production from D-[14C(U)]glucose-6-phosphate according to (43). At high substrate concentrations (30 mM), the enzyme activity was also evaluated by measuring glucose production with a glucose (Trinder) kit (Sigma).
Light Scattering MeasurementsOsmotically induced changes in microsomal vesicle size and shape were monitored at 400 nm at right angles to the incoming light beam using a fluorimeter (Perkin-Elmer model 650-10S) equipped with a temperature-controlled cuvette holder (22 °C) and magnetic stirrer as described elsewhere (30, 45). The mV output signals were acquired at 0.25 s intervals, using MacLabTM hardware (AD Instruments) equipped with Chart Ver. 3.2.5. software.
MaterialsGlucose-6-phosphate (monosodium salt),
mannose-6-phosphate (disodium salt), alamethicin, NADP+,
and 4,4-diisothiocyanostilbene-2,2
-disulfonic acid were obtained from
Sigma. Na3VO4 was from Fisher Science Co.
D-[14C(U)]glucose-6-phosphate (300 mCi/mMol)
was from American Radiolabeled Chemicals Inc., St. Louis, MO.
[3H]H2O (1 mCi/g) and
[3H(C)]inulin (500 mCi/g) were from DuPont NEN, Dreieich,
Germany. Glucose-6-phosphate dehydrogenase (from yeast, 350 IU/ml) was from Boehringer Mannheim, Germany. Cellulose acetate/nitrate filter membranes (pore size 0.22 µm) were from Millipore. All other
chemicals were of analytical grade.
In a first set of experiments,
rat liver microsomal vesicles were incubated in the presence of various
concentrations of glucose-6-phosphate (plus
[14C]glucose-6-phosphate as a tracer). The radioactivity
associated with microsomes was measured in vesicles incubated both in
the presence and absence of the pore-forming antibiotic alamethicin (41, 44) to determine net intravesicular accumulation. Because, in
addition to [14C]glucose-6-phosphate,
[14C]glucose (produced by glucose-6-phosphatase activity)
can contribute to the intravesicular measured radioactivity (as it was
indeed the case, see below), we expressed as "glucose-6-phosphate + glucose" the 14C-radioactivity accumulated (see Fig.
1). Glucose-6-phosphate did not likely undergo major
reactions other than dephosphorylation in our incubation system,
therefore glucose-6-phosphate + glucose concentrations could be
calculated on the basis of the concentrations of glucose-6-phosphate
added. Microsomes rapidly accumulated glucose-6-phosphate + glucose
until a steady-state level was reached over a 2-min period of
incubation (Fig. 1A). The steady-state intraluminal accumulation of glucose-6-phosphate + glucose increased by increasing the extravesicular concentration of glucose-6-phosphate although not in
a linearly proportional fashion (Fig. 1B). Based on the measured intravesicular water space of rat liver microsomes (3.6 ± 1.1 µl/mg protein, mean ± SD, n = 6) the
mM intravesicular concentrations of glucose-6-phosphate + glucose were also calculated (Fig. 1B). Relatively low
extravesicular concentrations (1 mM) of
glucose-6-phosphate resulted in intravesicular steady-state
concentrations of glucose-6-phosphate + glucose higher than those of
the extravesicularly added glucose-6-phosphate (Fig. 1B,
inset; concentrations of added glucose-6-phosphate are indicated by the dotted line). On the other hand, at
glucose-6-phosphate concentrations
5 mM, steady-state
intravesicular concentrations of glucose-6-phosphate + glucose were
lower than the added glucose-6-phosphate concentrations (Fig.
1B).
In theory, intravesicular concentrations of glucose-6-phosphate can
maximally equal the extravesicular ones since no energy, or ion
gradients, were present in the system to allow microsomal inward
transport of glucose-6-phosphate over the passive equilibrium. Therefore, the higher intravesicular concentrations of
glucose-6-phosphate + glucose, in the presence of glucose-6-phosphate
concentrations 1 mM, were logically contributed to by
glucose accumulation. Separate measurements of glucose and
glucose-6-phosphate present in the lumen of microsomal vesicles
revealed that accumulation of glucose was responsible for the apparent
increase in intravesicular concentration of 14C-labeled
compounds over that of extravesicular glucose-6-phosphate. However,
besides the intravesicular glucose pool, a glucose-6-phosphate pool
could also be demonstrated by two different methods. The intravesicular
steady-state glucose-6-phosphate content of the microsomes at 30 mM glucose-6-phosphate concentration was similarly estimated by either the isotopic (10.0 ± 1.6 nmol/mg protein, see
Table I) or the enzymatic (11.9 ± 3.9 nmol/mg
protein, mean ± SD, n = 5) method.
|
Intravesicular glucose-6-phosphate content was dependent on the extravesicular concentration of the hexose phosphate (Table I). To highlight the gradient between extra- and intravesicular glucose-6-phosphate concentrations, the apparent intravesicular glucose-6-phosphate space was also calculated. This value represents the relative intravesicular content of glucose-6-phosphate at any extravesicular concentration of the hexose phosphate investigated. Assuming a complete passive equilibrium between extra- and intravesicular glucose-6-phosphate (and no intraluminal metabolism of the hexose phosphate), this value should be equal to the intravesicular water space. The size of the measured intravesicular glucose-6-phosphate space, however, was smaller than the water space at every glucose-6-phosphate concentration investigated (Table I). Moreover, it was inversely related to glucose-6-phosphatase activity; at higher glucose-6-phosphate concentrations, which resulted in higher hydrolytic activity, the size of the apparent microsomal glucose-6-phosphate space was reduced. On the other hand, the absolute amount of intravesicularly accumulated glucose was directly related to the extravesicular glucose-6-phosphate concentrations and to the consecutive glucose-6-phosphatase activities, while its relative amount, expressed as the percentage of total glucose formed, was almost the same at all three glucose-6-phosphate concentrations applied (Table I).
Effect of Glucose-6-phosphatase Activity on the Intravesicular Glucose-6-phosphate PoolOur observations suggested that the
sizes of the intravesicular glucose-6-phosphate and glucose pools were
governed directly by glucose-6-phosphatase activity. To prove this
hypothesis, intravesicular glucose-6-phosphate and glucose contents
were determined when glucose-6-phosphatase was inactivated by a mild
acidic pretreatment of microsomes (16, 37), or inhibited by the
competitive inhibitor vanadate (46). At low glucose-6-phosphate
concentration (0.2 mM), these treatments slightly
influenced the intravesicular glucose-6-phosphate levels (data not
shown). At high (30 mM) glucose-6-phosphate concentration, the significant reduction of glucose-6-phosphatase activity was accompanied with an apparent increase of intraluminal
glucose-6-phosphate space in both treatments (Fig.
2A). Similarly, microsomes of two GSD 1a
patients showed very low (case 1), or virtually no (case 2), hydrolytic
activity and an apparently high intraluminal glucose-6-phosphate space.
In contrast, the increase of glucose-6-phosphatase activity by the
elevation of the incubation temperature to 37 °C resulted in the
reduction of intravesicular glucose-6-phosphate space. The apparent
intravesicular glucose-6-phosphate space always showed an inverse
relationship with glucose-6-phosphatase activity independently of the
experimental conditions (Fig. 2A). The accumulation of intravesicular glucose increased as a function of glucose-6-phosphatase activity independently of the experimental conditions (Fig.
2B).
Effect of Glucose-6-phosphatase Activity on Microsomal Glucose-6-phosphate Transport
On the basis of the measurement of
glucose-6-phosphate uptake in microsomes from glucose-6-phosphatase
knockout mice, it has been suggested that the presence of the
hydrolytic activity is necessary to allow efficient glucose-6-phosphate
transport (34). Although the experiments above did not seem to support
this suggestion, we have investigated the transport of
glucose-6-phosphate in microsomes with low glucose-6-phosphatase
activity (in the presence of vanadate and in samples from GSD 1a
patients) using the light-scattering method (30, 45). The osmotic
behavior of microsomes treated with vanadate (Fig.
3B) and genetically lacking
glucose-6-phosphatase enzyme (human liver microsomes GSD 1a, case
"2"; Fig. 3C) was similar to the one observed in control
rat liver microsomes (Fig. 3A). These observations clearly
indicate that microsomal glucose-6-phosphate uptake was not dependent
on glucose-6-phosphatase activity. These results are also consistent
with those obtained in rapid filtration experiments (Fig. 2), which
further validates the use of the light-scattering technique for
assaying glucose-6-phosphate microsomal transport.
Although several observations indicate the transport of glucose-6-phosphate through liver microsomal membrane (30, 47), the existence of an intraluminal glucose-6-phosphate functional pool has not been proven. Moreover, recent findings (20-21) suggest that after the addition of glucose-6-phosphate to microsomal vesicles, they accumulate mainly glucose rather than glucose-6-phosphate. It is also disputed whether glucose-6-phosphatase uses an intra- or an extravesicular substrate pool.
This study shows that liver microsomes have an intraluminal pool of glucose-6-phosphate at the steady-state phase of glucose-6-phosphate uptake although, according to previous observations (20, 21, 31), the majority of intravesicular glucose-6-phosphate has been converted to glucose. In native untreated rat liver microsomes, the size of the glucose-6-phosphate pool is directly dependent on the extravesicular glucose-6-phosphate concentration, while the apparent intravesicular glucose-6-phosphate space (i.e. the relative size of the pool, irrespective of the extravesicular concentrations of glucose-6-phosphate) is in an inverse relation with glucose-6-phosphatase activity (Table I). In addition, increasing glucose-6-phosphatase hydrolytic activity by elevating the temperature results in a reduction of the apparent intravesicular glucose-6-phosphate space while the decrease in enzyme activity by pH inactivation, by the competitive inhibitor vanadate and by genetic reasons, results in the highest intravesicular apparent spaces of glucose-6-phosphate. The inverse correlation between the apparent intravesicular space of glucose-6-phosphate and the enzyme activity, independently of substrate concentration, and of the treatment and source of microsomes (Fig. 2A) indicate that the catalytic unit directly acts on intravesicular glucose-6-phosphate.
The presence of a glucose-6-phosphatase-accessible intraluminal glucose-6-phosphate pool strongly supports the substrate transport model of the glucose-6-phosphatase system. In theory, however, these results could be explained in accordance with the modified version of the combined conformational flexibility-substrate transport model, assuming that the enzyme traverses the membrane and forms a glucose-6-phosphate channel at the same time. The active enzyme would consume glucose-6-phosphate and release glucose into the vesicular space while, in the relative or absolute absence of hydrolytic activity, the majority of glucose-6-phosphate molecules would cross the membrane without being hydrolyzed. This possibility, however, can be excluded because of the following points. (i) Glucose-6-phosphate transport is detectable even in the absence of the enzyme protein (i.e. in GSD 1a case "2" in which the immunodetectable liver glucose-6-phosphatase enzyme was absent). (ii) Family studies in GSD subtype 1b (29) indicate that the genes associated with glucose-6-phosphate transport are not located on human chromosome 17, the location of the glucose-6-phosphatase enzyme gene. (iii) No mutations were found in the glucose-6-phosphatase enzyme gene in GSD 1b (28). (iv) In liver microsomes from a patient with GSD subtype 1b, glucose-6-phosphate transport could not be detected by light-scattering technique despite the presence of the enzyme.3
The uptake of glucose-6-phosphate into microsomes isolated from the two GSD 1a patients is consistent with uptake into microsomes from one GSD 1a patient reported previously (48), but it is in contrast to the recent report of no microsomal uptake in one GSD 1a case (33). In the latter study, the liver specimen (and microsomes) was derived from a GSD 1a patient whose liver was transplanted because of an enlarging mass. Frequently, GSD 1a patients need liver transplants because their livers contain large masses (or hepatomas), which are also surrounded by parenchyma containing multiple small foci of adenoma cells. Liver transformed cells, however, do not usually express the glucose-6-phosphatase system, and no histological analysis was presented (33), thus it is difficult to unequivocally interpret the lack of uptake reported in (33).
In microsomes from glucose-6-phosphatase knockout mice, the radioactive tracer accumulation upon the addition of glucose-6-phosphate was lower than in controls. It has, therefore, been suggested that the presence of the enzyme somehow stimulates glucose-6-phosphate transport (34). In their control mice (34), the majority of the accumulated 14C was probably glucose (20, 21), and the apparently lower uptake of [14C]glucose-6-phosphate in knockout mice is likely to be due to the absence of lumenal [14C]glucose formation (and accumulation). In our experiments, glucose-6-phosphate transport registered by the light scattering method shows similar features in control, glucose-6-phosphatase enzyme deficient, or vanadate-treated microsomes (Fig. 3). Therefore, it is very unlikely that the glucose-6-phosphatase enzyme is, or directly cooperates with, the transporter.
The continuous consumption of the intravesicular glucose-6-phosphate pool by glucose-6-phosphatase means that the intravesicular concentration of glucose-6-phosphate must always be lower than the extravesicular one. The highest apparent glucose-6-phosphate space in native untreated rat liver microsomes was ~1.6 µl/mg of protein at 0.2 mM extravesicular glucose-6-phosphate concentration. This value is probably close to the maximal size of the glucose-6-phosphate-accessible microsomal space since similar spaces can be observed in vesicles with little or no enzyme activity, i.e. in the GSD type 1a human liver microsomes, and in rat liver microsomes pre-incubated at low pH (see Fig. 2). We have previously obtained comparable values for glucose-6-phosphate-accessible microsomal space by diluting vanadate-treated, [14C]glucose-6-phosphate-preloaded rat liver microsomes (30). Thus, the glucose-6-phosphate-accessible space appears to constitute only a fraction of the total water space of microsomes, which can theoretically be explained by a steady-state partial equilibration of glucose-6-phosphate across the microsomal membrane or/and by uneven distribution of the glucose-6-phosphatase system in microsomal vesicles. The latter possibility is not entirely consistent, however, with cytochemical ultrastructural evidence for a widespread distribution of glucose-6-phosphatase enzyme activity within liver endoplasmic reticulum in situ (7). In addition, liver microsomal preparations may well contain a (small) proportion of vesicles from membranes other than endoplasmic reticulum and lacking glucose-6-phosphate transporters. Several undetermined factors may also contribute to the uncompleted equilibration of extravesicular glucose-6-phosphate with microsomal intralumenal space, e.g. the presence of fixed negative internal charges (45) and/or the preferential transport of one of the dissociated forms of glucose-6-phosphate (16).
A transmembrane gradient of glucose-6-phosphate is present at all extravesicular glucose-6-phosphate concentrations studied, which is consistent with the phenomenon of latency exhibited by glucose-6-phosphatase activity; the lower intravesicular concentration of glucose-6-phosphate can account for the higher Km value of glucose-6-phosphatase in native microsomal vesicles (15). The reduction of vesicular glucose-6-phosphate space at higher extravesicular glucose-6-phosphate concentration means that the hydrolytic capacity is higher than that of the transport, in accord with the rate-limiting property of the latter. The intravesicular accumulation of glucose shows that, in the pre-steady-state phase, the velocity of glucose-6-phosphate hydrolysis surpasses that of the glucose transport. The relative accumulation of glucose (intravesicular glucose as percent of total glucose, Table I) does not increase when glucose-6-phosphatase activity and the consecutive intravesicular glucose content are increased. This finding is consistent with a low rate of glucose efflux from microsomes preloaded with glucose derived from intravesicular glucose-6-phosphate hydrolysis4 and with the previous observation for a slow release of radioactivity (presumably mostly labeled glucose) after pre-equilibration of liver microsomes with labeled glucose-6-phosphate (20).
Collectively, our results further validate the substrate transport model of the glucose-6-phosphatase system. The existence of the intravesicular glucose-6-phosphate and glucose pools upon addition of glucose-6-phosphate, the fact that the content of both pools is governed by glucose-6-phosphatase activity, and the gradient between the extra- and intravesicular concentrations of glucose-6-phosphate are consistent with an intraluminal enzyme activity supported by transporters for substrate and products.