Báo cáo khoa học: Investigation of the effects of sulfonylurea exposure on pancreatic beta cell metabolism

Investigation of the effects of sulfonylurea exposure on pancreatic beta cell metabolism Lorraine Brennan1, Chandralal Hewage1, J. P. G. Malthouse1, Neville H. McClenaghan2, Peter R. Flatt2 and Philip Newsholme1

1 UCD School of Biomolecular and Biomedical Science, UCD Conway Institute, University College Dublin, Belfield, Ireland 2 School of Biomedical Sciences, University of Ulster, Coleraine, UK

Keywords beta cells; metabolism; sulfonylurea

Correspondence L. Brennan, UCD School of Biomolecular and Biomedical Science, UCD Conway Institute, University College Dublin, Belfield, Dublin 4, Ireland Fax: +353 1 2837211 Tel: +353 1 7166781 E-mail: lorraine.brennan@ucd.ie

(Received 9 June 2006, revised 21 Septem- ber 2006, accepted 22 September 2006)

doi:10.1111/j.1742-4658.2006.05513.x

Prolonged exposure of pancreatic beta cells to the sulfonylureas glibenca- mide and tolbutamide induces subsequent desensitization to the actions of these drugs. The precise mechanisms underlying this desensitization remain unknown, prompting the present study, which investigated the impact of prolonged sulfonylurea exposure on glucose and energy metabolism using clonal pancreatic BRIN-BD11 beta cells. Following prolonged exposure to tolbutamide, BRIN-BD11 beta cells were incubated in the presence of [U-13C]glucose, and isotopomer analysis revealed that there was a change in the ratio of flux through pyruvate carboxylase (EC 6.4.1.1) and pyruvate dehydrogenase (EC 1.2.4.1, EC 2.3.1.12, EC 1.8.1.4). Energy status in intact BRIN-BD11 cells was determined using 31P-NMR spectroscopy. Exposure to tolbutamide did not alter the nucleotide triphosphate levels. Collectively, data from the present study demonstrate that prolonged expo- sure of beta cells to tolbutamide results in changes in flux through key enzymes involved in glucose metabolism that, in turn, may impact on glucose-induced insulin secretion.

(SUR1)

subunit of

been suggested that this effect is indirectly dependent on protein kinase C activation [4–6]. Interestingly, a recent study has proposed a mechanism by which sulfonylureas could be transported across the plasma membrane and ultimately interact with intracellular sites regulating insulin exocytosis [7].

Sulfonylureas are a major class of potent insulinotrop- ic drugs that are used extensively in the treatment of patients with type 2 diabetes. These drugs stimulate secretion of insulin from the pancreatic beta cell, primarily by interacting with the high-affinity sulfonyl- urea receptor the beta cell ATP-sensitive potassium ion channel (KATP) channel. Sulfonylurea drugs differ in their specificity for the SUR1 subunit. The interaction with the KATP channel closes the channel, causing membrane depolarization and subsequent opening of voltage-dependent Ca2+ channels [1]. The resulting influx of Ca2+ leads to a rapid rise in intracellular Ca2+ concentration and trig- gers insulin secretion [2,3]. However, a growing body of evidence suggests that the sulfonylureas additionally act in a KATP channel-independent manner by directly interacting with the secretory machinery, and it has

Treatment of patients with sulfonylureas for pro- longed periods (several years) often results in impaired sulfonylurea-induced insulin secretion [8,9]. Although the exact reasons underlying this phenomenon remain unclear, it is now believed that this may be at least partly attributed to desensitization of the pancreatic beta cells to the actions of these drugs. Experiments investigating the effects of chronic exposure of pancre- atic islets and beta cell lines to sulfonylureas in vitro have shown that the desensitization in certain cases limited to subsequent drug-induced insulin is not

Abbreviations KATP channel, ATP-sensitive potassium ion channel; NTP, nucleotide triphosphate; PC, pyruvate carboxylase; PDH, pyruvate dehydrogenase.

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Table 1. Amount of 13C-labelled amino acids present after incuba- tion for 1 h with [1-13C]glucose in the presence and absence of sul- fonylurea drugs. Values are given as nmol per mg protein ± SD (n ¼ 3). All experiments were carried out after a preincubation per- iod of 18 h in the presence or absence of drug.

Control

+ Tolbutamide

+ Glibencamide

[14].

Glu C2 Glu C3 Glu C4 Lactate C3 Alanine C3 Asp C2 Asp C3

5.8 ± 1.0 5.1 ± 1.0 15.8 ± 2.0 7.5 ± 2.6 4.8 ± 1.3 2.4 ± 0.5 2.8 ± 0.2

3.6 ± 0.4* 3.8 ± 0.8 12.5 ± 1.0 6.1 ± 2.8 4.6 ± 1.3 4.0 ± 0.4* 4.9 ± 0.8*

5.7 ± 0.6 6.0 ± 1.1 17.9 ± 3.2 6.2 ± 1.4 4.1 ± 0.6 2.6 ± 1.3 2.6 ± 1.3

*P < 0.05.

[12,13,16],

secretion, but may also affect nutrient-induced insulin secretion [10–13]. The precise mechanisms underlying beta cell drug-induced desensitization remains elusive, and it remains unclear as to whether it results from depletion of insulin stores or functional changes in signalling pathways In a study investigating desensitization due to chronic exposure to glibenca- mide in MIN6 cells, a decrease in the number of fun- ctional KATP channels on the plasma membrane was observed [15]. This would support a homologous desensitization theory, where the primary cause of the desensitization is due to the occupancy of receptor sites and subsequent modification of the downstream pathways [14]. However, other studies have demon- strated that prolonged treatment with sulfonylurea drugs affects the subsequent secretory response to indicating the presence of other stimuli heterogeneous desensitization.

enrichments of

significantly different

only

in

remaining was

Acute stimulation of insulin secretion by glucose involves metabolism via oxidative and anaplerotic pathways involving pyruvate dehydrogenase (PDH; EC 1.2.4.1, EC 2.3.1.12, EC 1.8.1.4) and pyruvate carboxylase (PC; EC 6.4.1.1) [17–19]. The resultant increase in ATP concentration closes the KATP chan- nels, resulting in membrane depolarization, opening of the voltage-dependent Ca2+ channels, Ca2+ influx, and a subsequent increase in cytosolic Ca2+ ([Ca2+]c) which in turn triggers insulin secretion. Additionally, the influx of Ca2+ results in an uptake of Ca2+ by the mitochondria, which may activate mitochondrial meta- bolism and result in further increases in ATP concen- tration [20–22]. The present study investigated the effects of prolonged exposure to sulfonylurea drugs on beta cell metabolism using a combination of different NMR techniques, and utilizing the well-characterized clonal glucose-responsive pancreatic beta cell line, BRIN-BD11 [23,24].

tolbutamide

Results

position C4 (Table 1). In the case of tolbutamide pre- treatment, there was a general trend for decreased labelling of glutamate in positions C2 and C3, but the changes were significant only for the C2 position. The total 13C concentration of alanine and lactate labelled at position C3 did not change significantly. However, in the presence of tolbutamide, the total amount of 13C label present in aspartate C2 and C3 increased significantly. The percentage the glutamate peaks in the presence and absence of the drugs are reported in Table 2. No significant changes were observed for glutamate C3 and C4. In the presence of tolbutamide, there was a decrease in the percentage enrichment for glutamate C2. The amount of glucose remaining in the medium was measured in the presence and absence of drugs, and was found to be the presence of glibencamide; under control conditions, the amount 19.5 ± 1.6 lmolÆmg)1 glucose of protein, whereas in the presence of glibencamide, the concentration was 14.3 ± 0.9 lmolÆmg)1 protein (P < 0.005). The concentration of glucose remaining exposure was in the medium after 17.9 ± 2.1 lmolÆmg)1 protein. The insulin released into the medium at the end of a 1 h incubation period following the preculture with and without the drugs

Metabolism of [1-13C]glucose in the presence and absence of sulfonylurea(s)

Table 2. Percentage enrichment in the glutamate carbons following incubation for 1 h with [1-13C]glucose in the presence and absence of sulfonylurea drugs. Values are expressed as a percentage ± SD (n ¼ 3). All experiments were carried out after a preincubation period of 18 h in the presence or absence of drug.

Control

+ Tolbutamide

+ Glibencamide

Glu C2 Glu C3 Glu C4

8.4 ± 0.6 7.4 ± 1.6 22.8 ± 1.3

6.6 ± 0.5* 7.0 ± 2.3 23.0 ± 3.0

8.3 ± 0.6 8.7 ± 1.2 26.0 ± 1.6

*P < 0.05.

Following 18 h of prior culture in the presence of tol- butamide or glibencamide, the cells were incubated for 1 h in the presence of [1-13C]glucose with or without the sulfonylurea drug. The main metabolites produced included glutamate labelled at positions C2, C3 and C4, lactate and alanine labelled at position C3, and aspartate labelled at positions C2 and C3. Comparison of the label distribution between the different treat- ments indicated that there was no significant change in the total concentration of glutamate labelled at

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7

6

5

*

*

4

e s a e l e r n

3

Table 3. Ratio of flux through pyruvate carboxylase (PC) and pyru- vate dehydrogenase (PDH) calculated from C2 and C4 resonances of glutamate in the presence and absence of a sulfonylurea drug. For all experiments, cells were incubated in the presence of [U-13C]glucose for 2 h following 18 h of prior culture in the presence or absence of the drug. Values are expressed as averages ± SD.

i l

] 1 – ) n i e t o r p g m

( · l

2

u s n

I

Condition

PC ⁄ PDH

1

o m p [

0

control

tol

glib

0.34 ± 0.04 0.24 ± 0.02* 0.30 ± 0.01

Control (n ¼ 3) Tolbutamide (n ¼ 3) Glibencamide (n ¼ 2)

*P < 0.05.

Fig. 1. Effects of culture (18 h) with 100 lM tolbutamide (Tol) or 1 lM glibencamide (Glib) on glucose-induced insulin release over a subsequent 1 h incubation period. Values are mean ± SD. Control incubation in the to culture and subsequent conditions refer absence of a drug. *P < 0.05.

was measured. Preincubation in the presence of the insulin significantly reduced the amount of drugs released (Fig. 1).

Table 4. Percentage of acetyl-CoA derived from [U-13C]glucose fol- lowing incubation in the presence and absence of a sulfonylurea drug. Values are expressed as a percentage ± SD. Cells were incu- bated in the presence of [U-13C]glucose with or without a drug for 2 h following a preincubation period of 18 h in the presence or absence of a drug.

Condition

Percentage labelled from [U-13C]glucose

Effects of tolbutamide and glibencamide on [U-13C]glucose metabolism

66 ± 10 65 ± 5 76 ± 1

Control (n ¼ 3) Tolbutamide (n ¼ 3) Glibencamide (n ¼ 2)

ence and absence of the drug, as described in Experi- mental procedures (Table 3). A significant reduction in the ratio was found in the presence of tolbutamide. The fraction of acetyl-CoA derived from [U-13C]glu- cose was determined, and is reported in Table 4. Preincubation with tolbutamide did not change the percentage significantly, indicating that the fraction of glucose entering the tricarboxylic acid cycle via the PDH-mediated conversion to acetyl-CoA did not

To probe further the effect of tolbutamide and to investigate the observed increase in aspartate produc- tion, flux analysis was carried out using [U-13C]glu- cose. Following prior culture for 18 h in the presence of tolbutamide, BRIN-BD11 cells were incubated in the presence of tolbutamide and [U-13C]glucose for 2 h. Control experiments were run in parallel with no drug present. A typical spectrum obtained from con- trol cellular extracts is shown in Fig. 2. There was no significant change in the total amount of labelled glu- tamate, lactate or alanine produced following culture with tolbutamide (data not shown). The ratio of the flux through PC and PDH was determined in the pres-

Glucose

l

3 C c a L

e s o c u G

l

l

l

l

l

2 C e t a t e c A

i

3 C a A

2 C a A

4 C u G

2 C u G

3 C u G

e n a x o D

80

70

60

50

40

30

20

Chemical Shift (p.p.m.)

Fig. 2. A typical 13C-NMR spectrum obtained for control conditions after incubation in the presence of 8.4 mM [U-13C]glucose for 2 h. Lac, lactate.

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Metabolic effects of sulfonylurea exposure

0.6

0.5

change. Thus, the observed change in the ratio of flux through PC and PDH must have been due to changes in anaplerotic metabolism through PC.

0.4

/

0.3

P D M P T N β

0.2

control

tolbutamide

0.1

When cells were preincubated in the presence of glibencamide followed by [U-13C]glucose, the ratio of the flux through PC and PDH did not differ signifi- cantly from the control value.

0

0

5

10

15

25

30

35

40

20 time (h)

31P-NMR studies of intact pancreatic BRIN-BD11 beta cells

Fig. 4. Nucleotide triphosphate levels in intact BRIN-BD11 cells from a representative culture of cells. After a control period of 15 h, the cells were perfused in medium with 100 lM tolbutamide for 24 h.

A typical spectrum obtained from cells grown on fibra- cel beads in a mini-bioreactor is shown in Fig. 3. The T1 (longitudinal relaxation) values for the NTP peaks were calculated using inversion recovery experiments. The following values were found: a, 0.65 ± 0.14 s; b, 0.55 ± 0.05 s; and c, 0.88 ± 0.19 s. Control condi- tions represent conditions where cells were maintained in standard RPMI-1640 medium supplemented with 2 mm glutamine, 10% (v ⁄ v) fetal bovine serum, and 0.1% antibiotics. When tolbutamide was added to the culture medium to give a final concentration of 100 lm, there were no significant changes in the nuc- leotide triphosphate (NTP) levels over a 24 h period (Fig. 4). The free cytoplasmic ADP concentration is to the phosphocreatine ⁄ ATP directly proportional ratio [25,26]. There was no significant change in this ratio on addition of tolbutamide, which, in the absence of a change in the intracellular pH or total creatine pool, indicated that there was no change in free ADP concentration.

(18 h) to sulfonylureas induces specific and readily reversible desensitization to subsequent treatment with the drugs [13,27]. It has also been reported that chro- nic exposure (72–144 h) can result in an irreversible concentration- and time-dependent decline in sulfonyl- urea-induced insulin secretion [28]. As the mechanisms underlying the latter effects remain to be determined, the principal aim of this study was to investigate the impact of sulfonylurea exposure on cellular metabo- lism using clonal pancreatic BRIN-BD11 beta cells. Under the experimental conditions used in this study, there was a significant decrease in acute insulin release following preincubation with the drugs compared to control conditions. Previous studies on tolbutamide have demonstrated that under the same conditions as described in this study, the insulin content does not change [27].

Discussion

Previous studies using clonal pancreatic BRIN-BD11 beta cells have demonstrated that prolonged exposure

Prolonged exposure to tolbutamide and glibenca- mide did not significantly alter the amount of glu- tamate labelled at positions C4 and C3 following a 1 h incubation with [1-13C]glucose. The amount of

i

P

NTP

E M P

R C P

P D M

20

10

-10

-20

0 Chemical Shift (p.p.m.)

Fig. 3. A typical 31P-NMR spectrum of intact BRIN-BD11 cells grown in the mini-bioreactor. MDP, methylene diphosphonate; PME, phospho- monoesters; Pi, inorganic phosphate; PCR, phosphocreatine; NTP, nucleotide triphosphate.

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In the present

study,

ted that the responsiveness of INS-1 cells to glucose- stimulated insulin secretion was linked to the cycling [31] of pyruvate (i.e. the flux through the pyruvate– malate and pyruvate–citrate cycles). In a recent study, Fransson et al. showed, by use of a PC inhibitor, the importance of flux through PC for responsiveness to glucose [32]. the observed decrease in flux through PC observed after prolonged exposure to tolbutamide may be a contributary factor to the resulting drug-induced desensitization to acute stimulation by glucose.

the fluxes

label at the C2 position showed a small decrease fol- lowing incubation in the presence of tolbutamide. The amount of labelled lactate and alanine did not significantly change following incubation with either drug. However, following prolonged exposure to tol- butamide, the amount of aspartate labelled at posi- tions C2 and C3 significantly increased. Aspartate can be formed via a transamination reaction with oxaloacetate, which is itself produced from pyruvate via a reaction catalysed by PC. Oxaloacetate is in equilibrium with malate, which can leave the mitoch- ondrial matrix and in the cytosol is converted back to pyruvate via malic enzyme (pyruvate cycling). To gain a better understanding of these changes, experi- ments were subsequently performed using [U-13C]glu- cose, and analysis of the isotopomers formed allowed through specific enzymes calculation of (Fig. 5).

The present data also indicate differential effects of the two sulfonylureas on beta cell metabolism, as glib- encamide did not change end-product concentrations or the ratio of fluxes through PC and PDH. Preincu- bation with either of the drugs resulted in reduction of subsequent glucose-stimulated insulin release, suggest- ing that there is not a common mechanism of desensi- tization. However, in the present studies, a relatively low concentration of glibencamide (1 lm) was used, due to the reported higher affinity of this drug for KATP channels [33] compared to tolbutamide. Glyb- encamide at 1 lm induces a similar secretory response to that observed for 100 lm tolbutamide [16,34,35].

Early studies investigating the effects of sulfonyl- ureas on ATP levels reported reduced concentrations in islets [36–38]. More recently Elmi et al. [29] showed that glibencamide reduced ATP concentration in the absence of glucose, but the effects were not observed at 10 mm glucose. These observations were used to suggest that the reduced ATP levels may result from increased consumption of ATP by activation of the Na+ ⁄ K+ pump. This is consistent with the results of a 31P-NMR study of intact b-HC9 cells, which revealed

A decrease in the ratio of fluxes through PC and PDH (PC ⁄ PDH) was determined following 18 h of exposure to tolbutamide. However, there was no change in the fraction of acetyl-CoA labelled from [U-13C]glucose via the PDH pathway, indicating that the change in ratio was attributable to a reduction in the flux through PC. Notably, other studies investi- gating the acute effects of glibencamide and megliti- nide on glucose oxidation in mouse pancreatic islets found no inhibitory effects, consistent with our obser- vations that oxidative pathways of glucose metabolism remain unchanged [29]. In recent years, the importance of flux through anaplerotic pathways in beta cells has been highlighted. Cline et al. [30] reported a strong positive correlation between insulin secretion and PC flux in INS-1 cells. Furthermore, Lu et al. demonstra-

[U-13C]glucose

pyruvate

PDH

Acetyl-CoA

PC

citrate

aspartate

OAA

PC

α-KG

malate

PDH PC 1 2 3 4 5

glu

glu

glu

Fig. 5. Overview of the metabolism of [U-13C]glucose. For simplicity, only the iso- topomers of glutamate formed after one turn of the tricarboxylic acid cycle (TCA) are shown. The filled circles represent labelling of the carbon position with 13C. [U-13C]Pyru- vate enters the TCA cycle via pyruvate dehydrogenase (PDH), forming [1,2-13C]acetyl-CoA and consequently [4,5-13C]glutamate. If pyruvate enters via pyruvate carboxylase (PC), two 13C isotopo- mers of oxaloacetate are derived, [1,2,3-13C]oxaloacetate and [3,4-13C]oxalo- acetate, consequently leading to [2,3-13C]glutamate and [1,2,3-13C]glutamate [48]. Glu, glutamate; OAA, oxaloacetate; a-KG, a-ketoglutarate.

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from ours,

in that

(tolbutamide 100 lm and glibencamide 1 lm). Cells were then washed with NaCl ⁄ Pi and preincubated at 37 (cid:2)C for 20 min in Krebs ⁄ Ringer bicarbonate buffer with 1.1 mm d-glucose (115 mm NaCl, 4.7 mm KCl, 1.28 mm CaCl2, 1.2 mm KH2PO4, 1.2 mm MgSO4.7H2O, 10 mm NaHCO3, 5 gÆL)1 BSA, pH 7.4). This was followed by incubation in the presence of 8.4 mm labelled glucose ([1-13C]glucose or [U-13C]glucose) and drug for a specified period (1 h or 2 h). in the Control experiments were carried out in parallel absence of the drug. Following the

that ATP levels did not change on addition of the sul- fonylurea glyburide at glucose concentrations of 5 mm [39]. However, another study using MIN-6 cells showed that if the cells were initally primed with tol- butamide (200 lm), the subsequent increase in ATP in response to 30 mm glucose was potentiated [40]. All of these studies are distinct they focused on the effects of acute sulfonylurea exposure, whereas we examined the effects of prolonged exposure on ATP levels using 31P-NMR. Our data are consistent with other studies, which reported no alteration in cel- lular ATP levels after addition of sulfonylureas in the presence of glucose.

Collectively,

the present data demonstrate novel changes to fluxes in glucose metabolism following pro- longed exposure to the important sulfonylurea drug resulting in a 25% decrease in the tolbutamide, PC ⁄ PDH ratio. Furthermore, these data reveal a reduction in anaplerotic flux through PC. These obser- vations are notable in that they raise the possibility that chronic sulfonylurea exposure in vivo may impact on glucose metabolism, which may contribute to the reported phenomena of sulfonylurea desensitization and, indeed, sulfonylurea failure in type 2 diabetes. Future studies determining the molecular mechanisms of tolbutamide-mediated reduction in flux through PC may lead to the design of more effective insulinotropic drugs in the future.

Experimental procedures

Reagents

the medium was incubation period, removed and stored at ) 20 (cid:2)C. Subsequently, the glucose concentration and the insulin released were measured. The insulin released was measured using a Mercodia (Uppsala, Sweden) ultrasensitive rat insulin ELISA. The metabolites were extracted using a perchloric acid extraction procedure. Briefly, the cells were washed with ice-cold NaCl ⁄ Pi. Per- chloric acid (6%) was added, and the cells were scraped off the culture flasks. The extracts of six culture flasks (approximately 108 cells) were pooled and centrifuged at 200 g with a Sigma 2-15 rotor. The resulting supernatant was neutralized with KOH (5 m and 0.1 m solutions), and the pellets were soaked overnight in 0.1 m NaOH. The pro- tein concentration was determined using the Lowry method [42]. The neutralized supernatant was centrifuged (200 g with a Sigma 2-15 rotor), and the supernatant was treated with Chelex-100 resin and then lyophilized. Each experi- ment was carried out on at least two independent cultures of the BRIN-BD11 cells. The lyophilized cell extracts were dissolved in 3 mL of potassium phosphate buffer (100 mm, pH 7.0) and then centrifuged at 200 g with a Sigma 2-15 rotor. The supernatant was carefully removed, 10% D2O was added, and the pH was checked and adjusted when necessary with 0.1 m NaOH and 0.1 m HCl. NMR experi- ments were performed as detailed below.

Culture of BRIN-BD11 cells at high density in a mini-bioreactor

d-[1-13C]Glucose and d-[U-13C]glucose were obtained from Goss Scientific (Great Baddow, Essex, UK). All other chemicals were obtained from Sigma-Aldrich Chemical Company (Poole, Dorset, UK). Culture media and fetal bovine serum were obtained from Gibco (Glasgow, UK).

Treatment of BRIN-BD11 cells with drugs

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A system was set up to monitor energy metabolism in intact BRIN-BD11 cells as previously described [43]. Briefly, it consists of a 2 L stirred tank fermenter in which the temperature, pH, CO2 content and dissolved O2 content of the culture medium were monitored and maintained within a specified range. The mini-bioreactor is a purpose- built bioreactor consisting of a capped polysulfone tube (10 mm diameter) with an inlet tube and an outlet tube. Cells were maintained attached to fibracel disks (New Brunswick Scientific, Edison, NJ) in the mini-bioreactor and were perfused with medium from the fermenter, which was pumped to the mini-bioreactor in the NMR magnet via water-jacketed tubing at 37 (cid:2)C. Medium in the ferment- er was replaced by fresh medium using a ‘feed and bleed’ the feed and bleed system, system. By adjustment of Pancreatic BRIN-BD11 beta cells were utilized in these in studies [41], representing a particularly useful model which to conduct extensive NMR studies [23,24]. BRIN- BD11 cells were maintained in RPMI-1640 tissue culture medium with 10% (v ⁄ v) fetal bovine serum, 0.1% antibiot- ics (100 UÆmL)1 penicillin and 0.1 mgÆmL)1 streptomycin) and 11.1 mm d-glucose (pH 7.4). The cells were maintained at 37 (cid:2)C in a humidified atmosphere of 5% CO2 and 95% air using a Forma Scientific (Waltham, MA) incubator. For experiments on prolonged exposure to sulfonylureas, the cells were grown in T175 flasks and treated for 18 h in the presence of the drug at the specified concentration

L. Brennan et al.

Metabolic effects of sulfonylurea exposure

nutrients can be maintained at a certain level. For seeding of the bioreactor, the cells were pumped into the mini-bio- reactor as a slow rate over a period of 2 h. Typically 1 · 108 to 3 · 108 cells were passed through the carriers, the cells was routinely and attachment of 85–90% of found.

NMR spectroscopy

13C-NMR of perchloric acid extracts

relaxation delay, and 512 scans. Spectra were recorded at 37 (cid:2)C. Chemical shifts in aqueous media were referenced to methylene diphosphonate at 17.0 p.p.m., which was contained in a sealed capillary in the mini-bioreactor. Expo- nential multiplications with 20 Hz line broadening were performed using winnmr software. The three phosphate groups in NTPs give three distinct peaks. These peaks were primarily attributed to ATP. The T1 values of the NTP peaks were determined using inversion recovery experiments in three independent sets of cells, and these values were then used to optimize the NMR acquisition parameters. To investigate the effects of tolbutamide on energy metabolism, the cells were perfused with medium containing 100 lm tol- butamide for a period of 24 h. Spectra were recorded every 40 min. In some cases, slight acidification of the bioreactor environment was apparent by appearance of a shoulder on the Pi peak attributed to intracellular Pi. When this through the bioreactor was the flow rate occurred, increased as previously described [43]. spectral width, 2.5 s

Statistical analysis

The results are presented as mean ± SD for n separate determinations. Groups of data were compared using Student’s unpaired t-test. Differences were considered signi- ficant at P < 0.05.

Acknowledgements

LB was in receipt of a Health Research Board of fellowship, which is gratefully Ireland postdoctoral acknowledged (PD ⁄ 2002 ⁄ 9).

References

calculated as

31P-NMR of intact cells

1 Aguilar-Bryan L, Nichols CG, Wechsler SW, Clement JPT, Boyd AE 3rd, Gonzalez G, Herrera-Sosa H, Nguy K, Bryan J & Nelson DA (1995) Cloning of the beta cell high-affinity sulfonylurea receptor: a regulator of insulin secretion. Science 268, 423–426. 2 Henquin JC (1998) A minimum of fuel is necessary for tolbutamide to mimic the effects of glucose on electrical activity in pancreatic beta-cells. Endocrinology 139, 993– 998. following the C4 the for For 13C-NMR experiments, an insert containing 5% v ⁄ v dioxane in water was used as an external signal intensity reference. A solution of l-alanine, l-glutamate, lactate and d-glucose, each at a concentration of 100 mm, was prepared and used to quantitate concentrations of metabolites in the 13C spectra. Proton-decoupled 13C spectra were acquired on a Bruker (Karlsruhe, Germany) DRX 500 spectrometer using a 10 mm broadband probe. Typically, spectra were acquired with 32 000 data points using 90(cid:2) pulses, 260 p.p.m. relaxation delay, and 12 000–20 000 scans. Spectra were recorded at 25 (cid:2)C. Chemical shifts were referenced to tetramethylsilane at 0 p.p.m. Data were processed with no zero filling using Bruker winnmr software, and exponential multiplications with 2 Hz line broadening were performed. The assign- ments of the intermediate metabolites were made by com- parison with chemical shift tables in the literature [44] or by addition of 100 mm unlabelled amino acid. The amount of 13C in each resonance was evaluated by integration of the extract peaks and the corresponding peaks in the stand- ard sample relative to the dioxane signal. Corrections for the natural abundance signal were made. In the case of the aspartate peaks, the amount of 13C was estimated by use of the integrals and the known dioxane concentration. The contributions of the individual isotopomers were assessed using the deconvolution routines in winnmr. The absolute enrichments of the l-glutamate were related to the glutam- ate concentration in the extracts, determined by enzymatic methods, to give the specific enrichments [45]. The fluxes reported were obtained by analysis of the isotopomers of glutamate C2 and C4. The ratio between flux through PC ([2,3-13C2] + follows and PDH was [1,2,3-13C3]) ⁄ [4,5-13C2] + [3,4,5-13C3] [46]. The fraction of acetyl-CoA labelled from [U-13C]glucose was calculated using peak: equation (3,4,5-13C) · C4 ⁄ C3 [47]. 3 Ashcroft FM & Gribble FM (1998) Correlating struc- ture and function in ATP-sensitive K+ channels. Trends Neurosci 21, 288–294.

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4 Eliasson L, Renstrom E, Ammala C, Berggren PO, Bertorello AM, Bokvist K, Chibalin A, Deeney JT, Flatt PR, Gabel J et al. (1996) PKC-dependent stimula- tion of exocytosis by sulfonylureas in pancreatic beta cells. Science 271, 813–815. 5 Tian YA, Johnson G & Ashcroft SJ (1998) Sulfonyl- Following removal of the upper barrel of the magnet, the mini-bioreactor was carefully guided into the probe head for the collection of NMR data with the aid of a custom- built holder. Typically, spectra were acquired with 8000 data points using 90(cid:2) pulses, 50 p.p.m. spectral width, 2.0 s ureas enhance exocytosis from pancreatic beta-cells by a

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Metabolic effects of sulfonylurea exposure

19 Schuit F, De Vos A, Farfari S, Moens K, Pipeleers D, mechanism that does not involve direct activation of protein kinase C. Diabetes 47, 1722–1726.

Brun T & Prentki M (1997) Metabolic fate of glucose in purified islet cells. Glucose-regulated anaplerosis in beta cells. J Biol Chem 272, 18572–18579.

6 Flatt PR, Shibier O, Szecowka J & Berggren PO (1994) New perspectives on the actions of sulphonylureas and hyperglycaemic sulphonamides on the pancreatic beta- cell. Diabete Metab 20, 157–162.

7 Kamp F, Kizilbash N, Corkey BE, Berggren PO & Hamilton JA (2003) Sulfonylureas rapidly cross phospholipid bilayer membranes by a free-diffusion mechanism. Diabetes 52, 2526–2531.

8 Pontiroli AE, Calderara A & Pozza G (1994) Secondary failure of oral hypoglycaemic agents: frequency, possible causes, and management. Diabetes Metab Rev 10, 31–43. 20 McCormack JG, Halestrap AP & Denton RM (1990) Role of calcium ions in regulation of mammalian intramitochondrial metabolism. Physiol Rev 70, 391–425. 21 Rutter GA, Burnett P, Rizzuto R, Brini M, Murgia M, Pozzan T, Tavare JM & Denton RM (1996) Subcellular imaging of intramitochondrial Ca2+ with recombinant targeted aequorin: significance for the regulation of pyruvate dehydrogenase activity. Proc Natl Acad Sci USA 93, 5489–5494. 9 Matthews DR, Cull CA, Stratton IM, Holman RR & 22 Kennedy HJ, Pouli AE, Ainscow EK, Jouaville LS,

Rizzuto R & Rutter GA (1999) Glucose generates sub- plasma membrane ATP microdomains in single islet beta-cells. Potential role for strategically located mito- chondria. J Biol Chem 274, 13281–13291. Turner RC (1998) UKPDS 26: sulphonylurea failure in non-insulin-dependent diabetic patients over six years. UK Prospective Diabetes Study (UKPDS) Group. Diabet Med 15, 297–303.

10 Gullo D, Rabuazzo AM, Vetri M, Gatta C, Vinci C, Buscema M, Vigneri R & Purrello F (1991) Chronic exposure to glibenclamide impairs insulin secretion in isolated rat pancreatic islets. J Endocrinol Invest 14, 287–291.

23 Brennan L, Shine A, Hewage C, Malthouse JP, Brindle KM, McClenaghan N, Flatt PR & Newsholme P (2002) A nuclear magnetic resonance-based demonstration of substantial oxidative 1-alanine metabolism and l-ala- nine-enhanced glucose metabolism in a clonal pancreatic beta-cell line: metabolism of l-alanine is important to the regulation of insulin secretion. Diabetes 51, 1714– 1721. 24 Brennan L, Corless M, Hewage C, Malthouse JP, 11 Rabuazzo AM, Buscema M, Vinci C, Caltabiano V, Vetri M, Forte F, Vigneri R & Purrello F (1992) Glyburide and tolbutamide induce desensitization of insulin release in rat pancreatic islets by different mechanisms. Endocrinology 131, 1815–1820.

McClenaghan NH, Flatt PR & Newsholme P (2003) 13C NMR analysis reveals a link between l-glutamine metabolism, d-glucose metabolism and gamma-glutamyl cycle activity in a clonal pancreatic beta-cell line. Diabe- tologia 46, 1512–1521. 12 Ball AJ, Flatt PR & McClenaghan NH (2000) Desensi- tization of sulphonylurea- and nutrient-induced insulin secretion following prolonged treatment with glibencla- mide. Eur J Pharmacol 408, 327–333.

25 Lawson JW & Veech RL (1979) Effects of pH and free Mg2+ on the Keq of the creatine kinase reaction and other phosphate hydrolyses and phosphate transfer reactions. J Biol Chem 254, 6528–6537. 13 McClenaghan NH, Ball AJ & Flatt PR (2001) Specific desensitization of sulfonylurea- but not imidazoline- induced insulin release after prolonged tolbutamide exposure. Biochem Pharmacol 61, 527–536. 14 Rustenbeck I (2002) Desensitization of insulin secretion. Biochem Pharmacol 63, 1921–1935.

26 Matthews PM, Bland JL, Gadian DG & Radda GK (1982) A 31P-NMR saturation transfer study of the regulation of creatine kinase in the rat heart. Biochim Biophys Acta 721, 312–320.

27 McClenaghan NH, Ball AJ & Flatt PR (2000) Induced desensitization of the insulinotropic effects of antidia- betic drugs, BTS 67 582 and tolbutamide. Br J Pharma- col 130, 478–484.

15 Kawaki J, Nagashima K, Tanaka J, Miki T, Miyazaki M, Gonoi T, Mitsuhashi N, Nakajima N, Iwanaga T, Yano H et al. (1999) Unresponsiveness to glibenclamide during chronic treatment induced by reduction of ATP- sensitive K+ channel activity. Diabetes 48, 2001–2006. 16 Anello M, Gilon P & Henquin JC (1999) Alterations of insulin secretion from mouse islets treated with sulpho- nylureas: perturbations of Ca2+ regulation prevail over changes in insulin content. Br J Pharmacol 127, 1883– 1891. 28 Ball AJ, McCluskey JT, Flatt PR & McClenaghan NH (2004) Chronic exposure to tolbutamide and glibencla- mide impairs insulin secretion but not transcription of K(ATP) channel components. Pharmacol Res 50, 41– 46. 17 MacDonald MJ (1993) Glucose enters mitochondrial 29 Elmi A, Idahl LA & Sehlin J (2000) Relationships

FEBS Journal 273 (2006) 5160–5168 ª 2006 The Authors Journal compilation ª 2006 FEBS

5167

metabolism via both carboxylation and decarboxylation of pyruvate in pancreatic islets. Metabolism 42, 1229– 1231. between the Na(+) ⁄ K(+) pump and ATP and ADP content in mouse pancreatic islets: effects of meglitinide and glibenclamide. Br J Pharmacol 131, 1700–1706. 30 Cline GW, Lepine RL, Papas KK, Kibbey RG & Shulman GI (2004) 13C NMR isotopomer analysis of 18 Khan A, Ling ZC & Landau BR (1996) Quantifying the carboxylation of pyruvate in pancreatic islets. J Biol Chem 271, 2539–2542.

L. Brennan et al.

Metabolic effects of sulfonylurea exposure

anaplerotic pathways in INS-1 cells. J Biol Chem 279, 44370–44375. magnetic resonance spectroscopy and respirometry stud- ies. Diabetes 52, 394–402. 31 Lu D, Mulder H, Zhao P, Burgess SC, Jensen MV,

40 Ainscow EK & Rutter GA (2001) Mitochondrial prim- ing modifies Ca2+ oscillations and insulin secretion in pancreatic islets. Biochem J 353, 175–180. 41 McClenaghan NH, Barnett CR, Ah-Sing E, Abdel-

Kamzolova S, Newgard CB & Sherry AD (2002) 13C NMR isotopomer analysis reveals a connection between pyruvate cycling and glucose-stimulated insulin secretion (GSIS). Proc Natl Acad Sci USA 99, 2708–2713. 32 Fransson U, Rosengren AH, Schuit FC, Renstrom E &

Wahab YH, O’Harte FP, Yoon TW, Swanston-Flatt SK & Flatt PR (1996) Characterization of a novel glucose-responsive insulin-secreting cell line, BRIN- BD11, produced by electrofusion. Diabetes 45, 1132–1140. Mulder H (2006) Anaplerosis via pyruvate carboxylase is required for the fuel-induced rise in the ATP:ADP ratio in rat pancreatic islets. Diabetologia 49, 1578–1586. 33 Panten U, Burgfeld J, Goerke F, Rennicke M,

42 Lowry OH, Rosebrough NJ, Farr AL & Randall RJ (1951) Protein measurement with the Folin phenol reagent. J Biol Chem 193, 265–275.

Schwanstecher M, Wallasch A, Zunkler BJ & Lenzen S (1989) Control of insulin secretion by sulfonylureas, meglitinide and diazoxide in relation to their binding to the sulfonylurea receptor in pancreatic islets. Biochem Pharmacol 38, 1217–1229. 43 Thelwall PE & Brindle KM (1999) Analysis of CHO-K1 cell growth in a fixed bed bioreactor using magnetic resonance spectroscopy and imaging. Cytotechnology 30, 121–132. 44 Fan TWM (1996) Metabolite profiling by one- and

34 McClenaghan NH & Flatt PR (1999) Physiological and pharmacological regulation of insulin release: insights offered through exploitation of insulin-secreting cell lines. Diabetes Obes Metab 1, 137–150. 35 Groop LC (1992) Sulfonylureas in NIDDM. Diabetes two-dimensional NMR analysis of complex mixtures. Prog Nucl Magnet Reson Spectrosc 28, 161–219. Care 15, 737–754.

45 Chateil J, Biran M, Thiaudiere E, Canioni P & Merle M (2001) Metabolism of [1-(13)C) glucose and [2- (13)C]acetate in the hypoxic rat brain. Neurochem Int 38, 399–407. 36 Hellman B, Idahl LA & Danielsson A (1969) Adenosine triphosphate levels of mammalian pancreatic B cells after stimulation with glucose and hypoglycemic sulfo- nylureas. Diabetes 18, 509–516.

37 Welsh M (1983) The effects of glibenclamide on rat islet radioactive nucleotide efflux, ATP contents and respirat- ory rates. Biochem Pharmacol 32, 2903–2908. 38 Detimary P, Gilon P & Henquin JC (1998) Interplay 46 Lapidot A & Gopher A (1994) Cerebral metabolic com- partmentation. Estimation of glucose flux via pyruvate carboxylase ⁄ pyruvate dehydrogenase by 13C NMR iso- topomer analysis of D-[U-13C]glucose metabolites. J Biol Chem 269, 27198–27208. 47 Malloy CR, Sherry AD & Jeffrey FM (1990) Analysis

of tricarboxylic acid cycle of the heart using 13C isotope isomers. Am J Physiol 259, H987–H995. between cytoplasmic Ca2+ and the ATP ⁄ ADP ratio: a feedback control mechanism in mouse pancreatic islets. Biochem J 333, 269–274. 39 Doliba NM, Vatamaniuk MZ, Buettger CW, Qin W,

FEBS Journal 273 (2006) 5160–5168 ª 2006 The Authors Journal compilation ª 2006 FEBS

5168

48 Haber S & Lapidot A (2001) Energy fuel utilization by fetal versus young rabbit brain: a 13C MRS isotopomer analysis of [U-(13)C]glucose metabolites. Brain Res 896, 102–117. Collins HW, Wehrli SL, Carr RD & Matschinsky FM (2003) Differential effects of glucose and glyburide on energetics and Na+ levels of betaHC9 cells: nuclear