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Sodium Palmitate Induces Partial Mitochondrial Uncoupling and Reactive Oxygen Species in Rat Pancreatic Islets in Vitro¹

Department of Medical Cell Biology, Uppsala University, Uppsala, Sweden

Address all correspondence and requests for reprints to: Dr. Nils Welsh, Department of Medical Cell Biology, Biomedical Center, P.O. Box 571, S-751 23 Uppsala, Sweden. E-mail: nils.welsh{at}medcellbiol.uu.se

	Abstract

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The aim of the present investigation was to study whether prolonged exposure of isolated rat islets to the long chain fatty acid sodium palmitate leads to uncoupling of respiration. It was found that culture of islets in the presence of palmitate abolished glucose-sensitive insulin release and decreased insulin contents. This was paralleled by decreased ATP contents, increased respiration, and decreased islet cell mitochondrial membrane potential. Using electron microscopy, an increase in the ß-cell mitochondrial volume in islets exposed to palmitate was observed. The addition of the uncoupler carbonyl cyanide p-(trifluoromethoxy)phenylhydrazone, at a concentration that decreased mitochondrial membrane potential to a similar extent as palmitate, diminished the glucose-induced insulin release. In addition, islet generation of reactive oxygen species, but not of nitric oxide, was increased in response to a long-term palmitate exposure. It is concluded that long-term exposure to a long chain fatty acid induces partial uncoupling of ß-cell oxidative phosphorylation and that this may contribute to the loss of glucose-sensitive insulin release.

	Introduction

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THE METABOLIC syndrome seen in type 2 diabetes is thought to result from an impaired action of insulin on target cells and an abnormal insulin secretion (1). Type 2 diabetes is often associated with obesity and increased levels of circulating FFA (2). In healthy individuals the levels of FFA usually range between 0.2–0.7 mM, whereas in diabetics the levels are higher and may reach concentrations of 1.0 mM (3, 4, 5). This has led to the proposal that high FFA levels might aggravate the diabetic condition by increasing the peripheral resistance to insulin and inducing hepatic gluconeogenesis (2). Moreover, increased levels of FFA seem to inhibit the function of the insulin-producing ß-cell. Indeed, reports have proposed that FFA directly impair the secretory capacity of pancreatic ß-cells (6, 7).

The long-term inhibitory effects of FFA on islet ß-cell function were first characterized by Zhou and Grill (7). It was observed that FFA induced inhibitory actions on islet glucose-induced insulin secretion and biosynthesis after a 48-h exposure period. Similar observations were made in an in vivo model in which a lipid emulsion was infused into rats (6). Inhibition of insulin release induced by long term FFA exposure was explained in terms of a glucose-fatty acid cycle (8), i.e. that addition of FFA leads to inhibition of glucose metabolism via a lowered pyruvate dehydrogenase activity (9) and an increased activity of carnitine palmitoyl transferase I (10). Other reports have suggested that inhibitory actions of palmitate are due to build-up of long chain fatty acyl-coenzyme A (acyl-CoA) thioesters, leading to enhanced activity of hexokinase and phosphofructokinase (11, 12), decreased activity of GLUT2 and glucokinase (13), increased oxidation of FFA (14), or activation of the ATP-sensitive K⁺ channel (15).

It has been well known for some 40 yr now that FFA act as weak uncouplers of mitochondrial respiration. FFA uncoupling is associated with a decrease in mitochondrial membrane potential (), enhanced state 4 respiration, lower ATP generation, and mitochondrial swelling (16). Although this effect of FFA has been observed in a wide variety of cells (17), FFA-induced uncoupling in insulin-producing cells has, to our knowledge, not yet been addressed. It was therefore the aim of the present investigation to study the in vitro effects of FFA on ß-cell mitochondrial function and morphology, and our findings suggest that palmitate induces partial mitochondrial uncoupling.

	Materials and Methods

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Islet isolation and culture
Three-month-old male Sprague Dawley rats (B&K Universal, Sollentuna, Sweden) were killed by cervical dislocation. Islets were isolated from pancreas by collagenase digestion (Boehringer Mannheim, Mannheim, Germany) and then used directly for acute experiments or precultured free-floating for 3–5 days in RPMI 1640 supplemented with 10% FCS, 2 mM L-glutamine, benzylpenicillin (100 U/ml), and streptomycin (0.1 mg/ml) at 37 C in a humidified atmosphere of air and 5% CO₂ (18). After preculture, the islets were transferred to the same medium containing either 0.24% (wt/vol) fatty acid-free BSA or 0.24% BSA and 0.32 mM sodium palmitate. To solubilize these additions, the media were first sonicated in a sonication bath for 2 min, heated briefly to 60 C, and then resonicated. After solubilization of the palmitate, the pH of the medium was adjusted to 7.4 using 2 M NaOH. The glucose concentrations of the medium were 2.8, 11.1, or 28 mM as given in tables and figures.

Islet insulin release and content
For determination of insulin release after culture for 48 h with or without palmitate, islets were incubated in groups of 10 in 100 µl Krebs-Ringer bicarbonate buffer supplemented with 10 mM HEPES (KRBH). The incubation was carried out at 37 C for 60 min in the presence of 1.7 or 17 mM glucose. Insulin release to the incubation buffer was determined according to the method of Heding (14). Islets were then recovered, sonicated in 200 µl H₂O, and subsequently used for DNA and insulin content determinations (19, 20).

Islet respiration
Islet respiration was measured by the Cartesian diver technique modified according to the method of Hellerström (21). Islets in groups of 5–10 were placed in a Cartesian diver, which is a glass capillary open at the top with an internal volume of approximately 10 µl, and were allowed to respire in ambient air for 60 min at 37 C in a 10 mM HEPES-buffered Krebs-Ringer solution (pH 7.4) in which the NaHCO₃ had been replaced with an equimolar amount of NaCl. The buffer contained 1.7 mM glucose. The glucose concentration was then increased to 17 mM by forcing a side drop to fuse with the islet-containing buffer, and the incubation was continued for another 60 min. Throughout the incubation periods the equilibrium pressure, i.e. an externally applied pressure, which makes the diver float at a specific point, was measured on a manometer. Oxygen uptake was expressed as nanoliters of O₂ per islet/h.

ATP contents
For determination of ATP contents, islets cultured for 48 h with or without palmitate were rapidly washed with cold PBS and then sonicated briefly in 50 µl ice-cold 5% (vol/vol) perchloric acid containing 2 mM EDTA. The samples were neutralized by adding 2 M NaOH. After dilution with 0.1 M Tris-acetate buffer supplemented with 2 mM EDTA, ATP reagent was added (Bio-Orbit, Turku, Finland), and determinations were performed using bioluminescence. ATP contents were calculated against an ATP standard curve.

5,5'6,6'-tetrachloro-1,1',3,3'-tetraethylbenzimidazol-carbocyanine iodide (JC-1) and dichlorofluoroscein (DCFH) fluorescence
For determination of JC-1 (Molecular Probes, Inc. Europe, Leiden, The Netherlands) fluorescence, islets in groups of 100 were either precultured for 24 h with or without palmitate or used directly. In these experiments, palmitate was dissolved in ethanol, and all groups received the same amount of vehicle (2%, vol/vol). The islets were then incubated for 20 min at room temperature in the same culture medium as that used during the preculture with the additional supplementation of 10 µg/ml JC-1 (solubilized in N,N-dimethylformamide; 1%, vol/vol). This was followed by trypsin digestion (0.5%, wt/vol) for 8 min at 37 C. The dispersed cells were resuspended in KRBH containing 5 mM glucose, and aliquots (100 µl) of the cell suspensions were applied to a 96-well plate. After preincubation for 20 min at 37 C, the fluorescence was determined using a Perkin-Elmer LS-5B luminescence spectrometer (Norwalk, CT) with excitation wavelength at 490 nm and emission wavelength at 590 nm. In other experiments, different concentrations of palmitate and carbonyl cyanide p-(trifluoromethoxy)phenylhydrazone (FCCP) were added, and the fluorescence was followed for an additional 60–90 min. Fluorescence was corrected by subtracting parallel blanks and expressed per µg DNA, which was recovered in each well (20).

For determination of DCFH oxidation, dispersed islet cells were preincubated for 20 min at 37 C in KRBH supplemented with 5 mM glucose and 10 µM DCFH diacetate (DCFH-DA; Acros Organics, Geel, Belgium). The fluorescence was determined (time zero) with excitation wavelength at 505 nm and emission wavelength at 535 nm (22). To some groups 0.2 mM palmitate was added at time zero. Determinations were performed every 20 min during 80 min at 37 C. Fluorescence was corrected by subtracting parallel blanks and expressed per µg DNA, which was recovered in each well.

Nitrite determination
For nitrite determinations, islets were cultured for 24 h in groups of 50 in 500 µl culture medium with or without 0.32 mM sodium palmitate or with 50 U/ml interleukin-1ß (provided by Dr. Klaus Bendtzen, Rigshospitalet, Copenhagen, Denmark). Blanks with or without sodium palmitate were run in parallel. Nitrite levels in culture medium samples (two, 80 µl each) were determined with the Greiss reagent as previously described (23).

Electron microscopy
Electron microscopy was essentially performed as previously described (24). Groups of 100 islets from two different preparations were cultured with or without 0.32 mM palmitate for 24 h, fixed in 2.5% (vol/vol) glutaraldehyde, and embedded in Epon 812. Ultrathin sections were contrasted with uranyl acetate and lead citrate. Electron microscopy was carried out with a Hitachi H-7100 transmission electron microscope at an accelerating voltage of 75 kV. In the morphometric analysis only islet ß-cells were taken into account. They were identified by the typical structure of their secretory granules. Measurements were made on 64 individual ß-cells from 9 islets not treated with palmitate and 49 individual ß-cells from 8 islets treated with palmitate. For each individual ß-cell profile in the tissue sections, the area, the number of mitochondria and the total mitochondrial section area were determined. All electron microscopic photographs were analyzed blindly with respect to treatment.

	Results

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Effects of palmitate on islet cell mitochondrial membrane potential
A short term (90-min) exposure to palmitate moderately increased JC-1 J-aggregate fluorescence (Fig. 1), which gives a quantitative estimate of (25). This effect was observed at 0.1 mM palmitate and reached its maximum at 0.2 mM palmitate (Fig. 1). The uncoupler FCCP promoted a rapid and pronounced loss of JC-1 fluorescence (Fig. 1). The FCCP effect was maximal at 1 µg/ml and only partial (20%) at 0.1 µg/ml (Fig. 2). Culture for 24 h in the presence of 0.2 mM palmitate induced a 24% decrease in JC-1 fluorescence in the presence of 28 mM glucose (Fig. 3). At 2.8 mM glucose, however, there was only a nonsignificant trend for lower JC-1 fluorescence in response to palmitate.

View larger version (14K): [in this window] [in a new window]   Figure 1. Short term effects of palmitate and FCCP on JC-1 fluorescence in dispersed islet cells. Isolated rat islets were loaded with 10 µg/ml JC-1 for 20 min at room temperature. The islets were dispersed, and cells were placed in 96-well plates. At time zero, basal fluorescence was determined, and additions of palmitate and FCCP (1 µg/ml) were made. The same amount of vehicle (ethanol) was added to control cells and to the experimental groups. Fluorescence was followed for 90 min, and the results are expressed as the change in fluorescence (arbitrary units) compared with that at time zero. Results are means of three observations.

View larger version (10K): [in this window] [in a new window]   Figure 2. Short term effects of FCCP on JC-1 fluorescence in dispersed islet cells. Isolated rat islets were loaded with 10 µg/ml JC-1 for 20 min at room temperature. The islets were dispersed, and cells were placed in 96-well plates. At time zero, basal fluorescence was determined, and additions of different concentrations of FCCP were made. Fluorescence was determined after 90 min, and the results are expressed as the change in fluorescence (arbitrary units) compared with that at time zero. Results are the mean ± SEM for three separate experiments.

View larger version (47K): [in this window] [in a new window]   Figure 3. Long-term effects of palmitate on DCFH and JC-1 fluorescence. For DCFH fluorescence, islets were cultured for 24 h at 11.1 mM glucose with or without 0.2 mM palmitate and then dispersed into free islet cells by trypsin digestion. The cells were incubated at 37 C in KRBH buffer containing 5 mM glucose and 10 µM DCFH-DA with or without 0.2 mM palmitate. DCFH fluorescence was determined after 60 min, and the cells were recovered for DNA content determinations. Results are expressed as a percentage of the control value and are the mean ± SEM for three observations. * and **, P < 0.05 and P < 0.01, respectively, for a chance difference vs. corresponding control, using Student’s paired t test. For JC-1 fluorescence, rat islets were cultured for 24 h in 2.8 or 28 mM glucose with or without 0.2 mM palmitate. Islets were then loaded for 20 min with 10 µg/ml JC-1, dispersed, and resuspended in KRBH containing 5 mM glucose. The fluorescence was determined after 30 min. Arbitrary fluorescent units were corrected for DNA content and expressed as a percentage of the control value (2.8 mM glucose). Results are the mean ± SEM for eight observations. *, P < 0.05 vs. 28 mM glucose, using Student’s paired t test.

View this table: [in this window] [in a new window]   Table 2. Effects of -ketoisocaproate and K+ on insulin release of palmitate-cultured islets

Effects of palmitate on islet ATP contents and oxygen uptake
High glucose culture induced a slight increase in ATP in control islets, an effect that was not seen in palmitate cultured islets (Table 3). Indeed, the ATP content of palmitate islets cultured at 28 mM glucose was significantly lower than that of corresponding control islets (Table 3). In 11 and 2.8 mM glucose-cultured islets, there was a slight trend of lower and higher ATP contents in response to palmitate, respectively (Table 3).

Effects of palmitate on islet cell reactive oxygen species (ROS) and nitric oxide (NO) generation
DCFH-DA produces a fluorescent signal after intracellular oxidation by ROS such as hydrogen peroxide and the hydroxyl radical. The generation of ROS was higher in islet cells exposed to palmitate for 24 h than in corresponding controls (Fig. 3). The acute addition of palmitate to control or palmitate-cultured islets did not enhance ROS production (Fig. 3). Islets exposed to palmitate for 24 h did not produce more nitrite, which is the stable end product of NO, than controls (0.12 ± 0.08 pmol nitrite/islet·h for controls and 0.18 ± 0.06 pmol nitrite/islet·h for palmitate-exposed islets; n = 6). However, increased nitrite production was observed in response to interleukin-1ß (0.64 ± 0.11 pmol nitrite/islet·h; P < 0.01 vs. controls, by Student’s paired t test), which is a well known activator of iNOS in rat islet cells (21).

Effects of palmitate on ß-cell mitochondrial morphology
The ultrastructural analysis showed a normal mitochondrial morphology of ß-cells in both control and palmitate-treated islets. No signs of disrupted mitochondrial cristae or other disturbances were seen. The area of the individual ß-cell profiles in the tissue sections was 31.6 ± 2.2 µm² in control islets and 36.2 ± 2.1 µm² in islets exposed to palmitate (P > 0.05), which indicates that there was no significant difference in the size and form of the cells between the two experimental groups. The total mitochondrial section area in the individual ß-cell profiles was 1.6 ± 0.2 µm² in islets incubated without palmitate and 2.1 ± 0.2 µm² in islets incubated with palmitate (P > 0.05). The frequency distribution for this area showed for both groups no significant deviation from the normal Gaussian distribution, and no specific subpopulation of ß-cells with diverging mitochondrial content was found. The number of mitochondria per individual ß-cell profile was 14.9 ± 1.4 in control and 16.2 ± 1.5 in palmitate-treated islets (P > 0.05). From the primary measurements, the average section area per mitochondrium was 0.104 ± 0.003 µm² in the absence and 0.134 ± 0.007 µm² in the presence of palmitate (P < 0.001, by Student’s unpaired t test). Thus, the section area was 29% greater in the ß-cells exposed to palmitate. Assuming a spherical shape of the mitochondria, this would correspond to a 46% greater mitochondrial volume.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

 
By culturing rat pancreatic islets in the presence of palmitate for 1–2 days, we observed that palmitate-inhibited insulin release was paralleled by increased respiration, decreased ATP content, lower , and increased mitochondrial volume, all signs typical of uncoupling (16). Somewhat unexpectedly, there was only a weak trend of lower ATP contents after culture at 11 mM glucose. However, as we did not determine ADP and AMP levels, it is possible that a palmitate-induced lowering of ATP was partially counteracted by an increase in the total ATP-ADP-AMP pool. Interestingly, uncoupling was not observed in short term experiments, which is in line with previous findings showing that ß-cell function is initially stimulated by exposure to FFA (6). Stimulation of ß-cell function by FFA has among other explanations been ascribed to the oxidation of FFA leading to increased generation of ATP (26). Indeed, we presently observed a modest increase in in response to an acute palmitate challenge. This dual role of FFA as both an uncoupler and a substrate for mitochondrial oxidation has long confounded investigations dealing with FFA-induced uncoupling. However, in a recent study (27), a nonmetabolizable FFA was used to demonstrate that uncoupling occurs in liver cells independently of its mitochondrial oxidation. The opposite situation can be achieved by using a short chain FFA, such as octanoate, which is known not to induce uncoupling. Long-term supplementation of octanoate to insulin-producing cells potentiates, rather than inhibits, glucose-stimulated insulin release (28). In line with this, our results with rat islet cells suggest that palmitate acts as an uncoupler also in the insulin-producing cell and that this effect predominates over the nutrient effect when the FFA is present for 24–48 h. Although the palmitate-induced decrease in was modest, it is likely that it contributes to the loss of insulin release, as a similar decrease in induced by FCCP affected the glucose-induced insulin release negatively. Thus, it is probable that FFA-induced uncoupling accounts at least in part for the loss of glucose-sensitive insulin release.

Other sites at which FFA and their CoA esters could interfere with glucose-induced insulin release are at the level of glucose phosphorylation and the ATP-sensitive K⁺ channel (13, 15). The present findings that the glucokinase-independent nutrient KIC did not stimulate insulin release in palmitate-cultured islets support the idea that mitochondrial events contribute to the poor insulin release of these cells. Moreover, it is possible to interpret the weak response to KCl to indicate that the secretory defect could involve an enhanced opening of the ATP-sensitive K⁺ channel, either by a lowering of the ATP/ADP ratio or by a direct effect of long chain acyl-CoA on the channel. The insulin release data are, however, not easily interpreted, because the increased basal insulin release of the palmitate-cultured islets could have masked the effects of KIC and KCl. In addition, it is not clear whether the high basal release of insulin is due to the increased hexokinase/glucokinase ratio or to passive leakage of insulin as a result of the beginning of palmitate-induced lipotoxicity.

FFA are thought to act as protonophores, which move from the outer to the inner lipid layer of the inner mitochondrial membrane in the protonized form and flip-flop back in the anionic form, leading to acidification of the matrix and loss of membrane potential (16). Flip-flopping of long chain FFA, but not of short chain FFA, occurs spontaneously when the fatty acid is protonized, but not when it is unprotonized (29). Thus, FFA will not affect conductance over artificial phospholipid bilayers that lack membrane proteins, as specific proteins are required for the uniport of amphiphilic anions. It has been demonstrated that at least four proteins facilitate the unilateral transport of the anionic fatty acid, namely the mammalian uncoupling protein (UCP) (30), the potato and tomato plant uncoupling mitochondrial protein (31), the ATP/ADP translocator (32), and the glutamate/aspartate transporter (33). Elegant studies have demonstrated that the presence of these proteins in lipid bilayers leads to uptake of amphiphilic anions, and that if the substrate (FFA) can associate with H⁺ at physiological pH, a proton flux is created, whereas with dissociated substrates (long chain alkylsulfonates) no proton flux is induced (30).

It is not clear which carrier translocates palmitate across the mitochondrial inner membrane in the insulin-producing cell. One possible candidate is the ATP/ADP translocator, which is differentially expressed in ß-cells in response to different ß-cell toxins and metabolic stimuli (34). A second possibility is the mammalian UCP-2, which is also expressed in pancreatic islets (35). We have presently observed that acute addition of palmitate (<2 h) does not induce uncoupling. This might indicate that a gradual build-up of FFA, fatty acyl-CoA thioesters, and triglycerides (36) leads to an altered gene expression, which precedes the uncoupling effect. Indeed, FFA have recently been shown to increase the expression of UCP-2 messenger RNA in islet cells (37). Therefore, it is tempting to speculate that palmitate-induced gene expression and uncoupling occur to decrease intracellular stores of triglycerides. Interestingly, it has recently been demonstrated that fatty acyl-CoA thioesters are ligands of the hepatic nuclear factor-4 and that specific fatty acids are ligands of peroxisome proliferator-activated receptor- (38, 39). These transcription factors are known to control the expression of genes that code for several metabolic enzymes (39, 40). Thus, it is possible that prolonged exposure to high levels of FFA promotes hepatic nuclear factor-4 or peroxisome proliferator-activated receptor- activation and thereby alters gene transcription of metabolic enzymes, possibly UCP-2, leading to uncoupling. This hypothesis could also explain why a decrease in ATP contents and was only observed after culture at 28 mM glucose. Hypothetically, the combination of high glucose and palmitate might synergize in the induction of UCPs, because glucose, by increasing malonyl-CoA contents (41), slows down FFA oxidation and thereby increases cellular contents of fatty acyl-CoA thioester and triglycerides.

It appears that FFA-induced regulated uncoupling plays an important role in processes such as ripening of fruit (31), heat production in brown fat and skeletal muscle (42), and enhanced hydrolysis and oxidation of lipids in white fat (35). Our findings suggest that the insulin-producing cell also responds to FFA by uncoupling. Whether this is a physiological response with the purpose of decreasing insulin release or only a way to diminish intracellular stores of triglycerides remains to be established. However, it is easily envisaged that FFA-induced ß-cell uncoupling in vivo would worsen the condition of a type 2 diabetic patient. Moreover, if the insulin-producing cell is exposed to high levels of both FFA and glucose for prolonged periods of time, it is conceivable that ROS-induced damage is inflicted. It is known that state 4 respiration is associated with enhanced ROS production (43), which is in line with our present findings. It is also noteworthy that insulin-producing cells have a low antioxidative capacity (44), which would predispose them to damage induced by prolonged regulated uncoupling.

	Acknowledgments

 
The excellent technical assistance of I.-B. Hallgren, C. Gökturk, and A. Nordin is gratefully acknowledged.

	Footnotes

 
¹ This work was supported by grants from the Swedish Medical Research Council (12X-109, 12X-11564), the Swedish Diabetes Association, the Novo-Nordisk Insulin Foundation Committee, the Juvenile Diabetes Foundation International, the Swedish-American Research Program, the Gustavsson Foundation, and the Family Ernfors Fund.

Received November 5, 1998.

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