©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
Activation of the ATP-sensitive K Channel by Long Chain Acyl-CoA
A ROLE IN MODULATION OF PANCREATIC beta-CELL GLUCOSE SENSITIVITY (*)

(Received for publication, November 3, 1995; and in revised form, February 7, 1996)

Olof Larsson (1) Jude T. Deeney (1) Robert Bränström (1) Per-Olof Berggren (1) Barbara E. Corkey (2)(§)

From the  (1)Department of Molecular Medicine, The Rolf Luft Center for Diabetes Research, Karolinska Institute, S-17176 Stockholm, Sweden and the (2)Diabetes and Metabolism Unit, Evans Department of Medicine and Department of Biochemistry, Boston University Medical Center, Boston, Massachusetts 02118

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
FOOTNOTES
REFERENCES

ABSTRACT

Long term exposure to elevated levels of long chain free fatty acids decreases glucose-induced insulin secretion from pancreatic islets and clonal pancreatic beta-cells. The mechanism for this loss of glucose sensitivity is at present not known. In this study, we evaluated the possibility that increases in long chain acyl-CoA esters (LC-CoA), the metabolically active form of free fatty acids, might mediate the loss of glucose sensitivity. We observed that cellular levels of LC-CoA increased more than 100% in response to overnight incubation with 0.5 mM palmitic acid complexed to albumin. In the same studies, the total CoA pool increased by about 40%. Patch-clamp studies demonstrated that saturated and unsaturated LC-CoA, but not malonyl-CoA or free CoASH, induced a rapid and slowly reversible opening of ATP-sensitive K channels. The effect was concentration-dependent between 10 nM and 1 µM. These findings indicate that the ATP-regulated K channel is a sensitive target for LC-CoA and suggest that high levels of LC-CoA, which accumulate in response to hyperglycemia or prolonged exposure to free fatty acids, may prevent channel closure and contribute to the development of beta-cell glucose insensitivity.


INTRODUCTION

Exposure to elevations in free fatty acids (FFA) (^1)decreases glucose-induced insulin secretion. The concept of gluco-lipo-toxicity is increasingly being invoked to explain such loss of glucose-induced insulin secretion, but the identity of putative effector molecules that might mediate these effects is unknown. Normal glucose-induced insulin secretion is associated with inhibition of FFA oxidation and increased lipid synthesis in pancreatic beta-cells(1, 2, 3, 4) . In addition, exogenous FFA acutely potentiate glucose-stimulated insulin secretion(4, 5) . We have demonstrated that glucose causes marked alterations in the acyl-CoA profile of clonal pancreatic beta-cells, with the largest (5-fold) and earliest (by 2 min) change occurring in malonyl-CoA(1, 5) . However, we did not obtain a good correlation between secretion and malonyl-CoA levels but rather between secretion and decreases in long chain acyl-CoA (LC-CoA) levels(5) .

The total CoA pool is fixed over short intervals and distributed between mitochondrial and cytosolic compartments that are not interchangeable(6, 7) . Thus, during an acute response, the maximum LC-CoA concentration is limited by the total CoA pool and its distribution between cytosol and mitochondria. In some cell types, high fat and certain drugs or steroids have the potential to increase the total CoA pool over a period of hours to days and also lead to increases in the LC-CoA pool(7) .

Our studies were undertaken to determine whether increased levels of LC-CoA occur in response to exposure of beta-cells to FFA and to assess the effect of physiological concentrations of LC-CoA on the ATP-sensitive K channel (K channel). We demonstrate, for the first time, that both total CoA and LC-CoA levels increase in cells cultured in elevated FFA and document dramatic increases in K channel activity in response to LC-CoA.


EXPERIMENTAL PROCEDURES

Growth and Incubation of Cells and Islets

Adult obese hyperglycemic mice (gene symbol ob/ob) of both sexes were obtained from a local non-inbred colony. The mice were starved for 24 h, and islets were isolated by collagenase digestion and dispersed into single cells as described previously(8) . The cells were resuspended in RPMI 1640 medium, supplemented with 100 units/ml penicillin, 100 µg/ml streptomycin, 60 µg/ml gentamycin, and 10% fetal calf serum. The cell suspension was plated in Petri dishes and incubated at 37 °C in 5% CO(2) for 1-3 days. Clonal pancreatic beta-cells (HIT-T15) were cultured in RPMI 1640 medium supplemented with 50 units/ml penicillin, 50 µg/ml streptomycin, and 10% fetal calf serum, used between passages 64 and 80, harvested with phosphate-buffered saline containing 0.02% EDTA, and washed in Hanks' Ca-Mg free buffer, pH 7.4(9) .

Electrophysiology

The electrophysiology experiments were carried out using the inside-out configuration of the patch-clamp technique (10) on dispersed mouse beta-cells. This type of recording mode allows access to the cytoplasmic side of the plasma membrane. The electrodes had resistances between 3 and 4 megaohms when filled with an extracellular buffer containing (in mM): 138 NaCl, 5.6 KCl, 1.2 MgCl(2), 2.6 CaCl(2) and 5 Hepes-NaOH, pH 7.4. The bath solution contained (in mM): 125 KCl, 1 MgCl(2), 10 EGTA, 30 KOH, 5 Hepes, pH 7.15. Channel activity was measured at 0 mV membrane potential. With the solutions used, ion currents are outward (i.e. into the pipette). Channel records are displayed with upward deflections denoting outward currents. The K channel activity is identified based on the unitary amplitude (1.5-2 pA) and its sensitivity to ATP. All experiments were carried out at room temperature (22-24 °C). ATP was added as the Mg salt, CoASH as the Na salt, CoA esters were dissolved in water and the Na salt of oleic acid was dissolved in 95% ethanol. The final concentration of ethanol was 0.1%. Patches were excised into nucleotide-free solution, and 0.1 mM ATP was first applied to test for channel inhibition. After inhibition had been demonstrated, ATP was removed and the patch was subsequently exposed to the test solutions indicated in figures.

Assays and Materials

Acyl-CoA esters were extracted and measured enzymatically as described previously(7, 11) . Insulin was assayed by radioimmunoassay using the assay protocol and reagents from Linco Research Inc. (St Louis, MO). RPMI 1640 medium, penicillin, and streptomycin were from Life Technologies, Inc. Fetal bovine serum was obtained from Hyclone Laboratories. Biochemicals were from Sigma or Boehringer Mannheim.

Data Analysis

Single K current records were filtered at 300 Hz (-3 db value, 8-pole Bessel filter, Frequency Devices, Haverhill, MA), digitized at 800 Hz using an Axon instrument ADC, and stored in a computer. Digitized segments of current records (30-40 s) were used to determine channel activity under different conditions. The mean current was calculated according to the equation,

where n is the number of samples, i(j) is the current registered in sample j and I(B) is the value of a user-defined base line. Traces represent experiments that were performed at least five times using cells from separate animals. Mean currents (i(x)) were determined during selected intervals designated by time lines in the figures. Statistical differences in concentrations of acyl-CoA esters were compared using Student's t test for unpaired two-tailed data.


RESULTS AND DISCUSSION

Culture of isolated rat islets or clonal beta-cells in elevated concentrations of FFA decreases the ability of glucose to stimulate insulin secretion. We performed studies in which clonal beta-cells (HIT-T15), incubated overnight in medium containing 0.5 mM palmitate, exhibited a 50% decrease in the ability of glucose to stimulate insulin secretion (data not shown). This observation is consistent with previously published findings in islets from starved animals or animals exposed to high circulating levels of FFA in which glucose-induced insulin release is diminished(12, 13) . Analysis of soluble and insoluble pools of acyl-CoA esters showed that overnight exposure to 0.5 mM palmitic acid increased the pool of LC-CoA, the metabolically active form of FFA, as well as the total CoA pool without affecting the short chain acyl-CoA ester pool (Table 1). The 100% increase in LC-CoA was opposite in direction and greater in magnitude than the change in secretion. These findings suggest that the accumulation of LC-CoA could be causally related to a loss of responsiveness to glucose.



It is well established that one of the initial events in the beta-cell stimulus secretion coupling is closure of the K channel. The activity of this channel is also the main determinant of the beta-cell resting potential(14) . One possible explanation for the inhibition of glucose responsiveness following exposure to high FFA levels could therefore be modulation of K channel activity. It should also be noted that the molecular structure of the CoA moiety in the LC-CoA molecule bears a very close resemblance to ADP, a known stimulator of the K channel(15, 16, 17) . To test the possibility of a direct effect of LC-CoA on the K channel, we assessed regulation using single channel recordings of dispersed mouse beta-cells with the inside-out configuration of the patch-clamp technique (Fig. 1). Fig. 1A illustrates a reversible stimulatory effect of 1 µM oleoyl-CoA on K channel activity. Mean current increased 5-fold, from 0.8 to 4.4 pA in the presence of the LC-CoA. The onset of the effect was considerably faster than the recovery. Channel activity is increased by the number of open channels and also by an increased mean open time (data not shown), similar to the effect exerted by low concentrations of ADP(17, 18) . The second trace (Fig. 1B) shows a slight stimulatory effect of 100 nM oleoyl-CoA with a long lag and slow recovery in which the mean current increased approximately 2-fold from 0.6 to 1.5 pA. The kinetics of the oleoyl-CoA effects are probably related to the lipophilicity of the compound. Addition of 10 nM oleoyl-CoA (Fig. 1C) induced little effect except to possibly diminish run down of channel activity. In a previous study, we found cytosolic binding sites for LC-CoA with an estimated K(D) of approximately 1 µM(9) , suggesting that the concentrations used are physiologically relevant.


Figure 1: Effects of different concentrations of oleoyl-CoA on K channel activity in an inside-out patch shortly after patch excision. A, mean K channel current increased 5-fold from 0.8 pA (i)to 4.4 pA (i) in the presence of 1 µM oleoyl-CoA. The onset of the effect is considerably faster than the recovery. B, a slight stimulatory effect is seen following addition of 100 nM of the ester. The mean current increased approximately 2-fold, from 0.6 pA (i) to 1.5 pA (i). C, the effect of 10 nM oleoyl-CoA on K channel activity is shown. The run down of channel activity is partly reversed in the presence of 10 nM oleoyl-CoA. Mean currents i and i were found to be 0.8 and 1.1 pA, respectively.



Interaction between ATP and oleoyl-CoA was observed (Fig. 2). When 0.1 mM ATP was present continuously, a concentration that fully blocks K channel activity, 1 µM oleoyl-CoA induced a pronounced increase in channel activity (Fig. 2A). When 0.1 mM ATP was added to the bath solution one min after exposure of the patch to LC-CoA, ATP had a considerably less pronounced inhibitory effect on channel activity ( Fig. 2B). This reduced blocking effect of ATP can be explained by the slow recovery of channel activity following exposure to the LC-CoA ester, due to its lipophilicity, since after approximately five min further washing, the normal sensitivity to ATP was regained (Fig. 2B). These experiments provide compelling evidence that LC-CoA esters have the ability to prevent ATP-induced closure of the K channel, in vitro. Interestingly, they may also be involved in the suppression of glucose-induced depolarization following exposure to high levels of lipids.


Figure 2: Interactions between oleoyl-CoA and ATP on K channel activity. A, the effect of 1 µM oleoyl-CoA on K channel activity in an inside-out patch in the continuous presence of 0.1 mM ATP. B, time dependence of the effectiveness of ATP in inhibiting K channel activity following removal of LC-CoA.



The specificity for oleoyl-CoA was tested by comparing the responses with the FFA and with free CoASH. As seen in Fig. 3, no effect was observed with 1 µM oleic acid in a patch that responded to ATP and oleoyl-CoA (Fig. 3A). Likewise, no effect on K channel activity was observed when CoASH was administered, either at low (data not shown) or at high concentrations, to a patch where oleoyl-CoA induced a potent increase in mean current (Fig. 3B). Thus, the stimulatory effect of the LC acyl-CoA is dependent on both the acyl group and the CoA component. We also studied the effects of LC-CoA of different chain lengths on channel activity (Fig. 4). Stimulatory effects were seen with CoA esters of chain length 14 (Fig. 4B) and 16 carbons (Fig. 4C) but not with the 3-carbon malonyl-CoA (Fig. 4A). The effect of myristoyl-CoA (C14:0) was less pronounced than that obtained with palmitoyl-CoA (C16:0) or oleoyl-CoA (C18:1), both with regard to stimulatory ability and to recovery of the effect. These findings indicate that the K channel is a target for LC-CoA with a responsiveness to both saturated and unsaturated LC-CoA esters from C-14 to C-18 and are consistent with the suggestion that high levels of LC-CoA, such as occur in response to elevated FFA, may prevent channel closure in response to glucose. This may explain the impairment in K channel closure that has been observed in islets from the diabetic Goto-Kakizaki rat(19) .


Figure 3: Specificity for oleoyl-CoA stimulation of channel activity. A, addition of 1 µM free oleic acid to an inside-out patch did not affect K channel activity. Mean currents were estimated to be 0.9 pA (i) in the absence and 0.7 pA (i) in the presence of 1 µM oleic acid. Subsequent addition of oleoyl-CoA to the same patch resulted in an increased mean current of 4.2 pA (i). B, addition of 100 µM CoASH was without effect on K channel activity. The mean current in the absence of CoASH was estimated to be 0.4 pA (i), compared with 0.3 pA (i) in the presence of CoASH. As a control 1 µM oleoyl-CoA was added, increasing mean channel current to 3.1 pA (i).




Figure 4: Effects of different acyl-CoA chain lengths on K channel activity. A, no effect on K channel activity could be observed when 1 µM malonyl-CoA was added, mean current was estimated to be 1.2 (i) compared to 0.9 (i) pA. B, in the presence of myristoyl-CoA, channel activity increased from 0.4 pA (i) to 1.1 pA (i). C, addition of palmitoyl-CoA to the intracellular solution also affected channel activity with an estimated 4-fold increase in mean current going from 1.2 (i) to 5.1 (i) pA.



A previous report of FFA modulation of K channel activity in clonal beta-cells did not differentiate between the effects of the FFA and their metabolically active LC-CoA esters(20) . Since added FFA can be rapidly converted to LC-CoA, it is necessary to compare the FFA and LC-CoA in an excised inside-out patch, as we have done. Such studies may also reveal a more general regulatory function of LC-CoA on K channel activity in other cell types.

Fig. 5compares the effect of oleoyl-CoA on different K channels present in the beta-cell. The upper trace shows that the big conductance K channel (K), which is voltage- and Ca-dependent, is not influenced by 1 µM oleoyl-CoA in contrast to the K channel, which is activated (compare the expanded regions in Fig. 5A). The addition of 100 µM CoASH had no effect on either the K channel or the K channel. Fig. 5B shows that the 8-picosiemens K channel, described previously in the beta-cell(21) , is also unaffected by the addition of oleoyl-CoA. Hence, the ability of LC-CoA to increase K conductance seems to be specific for the K channel. These findings identify a potent new regulator of the K channel which causes up to fivefold increases in mean channel current in response to the most common LC-CoA esters(7) . This is observed at concentrations that are physiologically relevant and approximately equal to the K(D) for cytosolic binding sites for LC-CoA(9) . On a molar basis, the LC-CoA esters are approximately 100-1000 times more potent than ADP in stimulating channel activity.


Figure 5: Illustration of the specificity of oleoyl-CoA to activate the K channel. A, response to CoASH and oleoyl-CoA of K and large conductance K channel (K) currents. Whereas the activity of the K channel is clearly increased, no effect on the K channel was observed. Insets show the indicated regions of the upper trace on an expanded time scale. B, recording of the 8-picosiemens K channel in the absence and presence of 1 µM oleoyl-CoA. No effect on the 8-picosiemens channel was observed, whereas a clear effect on K channel activity is registered. Insets show the indicated regions on an expanded time scale. Arrows indicate the number of channel levels and c denotes closed.



LC-CoA esters and products formed from them have also been shown to be potent regulators of a variety of enzymes (22) and channels(20, 23) . Thus, LC-CoA inhibits glucokinase activity, stimulates endoplasmic reticulum Ca-ATPase, prevents malonyl-CoA inhibition of carnitine palmitoyl transferase-1, and inhibits acetyl-CoA carboxylase (9, 22, 24, 25, 26, 27) . The adenine nucleotide translocase, which plays an important role in controlling the cytosolic ATP/ADP ratio(26) , and the sodium pump (28, 29, 30) are stimulated by LC-CoA in some cells. Based on these opposite effects on different established targets of LC-CoA and the ability of FFA to increase the total CoA pool in beta-cells, as in other tissues(7, 11) , the net effect of LC-CoA on glucose-induced insulin secretion can be either stimulatory or inhibitory and may depend on the LC-CoA level achieved.

We find it attractive to hypothesize that elevated circulating FFA, leading to increased cellular levels of LC-CoA, play a role in the development of glucose insensitivity and that elevated glucose levels, as in tissue culture or non-insulin-dependent diabetes mellitus, exacerbate the ``toxic'' action of lipids, because high glucose inhibits fatty acid oxidation and elevates cytosolic LC-CoA levels(1) . Thus, isolated islets from 48-h lipid-infused rats display reduced glucose oxidation and insulin release in response to glucose(12) , and the insulin secretory response of islets isolated from fat-fed mice is similar to the defective secretory pattern observed in human NIDDM (31) . Furthermore, perifusion of islets for 3 h with palmitate causes impaired insulin release in response to glucose(32) . This may also be compatible with the loss of insulin responsiveness to glucose seen during starvation, a condition that leads to increased levels of FFA (33) . How long term increases in FFA impair glucose-induced insulin secretion is not known. It may be that LC-CoA inhibits the action of glucose by preventing the closure or promoting the opening of K channels as we have shown in this study.


FOOTNOTES

*
This work was supported by United States Public Health Service Grants DK35914 and DK46200, the Juvenile Diabetes Foundation International, Swedish Medical Research Council Grants 04X-09891, 03X-09890, and 19X-00034, the Swedish Diabetes Association, the Nordic Insulin Foundation, and by Funds of the Karolinska Institute, Novo Industry. The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
To whom correspondence should be addressed: Diabetes & Metabolism Unit, E-205, Boston University School of Medicine, 88 E. Newton St., Boston, MA 02118. Tel.: 617-638-7091; Fax: 617-638-7094; bcorkey{at}med-med1.bu.edu.

(^1)
The abbreviations used are: FFA, free fatty acid(s); LC-CoA, long chain acyl-CoA ester(s); K channel, ATP-sensitive K channel; K channel, voltage- and Ca-sensitive big conductance K channel.


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©1996 by The American Society for Biochemistry and Molecular Biology, Inc.