About the Authors:
Nazzareno D'Avanzo
Affiliation: Department of Cell Biology and Physiology, and Center for Investigation of Membrane Excitability Diseases, Washington University School of Medicine, St. Louis, Missouri, United States of America
Krzysztof Hyrc
Affiliation: Department of Cell Biology and Physiology, and Center for Investigation of Membrane Excitability Diseases, Washington University School of Medicine, St. Louis, Missouri, United States of America
Decha Enkvetchakul
Affiliation: Department of Pharmacological and Physiological Science, Saint Louis University School of Medicine, St. Louis, Missouri, United States of America
Douglas F. Covey
Affiliation: Department of Developmental Biology, Washington University School of Medicine, St. Louis, Missouri, United States of America
Colin G. Nichols
* E-mail: [email protected]
Affiliation: Department of Cell Biology and Physiology, and Center for Investigation of Membrane Excitability Diseases, Washington University School of Medicine, St. Louis, Missouri, United States of America
Introduction
Cholesterol is the major sterol component of all mammalian cell plasma membranes and plays a critical role in cell function and growth. Excess cholesterol is cytotoxic [1]–[3] resulting in changes in the function of various membrane proteins, including potassium (K+) channels [4]–[8], voltage-gated calcium (Cav) channels [9]–[13], voltage-gated sodium (Nav) channels [14], [15], and chloride (Cl−) channels [16], [17]. Kir channels are expressed in a wide variety of cells including skeletal, cardiac, and vascular myocytes, neurons, and pancreatic β-cells and play numerous key physiological roles including stabilizing the resting membrane potential, regulating K+ ion flux across cellular membranes, and regulation of cellular excitability [18]. Previous studies have identified cholesterol suppression of inward rectifier K+ channels (“Kir” or “KCNJ” channels) in aortic endothelial cells [8] and by heterologous expression in chinese hamster ovary (CHO) cells [7], [19], [20].
The mechanism by which cholesterol regulates Kir channels has remained elusive since, until recently, experiments could only be done in cell lines where membrane lipid compositions are undefined, difficult to manipulate quantitatively and can vary dramatically from cell to cell and with time. While the reduced inhibitory effect of the C3-diastereomer, epi-cholesterol, on KirBac1.1 activity is suggestive that cholesterol inhibition may be mediated by direct interactions [8], [21], epi-cholesterol and cholesterol orient differently in membranes and may alter membrane properties differently [22], [23]. Thus, changes in Kir channel function due to changes in the physical properties of the lipid bilayer rather than direct binding cannot be excluded based on previous studies.
We have recently shown that Saccharomyces cerevisiae can be used to express and purify human Kir channels that can be functionally reconstituted in artificial membranes of defined composition [24]–[26]. In this study, we utilize purified human Kir2.1 channels as well as two bacterial inward rectifiers (KirBac1.1 and KirBac3.1) reconstituted into liposomes with or without cholesterol. With the use of the enantiomeric cholesterol (ent-cholesterol)—which has the same effects on membrane properties as natural cholesterol [27]–[29]—we show that in both the prokaryotic and eukaryotic Kir channels the effects of cholesterol are due to direct enantioselective binding of cholesterol to the channel protein, and not an indirect effect due to changes in lipid bilayer properties. Patch-clamp analysis suggests that cholesterol may reduce channel activity by locking the channels into prolonged closed states.
Methods
Human Kir2.1 Protein Purification
A Kir2.1-FLAG-His8 fusion protein (∼51.5 kDa per monomer) was expressed and purified from the FGY217 strain of Saccharomyces cerevisiae as previously described [24]–[26].
KirBac1.1 Purification
A KirBac1.1-His6 fusion protein (∼38.8 kDa per monomer) was expressed and purified from the BL21*(DE3) E. coli strain as previously described [30]. Briefly, cells were grown in 1L cultures and induced with 0.5 mM IPTG at OD600∼1 for 3 hrs at 37°C. Cells were pelleted and resuspended in 50 mM Tris-HCl pH 8.0, 150 mM KCl, and Complete EDTA-free protease inhibitor tablets (Roche Diagnostics). Cells were lysed by high pressure (20–25 kpsi) homogenization using a Microfluidics Cell Disrupter and solubilized with 30 mM DM for 2 hrs at room temperature. Following centrifugation at 30,000× g for 30 mins, the supernatant was applied to a cobalt affinity column, washed with 20–30 column volumes of wash buffer (50 mM Tris pH 8.0, 150 mM KCl, 10 mM imidazole, and 5 mM DM) and eluted with 1–2 mL of wash buffer containing 500 mM imidazole.
KirBac3.1 Purification
BL21 CodonPlus RP cells were transformed and grown at 37°C in a shaker to OD600∼0.5 then grown at 19°C until an OD600∼1.0, followed by induction of KirBac3.1 protein (∼33.7 kDa per monomer) expression with 1 mM IPTG. After 16 hours, cells were harvested by centrifugation, the pellet resuspended in 50 mM Tris-HCl 7.8, 100 mM NaCl, 10 mM KCl , and Complete EDTA-free protease inhibitor tablets (Roche). The resuspended cells were passed through a Parr cell disruptor 5 times, and then centrifuged at 10,000 g for 15 minutes to remove cell debris. Gycerol (26% v/v final) and decylmaltoside (37 mM final) were added to the supernatant and rocked at room tempearture for 3 hours. The mixture was then centrifuged at 10,000 g, for 40 minutes, and the supernatant was mixed with cobalt affinity beads (Talon) for 2 hours. The beads were washed in a disposable plastic column with ∼20 bed volumes of wash buffer (50 mm Tris-HCl, pH 8.0, 100 mm NaCl, 10 mM KCl, 2 mM tridecylmaltoside) and eluted with wash buffer containing 400 mm imidazole.
Synthesis of Enantiomeric Cholesterol
ent-cholesterol, the enantiomer of cholesterol, was synthesized as previously described [31].
86Rb+ Uptake Assay
POPE (1-palmitoyl-2-oleoyl-3-phosphatidylethanolamine) and POPG (1-palmitoyl-2-oleoyl-3-phosphatidylglycerol), cholesterol, and PI(4,5)P2 (phosphatidylinositol 4,5-bisphosphate from porcine brain) (Avanti Polar Lipids, Inc.) were solubilized in chloroform, mixed together in the desired concentrations, and dried into a thin film in glass tubes under a nitrogen stream. These lipids were then solubilized in buffer A (450 mM KCl, 10 mM HEPES, 4 mM N-methyl-D-Glucamine, pH 7.5) with 35 mM CHAPS at 10 mg/ml, mixed at the desired mass ratio, and incubated at room temperature for 2 h. Thus, when required, cholesterol was included in the liposomes at the time of formation. Polystyrene columns (Pierce Chemical Co.) were packed with Sephadex G-50 beads, presoaked overnight in buffer A, and spun on a Beckman TJ6 centrifuge until reaching 3,000 rpm. For each sample, 3 µg of protein was added to 100 µl of lipid (1 mg) and incubated for 30 min. Proteo-liposomes were formed by adding the protein/lipid sample to the partially dehydrated columns and centrifuging to 2,500 rpm [24], [25], [32], [33]. The extra-liposomal solution was exchanged by centrifuging the liposomes to 2,500 rpm in partially-dehydrated columns, now containing beads soaked in buffer B (400 mM sorbitol, 10 mM HEPES, 4 mM NMG, pH 7.5). 86Rb+ uptake was initiated by adding 400 µl of buffer B containing 86Rb+. At various time points, aliquots of the liposome uptake reaction were flowed through 0.5 ml Dowex cation exchange columns in the NMGH+ form to remove extraliposomal 86Rb+. These aliquots were then mixed with scintillation fluid and counted in a liquid scintillation counter. Valinomycin was used to measure maximal 86Rb+ uptake. Data were subtracted from uptake counts measured at each time point from protein-free liposomes, and plotted relative to valinomycin-induced uptake counts.
Electrophysiology of human Kir2.1 in Giant Liposomes
Giant liposomes were prepared in a similar manner as previously described for KirBac1.1 [32]. Briefly, POPE, POPG and PI(4,5)P2 were solubilized in K-MOPS buffer (10 mM MOPS acid, pH 7.4, 150 mM KCl) and 35 mM CHAPS and mixed at a 3∶1∶0.04 ratio (a total of 2 mg). Polystyrene columns (Pierce Chemical Co.) were packed with Sephadex G-50 beads, presoaked overnight in K-MOPS buffer, and spun on a Beckman TJ6 centrifuge until reaching 3,000 rpm. Purified Kir2.1 protein was added to the lipids at lipid to protein mass ratio of 33∶1 and incubated at room temperature for 30 min. Proteo-liposomes were formed by adding the protein/lipid sample to the partially-dehydrated columns and spinning to 2,500 rpm, and centrifuged at 100,000 g for 1 h at 4°C (TL-100; Beckman Coulter). The liposome pellet was resuspended in 2–3 µl K-MOPS buffer and dried in a desiccator as 2 µl spots on a clean microscope slide for ∼1 h or until completely dried. These spots were then rehydrated with 20 µl K-MOPS buffer overnight at 4°C. Rehydration at room temperature for ∼2 h the next day was sufficient to form giant liposomes.
For patch-clamp, the giant proteo-liposomes were pipetted onto a glass cover slip in an oil-gate chamber [34] and allowed to settle for ∼5 min before starting the solution exchange to wash away debris. Patch-clamp recordings were performed in symmetrical conditions of K-MOPS buffer. Membrane patches were voltage-clamped using a CV-4 headstage, an Axopatch 1-D amplifier, and a Digidata 1322A digitizer board (MDS Analytical Technologies). Patch pipettes were pulled from soda lime glass microhematocrit tubes (Kimble) to a resistance of ∼1–3 MΩ. Single-channel data were digitized at a sampling rate of 10 kHz, and a low-pass analogue filter was set to 1 kHz. Single-channel amplitude histograms were performed using the pClamp 9.2 software suite (MDS Analytical Technologies). The remaining data analysis was performed using Origin7.0 (Microcal).
Confocal Microscopy
Giant liposomes were formed as above, in the presence or absence of 5% NBD-cholesterol (chemical nomenclature: 22-(N-(7-nitrobenz-2-oxa-1,3-diazol-4-yl)amino)-23,24-bisnor-5-cholen-3β-ol) (Invitrogen). Confocal microscopy was performed using a Zeiss LSM5 Pascal confocal microscope (Zeiss Microimaging, ThornwooD, NY) with a H10×/0.3 Plan-NeoFluar lens (Zeiss). Fluorescence was excited using 488 nm Argon laser line (Lasos, Jena, Germany) and emission was collected using a 505 LP filter (Chroma, Brattleboro, VT). Simultaneously, we collected transmitted light images. Image acquisition and analysis was carried out using Zeiss AIM software.
Statistical Analysis
Statistical significance was analyzed using an unpaired T-test or one-way ANOVA with Tukey post-hoc analysis as appropriate, and statistical significance (P<0.05) is indicated by an asterisk.
Results
Cholesterol Inhibits Purified Prokaryotic and Eukaryotic Inward Rectifier K+ Channels
Bacterial inwardly rectifying K+ channels (KirBac1.1 and KirBac3.1) were expressed and purified from E. coli, while human Kir2.1 channels were expressed and purified from S. cerevisiae. By incorporating these channels into liposomes, previous studies have shown that these proteins form functional K+ channels [24]–[26], [30], [32], [35], and that KirBac1.1-mediated 86Rb+ flux is readily suppressed by the addition of cholesterol to 9∶1 POPE∶POPG liposomes [21]. Here we confirm these results (Fig. 1A and B). In addition, we also show that both KirBac3.1 and human Kir2.1 channel activity are suppressed in liposomes containing as little as 1% cholesterol (mg/mg total lipids) (Fig. 1A and B). Inhibition of channel activity increased in a concentration-dependent manner (Fig. 1B). Notably, cholesterol could not be incorporated into liposomes at concentrations higher than 10%, as indicated by the formation of a heavy precipitate. Interestingly, in this assay, the levels of cholesterol which have an inhibitory effect on Kir channels are well below those typically found in plasma membranes of mammalian cells (between 30–50% of total membrane lipids [2], [3]). However, the degree of inhibition is similar to that previously reported for KirBac1.1 [21]. Importantly, these results show that regulation of Kir channels does not require an intermediary protein that is sensitive to cholesterol.
[Figure omitted. See PDF.]
Figure 1. Cholesterol inhibits activity of reconstituted KirBac1.1, KirBac3.1 and human Kir2.1.
(A) Representative time course of 86Rb+ uptake into 9∶1 POPE∶POPG liposomes (+1% PI(4,5)P2 for Kir2.1) containing increasing amounts of cholesterol reconstituted (0% = ▪; 1% = •; 5% = ▴; 10% = ▾) with KirBac1.1 (left), KirBac3.1 (middle), or Kir2.1 (right) protein, incubated with 450 mM internal and 0 mM external [K+]. Uptake was normalized to valinomycin-induced uptake in the same liposomes. (B) Channel activity-cholesterol relationship obtained from 86Rb+ uptake at 240 s for KirBac1.1 (blue; n = 7±s.e.m), at 90 mins for KirBac3.1 (green; n = 6±s.e.m) and at 60 mins for human Kir2.1 (red; n = 6±s.e.m) for each cholesterol concentration. The data are renormalized to uptake in liposomes containing 0% cholesterol. (C) 86Rb+ uptake from KirBac1.1 (blue) and Kir2.1 (red) channels reconstituted into liposomes containing 25% POPG (+1% PI(4,5)P2 for Kir2.1) ±5% cholesterol on a POPE background (n = 8 for each). The data were normalized to valinomycin-induced uptake in the same liposomes and re-normalized to uptake in liposomes containing 0% cholesterol. (* P<0.05 assessed by ANOVA).
https://doi.org/10.1371/journal.pone.0019393.g001
We previously showed that Kir2.1 channels require anionic phospholipids in addition to PI(4,5)P2 for channel activity [24]. Conceivably cholesterol may compete directly or allosterically with POPG to reduce channel activity. Thus, cholesterol inhibition of Kir2.1 and KirBac1.1 channels was also assessed by 86Rb+ flux in liposomes containing elevated (25%) POPG (Fig. 1C). This does not appear to be the mechanism for cholesterol inhibition, since cholesterol still inhibited KirBac1.1 or Kir2.1 channels in proteo-liposomes containing 25% POPG (Fig. 1C) similarly to channels in proteo-liposomes containing only 10% POPG.
Cholesterol Does Not Alter Measurable Open Probability or Unitary Conductance in Kir2.1
To examine what property of Kir channel function is affected by the presence of cholesterol in the membrane, single-channel recordings were performed by reconstituting human Kir2.1 channels into POPE∶POPG giant liposomes containing 1% PI(4,5)P2 and either 0% or 5% cholesterol (Fig. 2A). We find empirically that giant liposomes cannot be formed under the 10% POPG condition used above. Thus, we generated giant liposomes with higher (25%) POPG on a POPE background for these experiments (ie. 25% POPG, 1% PI(4,5)P2, 74% POPE or 71% POPE+5% Cholesterol). In the absence of cholesterol, Kir2.1 channels exhibited a unitary conductance of 36.1±1.5 pS and a Popen of 0.35±0.01 (n = 8 patches each). In giant liposomes containing 5% cholesterol, no difference was observed in either the measured unitary conductance (33.9±2.9 pS; P = 0.49) (Fig. 2B) or Popen (0.34±0.02; P = 0.68) (Fig. 2C) (n = 7). These results cannot explain the inhibitory effect observed under identical conditions in flux experiments data, so to ensure that these results truly reflected single-channel behaviour, and not an inability to incorporate cholesterol into giant liposomes, we made giant liposomes in the presence of a fluorescent analogue of cholesterol (NBD-cholesterol) (Fig. 3). With excitation by 488 nm light, no fluorescence was observed from giant liposomes formed in the absence of cholesterol (Fig. 3 top), but robust fluorescence was detected from liposomes containing 5% NBD-cholesterol (Fig. 3 bottom), indicating that the patch-clamp experiments are not limited by the ability to incorporate cholesterol into giant liposomes.
[Figure omitted. See PDF.]
Figure 2. Cholesterol does not affect Kir2.1 open probability or unitary conductance.
(A) Representative single-channel recordings from human Kir2.1 channels reconstituted into 3∶1 POPE∶POPG giant liposomes at −100 mV in the absence (left) or presence (right) of 5% cholesterol. Neither the unitary conductance (i) – voltage (V) relationships (B; P = 0.49, n = 8) nor open probability (C; P = 0.68, n = 7) were significantly different for human Kir2.1 channels reconstituted into liposomes containing 0% (▪) or 5% (□) cholesterol.
https://doi.org/10.1371/journal.pone.0019393.g002
[Figure omitted. See PDF.]
Figure 3. Cholesterol is present in giant liposomes.
Giant liposomes were made with 3∶1 POPE∶POPG and 0% or 5% NBD-Cholesterol. Giant liposomes formed without NBD-cholesterol showed no emission above 505 nm following excitation at 488 nm. Robust fluorescence was observed for giant liposomes made in the presence of 5% NBD-cholesterol.
https://doi.org/10.1371/journal.pone.0019393.g003
Thus, our electrophysiological results do in fact reflect Kir2.1 single-channel behaviour, and support the idea that cholesterol may act to cause long-term “silencing” of channels by inducing prolonged closed states. One consequence of such a mechanism would be a reduction in the “observed” average number of channels in each patch with the inclusion of cholesterol in the membranes. Although not statistically significant, this appears to be the trend: we detected 6.7±1.8 channels per active patch (range = 1–14 channels/patch) in the absence of cholesterol, versus 4.2±1.8 channels per patch (1–10 channels/active patch) in the presence of 5% cholesterol (P = 0.29; n = 7 and n = 6 respectively). Power analysis indicates that for 80% power, data from more than 85 patches would have to be collected to determine if this trend is significant. Given the cost of protein purifications, and the variability of the patches, we have not attempted to perform this number of experiments.
Enantiospecific Binding of Cholesterol to Prokaryotic and Eukaryotic Inward Rectifier K+ Channels
Cholesterol can act to alter the function of membrane proteins either through direct binding or indirectly through changes in membrane fluidity, stiffness, thickness, permeability and/or phospholipid packing [2], [3], [36]–[41]. To distinguish between these possible mechanisms for cholesterol effects on Kir channel function we utilized the enantiomer of cholesterol (ent-cholesterol), which has the same effects on membrane properties as cholesterol [27], [28], [42], yet cannot interact identically with the anisotropic structure of proteins. By comparing the effect of either 5% cholesterol or ent-cholesterol on 86Rb+ uptake we show that the effect of cholesterol on KirBac1.1, KirBac3.1 and human Kir2.1 channel activity is enantioselective (Fig. 4A and B). This differential effect of cholesterol and ent-cholesterol on prokaryotic and eukaryotic inward rectifier K+ channels implies that in these channels, cholesterol inhibition depends on enantiospecific protein-sterol interactions, rather than on indirect changes of the physical properties of the lipid bilayer.
[Figure omitted. See PDF.]
Figure 4. Cholesterol enantiospecifically binds prokaryotic and eukaryotic Kir channels.
(A) Representative time course of 86Rb+ uptake into 9∶1 POPE∶POPG liposomes (+1% PI(4,5)P2 for Kir2.1) containing 0% cholesterol (▪), 5% cholesterol (•) or 5% ent-cholesterol (▴) reconstituted with KirBac1.1 (left), KirBac3.1 (middle), or Kir2.1 (right) protein, with 450 mM internal and 0 mM external [K+]. (B) KirBac1.1 (blue), KirBac3.1 (green) and human Kir2.1 (red) channel activity-cholesterol relationship obtained from 86Rb+ uptake counts. The data are renormalized to uptake in liposomes containing 0% cholesterol. (n = 6 for each protein, * P<0.05 assessed by ANOVA).
https://doi.org/10.1371/journal.pone.0019393.g004
Discussion
A growing number of ion channels have been shown to be regulated by components of the lipid membranes [4]–[8], [10], [11], [13], [19]–[21], and previous studies have indicated that cholesterol can inhibit both mammalian and bacterial Kir channel currents [7], [19], [20]. Here, we have shown that in POPE/POPG liposomes, containing prokaryotic KirBac1.1, KirBac3.1 or human Kir2.1 are similarly modulated by as little as 1% cholesterol (mg/mg total lipids). This is in stark contrast to the opposing effects of PI(4,5)P2 on prokaryotic and eukaryotic Kirs [25], [35]. Interestingly, the levels of cholesterol necessary to regulate Kir2.1 channels are well below the levels reported in plasma membranes of mammalian cells, which range between 30–50% of total membrane lipids [2], [3].
Effects of sterols on lipid membrane properties generally show no entantioselectivity. In particular, no enantioselective effects on phase-transition properties [42] and lipid packing in monolayers, and on bilayer properties as measured by calorimetrey, X-ray diffraction, and neutron density measurements have been reported between cholesterol and ent-cholesterol [27]. On the other hand, studies with enzymes and transporters that use cholesterol as a substrate demonstrate a high entantiomer selectivity of interaction [43], [44], while lipid domain forming peptides have also been shown to have differential interactions with cholesterol entantiomers [42]. Thus, the differential actions of cholesterol versus ent-cholesterol on protein function reflect the existence of direct protein-sterol interactions [27]–[29].
Previous studies have attempted to address whether the regulation of Kir channel function results from direct channel-sterol interactions or indirect effects such as changes to the physical properties of the lipid bilayer or regulation by an intermediary cholesterol-sensitive protein through the use of the C3-diastereomer, epi-cholesterol [8], [21]. Epi-cholesterol inhibited KirBac1.1 channels less than the equivalent amount of cholesterol [8], [21]. Partial substitution of cholesterol with epi-cholesterol in mammalian cells resulted in an increase in current relative to control, which may suggest specific protein-sterol interactions [8], [21]. However, the interpretation of such studies is not trivial since (a) mediation through accessory proteins cannot be excluded from recordings done in eukaryotic cell membranes and (b) epi- and natural cholesterol orient differently in membranes, and can thus alter membrane properties differently [22], [23]. No enantioselectivity has been observed for cholesterol effects on various lipid bilayer and monolayer properties [27], [28]. Thus, determining the enantioselectivity of purified channel regulation by cholesterol with the use of ent-cholesterol is a more suitable approach. This assay has been used to determine the enantioselectivity of cholesterol regulation of numerous channels and receptors (for complete list see review by Covey, 2009 [45]), including a recent study of calcium-activated BK channels [46]. Using this assay, we observed that both prokaryotic and eukaryotic Kir channels are indeed enantioselective for cholesterol, indicating that modulation by this sterol is mediated by direct binding to the channel. Since the degree of channel modulation by cholesterol is similar between prokaryotic and eukaryotic Kir channels and since cholesterol is not present in prokaryotic membranes [47], we speculate that modulation of eukaryotic Kirs by cholesterol utilizes a conserved “binding pocket” also found in prokaryotic Kirs. It has been previously suggested that cholesterol may bind to Kir channels in a confirmation that requires the cytoplasmic domain to be close to the membrane [48] and that this confirmation may be favored when residue 222 in Kir2.1 channels is a leucine, and unfavourable when isoleucine [48]. Although KirBac channels do not have leucine at the equivalent position, comparison of the eukaryotic and bacterial channel structures indicates that the cytoplasmic domains of KirBac channels are already closer to the bilayer than eukaryotic Kir channels [49] and may be already close enough to interact with cholesterol.
Unitary conductances and open probabilities were not significantly different for human Kir2.1 in the presence or absence of cholesterol in liposomes containing 25% POPG. The presence of cholesterol in giant liposomes under these conditions was verified using fluorescent NBD-cholesterol (Fig. 3). Similarly, despite decreases in whole-cell currents, no changes in single-channel properties were reported for either IK1 in bovine aortic endothelial cells or for Kir2.1 currents over-expressed in CHO cells treated with MβCD-cholesterol [7], [8]. We show that increasing POPG concentration does not alter cholesterol inhibition of Kir2.1 or KirBac1.1 channels (Fig. 1C), and thus cannot account for the discrepancy between flux experiments where cholesterol reduced channel activity by ∼45% (Fig. 1) and our patch clamp experiments on giant liposomes where no effect on channel conductance or Popen were observed (Fig. 2). Together with our observation that cholesterol binds directly to Kir channels, these data support the idea that when bound, cholesterol induces conformational changes that lead to a prolonged closed state that cannot be detected by single-channel analysis [7]. Consequently, we are only able to detect single-channel currents from proteins not interacting with cholesterol.
Author Contributions
Conceived and designed the experiments: ND DFC CGN. Performed the experiments: ND KH. Analyzed the data: ND. Contributed reagents/materials/analysis tools: DE DFC CGN. Wrote the paper: ND KH DE DFC CGN.
Citation: D'Avanzo N, Hyrc K, Enkvetchakul D, Covey DF, Nichols CG (2011) Enantioselective Protein-Sterol Interactions Mediate Regulation of Both Prokaryotic and Eukaryotic Inward Rectifier K+ Channels by Cholesterol. PLoS ONE6(4): e19393. https://doi.org/10.1371/journal.pone.0019393
1. Kellner-Weibel G, Geng YJ, Rothblat GH (1999) Cytotoxic cholesterol is generated by the hydrolysis of cytoplasmic cholesteryl ester and transported to the plasma membrane. Atherosclerosis 146(2): 309–19.G. Kellner-WeibelYJ GengGH Rothblat1999Cytotoxic cholesterol is generated by the hydrolysis of cytoplasmic cholesteryl ester and transported to the plasma membrane.Atherosclerosis146230919
2. Yeagle PL (1985) Cholesterol and the cell membrane. Biochim Biophys Acta 822(3–4): 267–87.PL Yeagle1985Cholesterol and the cell membrane.Biochim Biophys Acta8223–426787
3. Yeagle PL (1991) Modulation of membrane function by cholesterol. Biochimie 73(10): 1303–10.PL Yeagle1991Modulation of membrane function by cholesterol.Biochimie7310130310
4. Bolotina V, Omelyanenko V, Heyes B, Ryan U, Bregestovski P (1989) Variations of membrane cholesterol alter the kinetics of Ca2(+)-dependent K+ channels and membrane fluidity in vascular smooth muscle cells. Pflugers Arch 415(3): 262–8.V. BolotinaV. OmelyanenkoB. HeyesU. RyanP. Bregestovski1989Variations of membrane cholesterol alter the kinetics of Ca2(+)-dependent K+ channels and membrane fluidity in vascular smooth muscle cells.Pflugers Arch41532628
5. Heaps CL, Tharp DL, Bowles DK (2005) Hypercholesterolemia abolishes voltage-dependent K+ channel contribution to adenosine-mediated relaxation in porcine coronary arterioles. Am J Physiol Heart Circ Physiol 288(2): H568–76.CL HeapsDL TharpDK Bowles2005Hypercholesterolemia abolishes voltage-dependent K+ channel contribution to adenosine-mediated relaxation in porcine coronary arterioles.Am J Physiol Heart Circ Physiol2882H56876
6. Martens JR, Navarro-Polanco R, Coppock EA, Nishiyama A, Parshley L, et al. (2000) Differential targeting of Shaker-like potassium channels to lipid rafts. J Biol Chem 275(11): 7443–6.JR MartensR. Navarro-PolancoEA CoppockA. NishiyamaL. Parshley2000Differential targeting of Shaker-like potassium channels to lipid rafts.J Biol Chem2751174436
7. Romanenko VG, Fang Y, Byfield F, Travis AJ, Vandenberg CA, et al. (2004) Cholesterol sensitivity and lipid raft targeting of Kir2.1 channels. Biophys J 87(6): 3850–61.VG RomanenkoY. FangF. ByfieldAJ TravisCA Vandenberg2004Cholesterol sensitivity and lipid raft targeting of Kir2.1 channels.Biophys J876385061
8. Romanenko VG, Rothblat GH, Levitan I (2002) Modulation of endothelial inward-rectifier K+ current by optical isomers of cholesterol. Biophys J 83(6): 3211–22.VG RomanenkoGH RothblatI. Levitan2002Modulation of endothelial inward-rectifier K+ current by optical isomers of cholesterol.Biophys J836321122
9. Ambudkar IS (2004) Cellular domains that contribute to Ca2+ entry events. Sci STKE 2004(243): pe32.IS Ambudkar2004Cellular domains that contribute to Ca2+ entry events.Sci STKE2004243pe32
10. Bowles DK, Heaps CL, Turk JR, Maddali KK, Price EM (2004) Hypercholesterolemia inhibits L-type calcium current in coronary macro-, not microcirculation. J Appl Physiol 96(6): 2240–8.DK BowlesCL HeapsJR TurkKK MaddaliEM Price2004Hypercholesterolemia inhibits L-type calcium current in coronary macro-, not microcirculation.J Appl Physiol96622408
11. Lockwich TP, Liu X, Singh BB, Jadlowiec J, Weiland S, et al. (2000) Assembly of Trp1 in a signaling complex associated with caveolin-scaffolding lipid raft domains. J Biol Chem 275(16): 11934–42.TP LockwichX. LiuBB SinghJ. JadlowiecS. Weiland2000Assembly of Trp1 in a signaling complex associated with caveolin-scaffolding lipid raft domains.J Biol Chem275161193442
12. Lundbaek JA, Birn P, Girshman J, Hansen AJ, Andersen OS (1996) Membrane stiffness and channel function. Biochemistry 35(12): 3825–30.JA LundbaekP. BirnJ. GirshmanAJ HansenOS Andersen1996Membrane stiffness and channel function.Biochemistry3512382530
13. Toselli M, Biella G, Taglietti V, Cazzaniga E, Parenti M (2005) Caveolin-1 expression and membrane cholesterol content modulate N-type calcium channel activity in NG108-15 cells. Biophys J 89(4): 2443–57.M. ToselliG. BiellaV. TagliettiE. CazzanigaM. Parenti2005Caveolin-1 expression and membrane cholesterol content modulate N-type calcium channel activity in NG108-15 cells.Biophys J894244357
14. Lundbaek JA, Birn P, Hansen AJ, Sogaard R, Nielsen C, et al. (2004) Regulation of sodium channel function by bilayer elasticity: the importance of hydrophobic coupling. Effects of Micelle-forming amphiphiles and cholesterol. J Gen Physiol 123(5): 599–621.JA LundbaekP. BirnAJ HansenR. SogaardC. Nielsen2004Regulation of sodium channel function by bilayer elasticity: the importance of hydrophobic coupling. Effects of Micelle-forming amphiphiles and cholesterol.J Gen Physiol1235599621
15. Wu CC, Su MJ, Chi JF, Chen WJ, Hsu HC, et al. (1995) The effect of hypercholesterolemia on the sodium inward currents in cardiac myocyte. J Mol Cell Cardiol 27(6): 1263–9.CC WuMJ SuJF ChiWJ ChenHC Hsu1995The effect of hypercholesterolemia on the sodium inward currents in cardiac myocyte.J Mol Cell Cardiol27612639
16. Levitan I, Christian AE, Tulenko TN, Rothblat GH (2000) Membrane cholesterol content modulates activation of volume-regulated anion current in bovine endothelial cells. J Gen Physiol 115(4): 405–16.I. LevitanAE ChristianTN TulenkoGH Rothblat2000Membrane cholesterol content modulates activation of volume-regulated anion current in bovine endothelial cells.J Gen Physiol115440516
17. Romanenko VG, Rothblat GH, Levitan I (2004) Sensitivity of volume-regulated anion current to cholesterol structural analogues. J Gen Physiol 123(1): 77–87.VG RomanenkoGH RothblatI. Levitan2004Sensitivity of volume-regulated anion current to cholesterol structural analogues.J Gen Physiol12317787
18. Hille B (2001) Ion Channels of Excitable Membranes. Third ed. Sunderland: Sinauer Assiciates Inc. B. Hille2001Ion Channels of Excitable Membranes. Third edSunderlandSinauer Assiciates Inc
19. Rosenhouse-Dantsker A, Leal-Pinto E, Logothetis DE, Levitan I (2010) Comparative analysis of cholesterol sensitivity of Kir channels: role of the CD loop. Channels (Austin) 4(1): 63–6.A. Rosenhouse-DantskerE. Leal-PintoDE LogothetisI. Levitan2010Comparative analysis of cholesterol sensitivity of Kir channels: role of the CD loop.Channels (Austin)41636
20. Tikku S, Epshtein Y, Collins H, Travis AJ, Rothblat GH, et al. (2007) Relationship between Kir2.1/Kir2.3 activity and their distributions between cholesterol-rich and cholesterol-poor membrane domains. Am J Physiol Cell Physiol 293(1): C440–50.S. TikkuY. EpshteinH. CollinsAJ TravisGH Rothblat2007Relationship between Kir2.1/Kir2.3 activity and their distributions between cholesterol-rich and cholesterol-poor membrane domains.Am J Physiol Cell Physiol2931C44050
21. Singh DK, Rosenhouse-Dantsker A, Nichols CG, Enkvetchakul D, Levitan I (2009) Direct regulation of prokaryotic Kir channel by cholesterol. J Biol Chem 284(44): 30727–36.DK SinghA. Rosenhouse-DantskerCG NicholsD. EnkvetchakulI. Levitan2009Direct regulation of prokaryotic Kir channel by cholesterol.J Biol Chem284443072736
22. Cadenhead DA, Mueller-Landau F (1979) Molecular packing in steroid-lecithin monolayers. Part III. Mixed films of 3-doxy cholestane and 3-doxyl-17-hydroxylandrostane with dipalmitoylphosphatidycholine. Chem Phys Lipids 25: 329–43.DA CadenheadF. Mueller-Landau1979Molecular packing in steroid-lecithin monolayers. Part III. Mixed films of 3-doxy cholestane and 3-doxyl-17-hydroxylandrostane with dipalmitoylphosphatidycholine.Chem Phys Lipids2532943
23. Murari R, Murari MP, Baumann WJ (1986) Sterol orientations in phosphatidylcholine liposomes as determined by deuterium NMR. Biochemistry 25(5): 1062–7.R. MurariMP MurariWJ Baumann1986Sterol orientations in phosphatidylcholine liposomes as determined by deuterium NMR.Biochemistry25510627
24. Cheng WW, D'Avanzo N, Doyle DA, Nichols CG (2011) Dual-Mode Phospholipid Regulation of Human Inward Rectifying Potassium Channels. Biophys J 100(3): 620–8.WW ChengN. D'AvanzoDA DoyleCG Nichols2011Dual-Mode Phospholipid Regulation of Human Inward Rectifying Potassium Channels.Biophys J10036208
25. D'Avanzo N, Cheng WW, Doyle DA, Nichols CG (2010) Direct and specific activation of human inward rectifier K+ channels by membrane phosphatidylinositol 4,5-bisphosphate. J Biol Chem 285(48): 37129–32.N. D'AvanzoWW ChengDA DoyleCG Nichols2010Direct and specific activation of human inward rectifier K+ channels by membrane phosphatidylinositol 4,5-bisphosphate.J Biol Chem285483712932
26. D'Avanzo N, Cheng WW, Xia X, Dong L, Savitsky P, et al. (2010) Expression and purification of recombinant human inward rectifier K+ (KCNJ) channels in Saccharomyces cerevisiae. Protein Expr Purif 71(1): 115–21.N. D'AvanzoWW ChengX. XiaL. DongP. Savitsky2010Expression and purification of recombinant human inward rectifier K+ (KCNJ) channels in Saccharomyces cerevisiae.Protein Expr Purif71111521
27. Mannock DA, McIntosh TJ, Jiang X, Covey DF, McElhaney RN (2003) Effects of natural and enantiomeric cholesterol on the thermotropic phase behavior and structure of egg sphingomyelin bilayer membranes. Biophys J 84(2 Pt 1): 1038–46.DA MannockTJ McIntoshX. JiangDF CoveyRN McElhaney2003Effects of natural and enantiomeric cholesterol on the thermotropic phase behavior and structure of egg sphingomyelin bilayer membranes.Biophys J842 Pt 1103846
28. Westover EJ, Covey DF (2003) First synthesis of ent-desmosterol and its conversion to ent-deuterocholesterol. Steroids 68(2): 159–66.EJ WestoverDF Covey2003First synthesis of ent-desmosterol and its conversion to ent-deuterocholesterol.Steroids68215966
29. Alakoskela JM, Sabatini K, Jiang X, Laitala V, Covey DF, et al. (2008) Enantiospecific interactions between cholesterol and phospholipids. Langmuir 24(3): 830–6.JM AlakoskelaK. SabatiniX. JiangV. LaitalaDF Covey2008Enantiospecific interactions between cholesterol and phospholipids.Langmuir2438306
30. Enkvetchakul D, Bhattacharyya J, Jeliazkova I, Groesbeck DK, Cukras CA, et al. (2004) Functional characterization of a prokaryotic Kir channel. J Biol Chem 279(45): 47076–80.D. EnkvetchakulJ. BhattacharyyaI. JeliazkovaDK GroesbeckCA Cukras2004Functional characterization of a prokaryotic Kir channel.J Biol Chem279454707680
31. Jiang X, Covey DF (2002) Total synthesis of ent-cholesterol via a steroid C,D-ring side-chain synthon. J Org Chem 67(14): 4893–900.X. JiangDF Covey2002Total synthesis of ent-cholesterol via a steroid C,D-ring side-chain synthon.J Org Chem67144893900
32. Cheng WW, Enkvetchakul D, Nichols CG (2009) KirBac1.1: it's an inward rectifying potassium channel. J Gen Physiol 133(3): 295–305.WW ChengD. EnkvetchakulCG Nichols2009KirBac1.1: it's an inward rectifying potassium channel.J Gen Physiol1333295305
33. Nimigean CM (2006) A radioactive uptake assay to measure ion transport across ion channel-containing liposomes. Nat Protoc 1(3): 1207–12.CM Nimigean2006A radioactive uptake assay to measure ion transport across ion channel-containing liposomes.Nat Protoc13120712
34. Lederer WJ, Nichols CG (1989) Nucleotide modulation of the activity of rat heart ATP-sensitive K+ channels in isolated membrane patches. J Physiol 419: 193–211.WJ LedererCG Nichols1989Nucleotide modulation of the activity of rat heart ATP-sensitive K+ channels in isolated membrane patches.J Physiol419193211
35. Enkvetchakul D, Jeliazkova I, Nichols CG (2005) Direct modulation of Kir channel gating by membrane phosphatidylinositol 4,5-bisphosphate. J Biol Chem 280(43): 35785–8.D. EnkvetchakulI. JeliazkovaCG Nichols2005Direct modulation of Kir channel gating by membrane phosphatidylinositol 4,5-bisphosphate.J Biol Chem28043357858
36. Demel RA, De Kruyff B (1976) The function of sterols in membranes. Biochim Biophys Acta 457(2): 109–32.RA DemelB. De Kruyff1976The function of sterols in membranes.Biochim Biophys Acta457210932
37. Evans E, Needham D (1987) Physical properties of surfactant bilayer membranes: thermal transtions, elasticity, rigidity, cohesion, and colloidal interactions. J Phys chem 91: 4219–4228.E. EvansD. Needham1987Physical properties of surfactant bilayer membranes: thermal transtions, elasticity, rigidity, cohesion, and colloidal interactions.J Phys chem9142194228
38. Gidwani A, Holowka D, Baird B (2001) Fluorescence anisotropy measurements of lipid order in plasma membranes and lipid rafts from RBL-2H3 mast cells. Biochemistry 40(41): 12422–9.A. GidwaniD. HolowkaB. Baird2001Fluorescence anisotropy measurements of lipid order in plasma membranes and lipid rafts from RBL-2H3 mast cells.Biochemistry4041124229
39. Kahya N, Schwille P (2006) Fluorescence correlation studies of lipid domains in model membranes. Mol Membr Biol 23(1): 29–39.N. KahyaP. Schwille2006Fluorescence correlation studies of lipid domains in model membranes.Mol Membr Biol2312939
40. Needham D, Nunn RS (1990) Elastic deformation and failure of lipid bilayer membranes containing cholesterol. Biophys J 58(4): 997–1009.D. NeedhamRS Nunn1990Elastic deformation and failure of lipid bilayer membranes containing cholesterol.Biophys J5849971009
41. Yeagle PL (1985) “The biophysics and cell biology of cholesterol: An hypothesis for the essential role of cholesterol in mammalian cells” in Cholesterol in Membrane Models. pp. 1–10.PL Yeagle1985“The biophysics and cell biology of cholesterol: An hypothesis for the essential role of cholesterol in mammalian cells” in Cholesterol in Membrane Models.110CRC Press. Boca Raton. CRC Press. Boca Raton.
42. Epand RM, Rychnovsky SD, Belani JD, Epand RF (2005) Role of chirality in peptide-induced formation of cholesterol-rich domains. Biochem J 390(Pt 2): 541–8.RM EpandSD RychnovskyJD BelaniRF Epand2005Role of chirality in peptide-induced formation of cholesterol-rich domains.Biochem J390Pt 25418
43. Liu J, Chang CC, Westover EJ, Covey DF, Chang TY (2005) Investigating the allosterism of acyl-CoA:cholesterol acyltransferase (ACAT) by using various sterols: in vitro and intact cell studies. Biochem J 391(Pt 2): 389–97.J. LiuCC ChangEJ WestoverDF CoveyTY Chang2005Investigating the allosterism of acyl-CoA:cholesterol acyltransferase (ACAT) by using various sterols: in vitro and intact cell studies.Biochem J391Pt 238997
44. Wang J, Sun F, Zhang DW, Ma Y, Xu F, et al. (2006) Sterol transfer by ABCG5 and ABCG8: in vitro assay and reconstitution. J Biol Chem 281(38): 27894–904.J. WangF. SunDW ZhangY. MaF. Xu2006Sterol transfer by ABCG5 and ABCG8: in vitro assay and reconstitution.J Biol Chem2813827894904
45. Covey DF (2009) ent-Steroids: novel tools for studies of signaling pathways. Steroids 74(7): 577–85.DF Covey2009ent-Steroids: novel tools for studies of signaling pathways.Steroids74757785
46. Bukiya AN, Belani JD, Rychnovsky S, Dopico AM (2010) Specificity of cholesterol and analogs to modulate BK channels points to direct sterol-channel protein interactions. J Gen Physiol 137(1): 93–110.AN BukiyaJD BelaniS. RychnovskyAM Dopico2010Specificity of cholesterol and analogs to modulate BK channels points to direct sterol-channel protein interactions.J Gen Physiol137193110
47. Salton MR (1997) The bacterial membrane in Biomembranes Volume 1. Plenum Press. pp. 1–65.MR Salton1997The bacterial membrane in Biomembranes Volume 1.Plenum Press165
48. Epshtein Y, Chopra AP, Rosenhouse-Dantsker A, Kowalsky GB, Logothetis DE, et al. (2009) Identification of a C-terminus domain critical for the sensitivity of Kir2.1 to cholesterol. Proc Natl Acad Sci U S A 106(19): 8055–60.Y. EpshteinAP ChopraA. Rosenhouse-DantskerGB KowalskyDE Logothetis2009Identification of a C-terminus domain critical for the sensitivity of Kir2.1 to cholesterol.Proc Natl Acad Sci U S A10619805560
49. D'Avanzo N, Cheng WW, Wang S, Enkvetchakul D, Nichols CG (2010) Lipids driving protein structure? Evolutionary adaptations in Kir channels. Channels (Austin) 4(3): 139–41.N. D'AvanzoWW ChengS. WangD. EnkvetchakulCG Nichols2010Lipids driving protein structure? Evolutionary adaptations in Kir channels.Channels (Austin)4313941
You have requested "on-the-fly" machine translation of selected content from our databases. This functionality is provided solely for your convenience and is in no way intended to replace human translation. Show full disclaimer
Neither ProQuest nor its licensors make any representations or warranties with respect to the translations. The translations are automatically generated "AS IS" and "AS AVAILABLE" and are not retained in our systems. PROQUEST AND ITS LICENSORS SPECIFICALLY DISCLAIM ANY AND ALL EXPRESS OR IMPLIED WARRANTIES, INCLUDING WITHOUT LIMITATION, ANY WARRANTIES FOR AVAILABILITY, ACCURACY, TIMELINESS, COMPLETENESS, NON-INFRINGMENT, MERCHANTABILITY OR FITNESS FOR A PARTICULAR PURPOSE. Your use of the translations is subject to all use restrictions contained in your Electronic Products License Agreement and by using the translation functionality you agree to forgo any and all claims against ProQuest or its licensors for your use of the translation functionality and any output derived there from. Hide full disclaimer
© 2011 D'Avanzo et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License: https://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.
Abstract
Cholesterol is the major sterol component of all mammalian cell plasma membranes and plays a critical role in cell function and growth. Previous studies have shown that cholesterol inhibits inward rectifier K+ (Kir) channels, but have not distinguished whether this is due directly to protein-sterol interactions or indirectly to changes in the physical properties of the lipid bilayer. Using purified bacterial and eukaryotic Kir channels reconstituted into liposomes of controlled lipid composition, we demonstrate by 86Rb+ influx assays that bacterial Kir channels (KirBac1.1 and KirBac3.1) and human Kir2.1 are all inhibited by cholesterol, most likely by locking the channels into prolonged closed states, whereas the enantiomer, ent-cholesterol, does not inhibit these channels. These data indicate that cholesterol regulates Kir channels through direct protein-sterol interactions likely taking advantage of an evolutionarily conserved binding pocket.
You have requested "on-the-fly" machine translation of selected content from our databases. This functionality is provided solely for your convenience and is in no way intended to replace human translation. Show full disclaimer
Neither ProQuest nor its licensors make any representations or warranties with respect to the translations. The translations are automatically generated "AS IS" and "AS AVAILABLE" and are not retained in our systems. PROQUEST AND ITS LICENSORS SPECIFICALLY DISCLAIM ANY AND ALL EXPRESS OR IMPLIED WARRANTIES, INCLUDING WITHOUT LIMITATION, ANY WARRANTIES FOR AVAILABILITY, ACCURACY, TIMELINESS, COMPLETENESS, NON-INFRINGMENT, MERCHANTABILITY OR FITNESS FOR A PARTICULAR PURPOSE. Your use of the translations is subject to all use restrictions contained in your Electronic Products License Agreement and by using the translation functionality you agree to forgo any and all claims against ProQuest or its licensors for your use of the translation functionality and any output derived there from. Hide full disclaimer