Direct and Specific Activation of Human Inward Rectifier K+ Channels by Membrane Phosphatidylinositol 4,5-Bisphosphate*

Many ion channels are modulated by phosphatidylinositol 4,5-bisphosphate (PIP2), but studies examining the PIP2 dependence of channel activity have been limited to cell expression systems, which present difficulties for controlling membrane composition. We have characterized the PIP2 dependence of purified human Kir2.1 and Kir2.2 activity using 86Rb+ flux and patch clamp assays in liposomes of defined composition. We definitively show that these channels are directly activated by PIP2 and that PIP2 is absolutely required in the membrane for channel activity. The results provide the first quantitative description of the dependence of eukaryotic Kir channel function on PIP2 levels in the membrane; Kir2.1 shows measureable activity in as little as 0.01% PIP2, and open probability increases to ∼0.4 at 1% PIP2. Activation of Kir2.1 by phosphatidylinositol phosphates is also highly selective for PIP2; PI, PI(4)P, and PI(5)P do not activate channels, and PI(3,4,5)P3 causes minimal activity. The PIP2 dependence of eukaryotic Kir activity is almost exactly opposite that of KirBac1.1, which shows marked inhibition by PIP2. This raises the interesting hypothesis that PIP2 activation of eukaryotic channels reflects an evolutionary adaptation of the channel to the appearance of PIP2 in the eukaryotic cell membrane.

Ion channels are modulated by their lipid environment (1)(2)(3)(4)(5)(6), and perhaps the best characterized lipid modulator of ion channel activity is phosphatidylinositol 4,5-bisphosphate (PIP 2 ) 3 (7). Inward rectifying potassium channels (Kir) are just one of a host of ion channels that are regulated by PIP 2 (7), and a number of genetic diseases, including Andersen-Tawil syndrome (8,9), Bartter syndrome (9), and neonatal diabetes (10), result from Kir channel mutations that alter PIP 2 sensitivity. Structurefunction studies and molecular simulations suggest a PIP 2 binding site at the top of the cytoplasmic domain, just below the surface of the inner membrane leaflet (9,(11)(12)(13)(14)(15). These studies, however, have provided limited and largely qualitative information on how such lipids influence Kir channel function because they all utilize cell-based systems, in which the membrane composition is unknown and cannot be precisely controlled. Alternative approaches using recombinant systems in which the components can be fully controlled are needed to expand our current knowledge (7).
Until recently, high yield recombinant expression and purification of functional ion channels have been technically prohibitive and restricted to prokaryotic channels (3,16). We have recently demonstrated the feasibility of purifying functional eukaryotic Kir channel after recombinant expression in Saccharomyces cerevisiae (17). To quantitatively examine the PIP 2 dependence of eukaryotic Kir channel activity, we have purified human Kir2.1 (KCNJ2) and Kir2.2 (KCNJ12) and performed functional studies using both liposomal 86 Rb ϩ flux assays and patch clamp assays of giant liposomes.

EXPERIMENTAL PROCEDURES
Human Kir2.1 (KCNJ2) and Kir2.2 (KCNJ12) were subcloned into the pND-CTFH vector and expressed in the FGY217 strain of S. cerevisiae as described previously (17). Starter cultures were grown in SC Ϫ Ura medium ϩ 2% glucose and then scaled up overnight at 250 rpm and 30°C in Ultrayield shaker flasks (A 600 ϳ1.5). SC Ϫ Ura ϩ 2% galactose/flask were then inoculated with these cultures for induction (A 600 ϳ0.2) and grown for ϳ48 or 72 h respectively. Cells were harvested by centrifugation at 4000 ϫ g, washed in TBS, resuspended in lysis buffer (50 mM Tris, pH 7.5, 10 mM EDTA, 0.6 M sorbitol, Complete EDTA-free tablets, protease inhibitor set IV (Calbiochem)) and ruptured by 10 passes at high pressure (25,000 -35,000 p.s.i) using a Microfluidics cell disrupter. KCl was added to cell lysate 500 mM final, and cell debris was removed by 5 min of centrifugation at 500 ϫ g followed by 25 min at 4000 ϫ g. Crude membranes were collected by centrifugation for 1 h at 120,000 ϫ g and homogenized in resuspension buffer (50 mM Tris 7.5, 10 mM EDTA, 500 mM KCl, 2 mM DTT, 10% glycerol, Complete EDTA-free protease inhibitor) to ϳ3.5 mg/ml total protein and then solubilized by the addition of 1% fos-choline 14 (Anatrace) for 3 h at 4°C. Solubilized membranes were clarified by centrifugation at 56,500 ϫ g. M2 anti-FLAG resin (Sigma-Aldrich) was added to the supernatant and spun slowly on a blood wheel for 3 h at 4°C. The resin was batch-washed in 0.5% fos-choline 14, packed into a drip column, washed with 25 column volumes of wash buffer with progressively reduced detergent concentrations to 0.03% fos-choline 14, and eluted with 0.2 mg/ml 3ϫFLAG peptide (Sigma-Aldrich). Elution fractions were combined, concentrated using a 100,000 molecular weight cut-off concentrator (Vivaspin), and separated by gel filtration on a Superdex 200 10/300 GL column (GE Healthcare). Peak fractions were combined, concentrated to ϳ3-6 mg/ml, and used for functional studies. 86 Rb ϩ flux assay was performed as reported previously (18) using liposomes made of 3:1 1-palmitoyl-2-oleoyl-3-phosphatidylethanolamine (POPE) and 1-palmitoyl-2-oleoyl-3-phosphatidylglycerol (POPG), respectively (mass percentage), and the desired phosphatidylinositol phosphates (PIPs) purchased from Avanti. Lipids were solubilized in buffer A (450 mM KCl, 10 mM HEPES, 4 mM N-methyl-D-glucamine, pH 7) with 35 mM CHAPS at 10 mg/ml and mixed with 5 g of Kir2.1 or Kir2.2 protein/1 mg of lipid. Liposomes were formed by spinning through partially dehydrated Sephadex G-50 columns, first in buffer A and then in buffer B (450 mM sorbitol, 10 mM HEPES, 4 mM N-methyl-D-glucamine, pH 7). Uptake was initiated by adding 400 l of buffer B with 1-5 l of 1 Ci of 86 Rb ϩ (PerkinElmer Life Sciences). At various time points, aliquots were flowed through 0.5-ml Dowex cation exchange columns, mixed with scintillation fluid, and counted on a liquid scintillation counter. Each sample was normalized to maximum uptake in valinomycin.
For patch clamping of giant liposomes, 30 g of protein was solubilized with 2 mg of lipids, and liposomes were formed as described for flux assay. Giant liposomes were formed by a dehydration-rehydration cycle procedure (19). All recordings were done 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 (Axon Instruments). Patch pipettes were pulled from soda lime glass microhematocrit tubes (Kimble) to a resistance of ϳ2-3 megaohms. Single channel data were digitized at a sampling rate of 10 kHz, and a low pass analog filter was set to 1 kHz. Analysis of single channel data was performed on the pClamp 9.2 software suite (Axon Instruments).
Tests for statistical significance were performed using an unpaired t test or one-way analysis of variance as appropriate, and statistical significance, reported by an asterisk in Fig. 2

RESULTS AND DISCUSSION
Human Kir2.1 and Kir2.2 proteins were expressed in S. cerevisiae, purified in milligram quantities as mono-dispersed tetrameric complexes, reconstituted in liposomes, and assayed for activity by 86 Rb ϩ flux assay (17). All experiments were performed on liposomes composed of 3:1 POPE:POPG with replacement of POPE by varying amounts of PIPs, reported as a mass:mass ratio. Without PIP 2 incorporated in the membrane, we detected no activity from either Kir2.1 or Kir2.2 channels, but there was a robust dose-dependent increase in channel-dependent 86 Rb ϩ flux with incorporation of PIP 2 (Fig. 1, A and B). Kir2.1 and Kir2.2 activity is detectable in as little as 0.01% PIP 2 and appears to plateau at ϳ1-3% (Fig. 1B). These data demonstrate that low levels of PIP 2 are sufficient and necessary for channel activity on the POPE:POPG background. We have shown previously that the prokaryotic Kir channel, KirBac1.1, is also directly modulated by PIP 2 in reconstituted liposomes, except that PIP 2 has the opposite effect and inhibits the channel (Fig. 1B) (16,19). Interestingly, the dynamic ranges of PIP 2 modulation of Kir2.1, Kir2.2, and KirBac1.1 activity are almost identical (Fig. 1B), although Kir2.1 and Kir2.2 appear to be more sensitive. Indeed, Kir2 channels may be more sensitive to PIP 2 than other Kir channels such as Kir3.1 (2). To permit detailed voltage clamp analysis of the PIP 2 dependence of channel activity, Kir2.1 was reconstituted in giant liposomes (19). Measured single channel currents have a unitary conductance (ϳ35 pS slope conductance) similar to Kir2.1 currents measured from heterologous or native expression systems ( Fig. 2A) (20,21). Increasing PIP 2 over the range of concentrations expected in cell membranes increases open probability (Fig. 2B), with no effect on unitary conductance (Fig. 2C), consistent with previous reports of the effects of exogenous PIP 2 incorporation into cellular membranes (21,22). The PIP 2 activity relationship plateaus at ϳ1-3% PIP 2 in both patch clamp and 86 Rb ϩ flux assays (Figs. 1C and 2B). Interestingly, the open probability reaches a maximum of ϳ0.4 at 1% PIP 2 (Fig.  2B) over the range of Ϫ80 to Ϫ120 mV (data not shown), much lower than the high open probabilities (Ͼ0.9) previously reported in heterologous expression systems (21). This discrepancy might suggest that other lipid/protein modulators may be involved in activating Kir2.1 in cellular membranes.
Prior studies of PIP 2 modulation of eukaryotic Kir channels have relied on cell-based systems, which pose a number of limitations. First, changing the lipid composition typically requires diffusing micelles onto a membrane patch, a poorly controlled method that provides no quantification of lipid incorporation into the membrane (24). Even perfusing water-soluble dioctanoyl PIP derivatives onto membranes permits only relative quantification of the effects of different lipids (25) because partitioning is not easily quantified. Second, because the exact composition is unknown, the influence of other protein or lipid modulators cannot be excluded (26). We have overcome these limitations by using reconstituted liposomes of defined lipid composition, permitting us to describe, for the first time, the dependence of a eukaryotic channel activity on membrane PIP 2 level. The minimum range in which reconstituted Kir2.1 and Kir2.2 are modulated by PIP 2 (Fig. 1B) lies well within physiological levels of PIP 2 in eukaryotic plasma membranes (ϳ0.25-1%) (27,28). Furthermore, this result definitively shows that Kir2.1 and Kir2.2 activity (and by extension probably activity of all eukaryotic Kir channels) can be directly stimulated by PIP 2 in the membrane and that activation occurs without intermediary proteins. Kir channel activity may also be modulated by other lipids and cholesterol (29), and this can now be quantitatively addressed using the approach described.
It is striking that both human Kir channels (Kir2.1 and Kir2.2) and the prokaryotic KirBac1.1 are directly modulated by PIP 2 when reconstituted in liposomes yet exhibit completely opposite effects; Kir2.1 and Kir2.2 are activated by PIP 2 (Figs. 1,  A and B, and 2), whereas KirBac1.1 is inhibited (Fig. 1B) (16,19). We have suggested that such a marked difference in PIP 2 action may be attributed to the absence of three highly conserved residues in the transmembrane-cytoplasmic linkers of prokaryotic KirBacs as compared with eukaryotic Kir channels (16,19). This structural difference may result in intracellular displacement of the cytoplasmic domain of Kir2.2 as compared with KirBac1.1, as apparent in crystal structure alignments (Fig. 1C) (30,31), and may affect interactions between the slide helix and cytoplasmic domain and perhaps therefore gating in these channels (32). The marked difference in PIP 2 modulation between eukaryotic and prokaryotic Kir channels raises the  interesting hypothesis that membrane lipids can drive the evolution of protein structure and function (32). PIP 2 and other phosphoinositide species are typically absent in prokaryotes (33)(34)(35), an environment in which KirBac1.1 is active (18). The sensitivity of KirBac1.1 to inhibition by PIP 2 may have been a byproduct of the evolution of regulatory domains for soluble ligands such as ATP. In eukaryotic membranes, where PIP 2 is one of the most abundant PIPs and is primarily localized at the plasma membrane (27,36), Kir channels could not retain the same dependence on PIP 2 because KirBac1.1 would be almost completely inhibited at cellular PIP 2 levels (16). Rather, because Kir channel activity either needed to be reduced, silenced during trafficking in intracellular organelles, or activated by localized changes in plasma membrane PIP 2 (28,37), eukaryotic Kir channels evolved to be highly sensitive to PIP 2 for activation by relatively minor changes in channel sequence and structure. As multiple ion channels and transporters are regulated by PIP 2 (7), it is possible that this same pattern and potential evolutionary mechanism is present between other proteins and their prokaryotic counterparts.