Voltage-gated ion channels are key players in cellular excitability. Recent studies suggest that their behavior can depend strongly on the membrane lipid composition and physical state. In vivo studies of membrane/channel and channel/channel interactions are challenging as membrane properties are actively regulated in living cells, and are difficult to control in experimental settings. We developed a method to reconstitute functional voltage-gated ion channels into cell-sized Giant Unilamellar Vesicles (GUVs) in which membrane composition, tension and geometry can be controlled. First, a voltage-gated potassium channel, KvAP, was purified, fluorescently labeled and reconstituted into small proteoliposomes. Small proteoliposomes were then converted into GUVs via electroformation. GUVs could be formed using different lipid compositions and buffers containing low (5 mM) or near-physiological (100 mM) salt concentrations. Protein incorporation into GUVs was characterized with quantitative confocal microscopy, and the protein density of GUVs was comparable to the small proteoliposomes from which they were formed. Furthermore, patch-clamp measurements confirmed that the reconstituted channels retained potassium selectivity and voltage-gated activation. GUVs containing functional voltage-gated ion channels will allow the study of channel activity, distribution and diffusion while controlling membrane state, and should prove a powerful tool for understanding how the membrane modulates cellular excitability.
Different patterns of channel activity have been detected by patch clamping excised membrane patches from reconstituted giant liposomes containing purified KcsA, a potassium channel from prokaryotes. The more frequent pattern has a characteristic low channel opening probability and exhibits many other features reported for KcsA reconstituted into planar lipid bilayers, including a moderate voltage dependence, blockade by Na ؉ , and a strict dependence on acidic pH for channel opening. The predominant gating event in this low channel opening probability pattern corresponds to the positive coupling of two KcsA channels. However, other activity patterns have been detected as well, which are characterized by a high channel opening probability (HOP patterns), positive coupling of mostly five concerted channels, and profound changes in other KcsA features, including a different voltage dependence, channel opening at neutral pH, and lack of Na During the last decades, the use of high resolution electrophysiological techniques to study ion channels has provided a large amount of information on functional aspects of these important membrane proteins. Such a detailed information on channel function, however, has not been accompanied by structural knowledge until recently, when several structurally simpler homologues of mammalian ion channels found in extremophyle bacteria or Archaea and remarkably resistant to harsh experimental conditions, have been purified, crystallized and their structure solved at high resolution by x-ray diffraction methods (1-4). A K ϩ channel from the soil bacteria Streptomyces lividans named KcsA 4 (1), a homotetramer made up of identical 160-amino acid subunits, was the first of such structures to be solved (5, 6), and, although the x-ray structure corresponds to a closed channel conformation, it has contributed much to our current understanding of ion selectivity and permeation. Ironically, there was little or no functional information on KcsA by the time its structure was solved, and then several groups undertook the task of characterizing its single channel properties, which has been surrounded by controversy. For instance, Schrempf's group, discoverers of KcsA in S. lividans, reported a strong dependence of channel opening on acidic pH, multiple conductance states with opening probabilities near 0.5, and unusual permeabilities to Na ϩ , Li ϩ , Ca 2ϩ , or Mg 2ϩ , along with K ϩ (7-9). In contrast, Miller's group (10, 11) using purified KcsA reconstituted into planar lipid bilayers found a single conductance state with a much lower opening probability, as well as orthodox ion selectivity and other properties to validate KcsA as a bona fide K ϩ channel and as a faithful structural model for these molecules. The above discrepancies were never fully explained but, still, it became generally accepted that KcsA behaves as a moderately voltage-dependent, K ϩ -selective channel with a characteristic low opening probability and the peculiar property of opening only in response to very acidic pH condit...
2,2,2-Trifluoroethanol (TFE) effectively destabilizes the otherwise highly stable tetrameric structure of the potassium channel KcsA, a predominantly alpha-helical membrane protein [Valiyaveetil, F. I., Zhou, Y., and MacKinnon, R. (2002) Biochemistry 41, 10771-10777]. Here, we report that the effects on the protein structure of increasing concentrations of TFE in detergent solution include two successive protein concentration-dependent, cooperative transitions. In the first of such transitions, occurring at lower TFE concentrations, the tetrameric KcsA simultaneously increases the exposure of tryptophan residues to the solvent, partly loses its secondary structure, and dissociates into its constituent subunits. Under these conditions, simple dilution of the TFE permits a highly efficient refolding and tetramerization of the protein in the detergent solution. Moreover, following reconstitution into asolectin giant liposomes, the refolded protein exhibits nativelike potassium channel activity, as assessed by patch-clamp methods. Conversely, the second cooperative transition occurring at higher TFE concentrations results in the irreversible denaturation of the protein. These results are interpreted in terms of a protein and TFE concentration-dependent reversible equilibrium between the folded tetrameric protein and partly unfolded monomeric subunits, in which folding and oligomerization (or unfolding and dissociation in the other direction of the equilibrium process) are seemingly coupled processes. At higher TFE concentrations this is followed by the irreversible conversion of the unfolded monomers into a denatured protein form.
Binding of the C-terminal Sterile α Motif (SAM) Domain of Human p73 to Lipid Membranes
The ␣ splice variant of p73 (p73␣), a homologue of the tumor suppressor p53, has close to its C terminus a sterile ␣ motif (SAM), SAMp73, that is thought to be involved in protein-protein interactions. Here, we report the lipid binding properties of this domain. Binding was assayed against zwitterionic (phosphatidylcholine) and anionic (phosphatidic acid) lipids and was studied by different biophysical techniques, namely, circular dichroism and fluorescence spectroscopies and differential scanning calorimetry. These techniques unambiguously indicate that SAMp73 binds to lipids. The binding involves protein surface attachment and partial membrane penetration, accompanied by changes in SAMp73 structure.p73 and p63 are members of the p53 gene family (1, 2). As the tumor suppressor p53, p73 and p63 are also transcription factors that contain an N-terminal transactivation domain, a sequence-specific DNA-binding domain, and an oligomerization domain with a high sequence homology to the corresponding domains of p53. For instance, p73 shares 63% identity with the DNA-binding region of p53 (including the conservation of all DNA-binding residues), 38% identity with the tetramerization domain, and 29% with the transactivation domain. Furthermore, p73 and p63 share a relative functional homology with p53, because they can both activate transcription from p53-responsive genes, stop the cell cycle, and induce apoptosis when overexpressed. Moreover, p73 is positively regulated in p53-
Binding of K+ and Na+ to the potassium channel KcsA has been characterized from the stabilization observed in the heat-induced denaturation of the protein as the ion concentration is increased. KcsA thermal denaturation is known to include (i) dissociation of the homotetrameric channel into its constituent subunits and (ii) protein unfolding. The ion concentration-dependent changes in the thermal stability of the protein, evaluated as the Tm value for thermal-induced denaturation of the protein, may suggest the existence of both high- and low-affinity K+ binding sites of KcsA, which lend support to the tenet that channel gating may be governed by K+ concentration-dependent transitions between different affinity states of the channel selectivity filter. We also found that Na+ binds to KcsA with a KD similar to that estimated electrophysiologically from channel blockade. Therefore, our findings on ion binding to KcsA partly account for K+ over Na+ selectivity and Na+ blockade and argue against the strict “snug fit” hypothesis used initially to explain ion selectivity from the X-ray channel structure. Furthermore, the remarkable effects of increasing the ion concentration, K+ in particular, on the Tm of the denaturation process evidence that synergistic effects of the metal-mediated intersubunit interactions at the channel selectivity filter are a major contributor to the stability of the tetrameric protein. This observation substantiates the notion of a role for ions as structural “effectors” of ion channels.
Effects of Conducting and Blocking Ions on the Structure and Stability of the Potassium Channel KcsA
This article reports on the interaction of conducting (K ؉ ) and blocking (Na ؉ ) monovalent metal ions with detergent-solubilized and lipid-reconstituted forms of the K ؉ channel KcsA. Monitoring of the protein intrinsic fluorescence reveals that the two ions bind competitively to KcsA with distinct affinities (dissociation constants for the KcsA⅐K ؉ and KcsA⅐Na ؉ complexes of ϳ8 and 190 mM, respectively) and induce different conformations of the ion-bound protein. The differences in binding affinity as well as the higher K ؉ concentration bathing the intracellular mouth of the channel, through which the cations gain access to the protein binding sites, should favor that only KcsA⅐K ؉ complexes are formed under physiological-like conditions. Nevertheless, despite such prediction, it was also found that concentrations of Na ؉ well below its dissociation constant and even in the presence of higher K ؉ concentrations, cause a remarkable decrease in the protein thermal stability and facilitate thermal dissociation into subunits of the tetrameric KcsA, as concluded from the temperature dependence of the protein infrared spectra and from gel electrophoresis, respectively. These latter observations cannot be explained based on the occupancy of the binding sites from above and suggest that there must be additional ion binding sites, whose occupancy could not be detected by fluorescence and in which the affinity for Na ؉ must be higher or at least similar to that of K ؉ . Moreover, cation binding as reported by means of fluorescence does not suffice to explain the large differences in free energy of stabilization involved in the formation of the KcsA⅐Na ؉ and KcsA⅐K ؉ complexes, which for the most part should arise from synergistic effects of the ion-mediated intersubunit interactions.
Ion channel conformational changes within the lipid membrane are a key requirement to control ion passage. Thus, it seems reasonable to assume that lipid composition should modulate ion channel function. There is increasing evidence that this implicates not just an indirect consequence of the lipid influence on the physical properties of the membrane, but also specific binding of selected lipids to certain protein domains. The result is that channel function and its consequences on excitability, contractility, intracellular signaling or any other process mediated by such channel proteins, could be subjected to modulation by membrane lipids. From this it follows that development, age, diet or diseases that alter lipid composition should also have an influence on those cellular properties. The wealth of data on the non-annular lipid binding sites in potassium channel from Streptomyces lividans (KcsA) makes this protein a good model to study the modulation of ion channel structure and function by lipids. The fact that this protein is able to assemble into clusters through the same non-annular sites, resulting in large changes in channel activity, makes these sites even more interesting as a potential target to develop lead compounds able to disrupt such interactions and hopefully, to modulate ion channel function. This Article is Part of a Special Issue Entitled: Membrane Structure and Function: Relevance in the Cell's Physiology, Pathology and Therapy.
Potassium channels selectivity filter (SF) conformation is modulated by several factors, including ion-protein and protein-protein interactions. Here, we investigate the SF dynamics of a single Trp mutant of the potassium channel KcsA (W67) using polarized time-resolved fluorescence measurements. For the first time, an analytical framework is reported to analyze the homo-Förster resonance energy transfer (homo-FRET) within a symmetric tetrameric protein with a square geometry. We found that in the closed state (pH 7), the W67-W67 intersubunit distances become shorter as the average ion occupancy of the SF increases according to cation type and concentration. The hypothesis that the inactivated SF at pH 4 is structurally similar to its collapsed state, detected at low K + , pH 7, was ruled out, emphasizing the critical role played by the S2 binding site in the inactivation process of KcsA. This homo-FRET approach provides complementary information to X-ray crystallography in which the protein conformational dynamics is usually compromised.
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