Valerij S. Sokolov

Fluorescent styryl dyes of the RH series affect a potential drop on the membrane/solution boundary

The effects of the adsorption of the fluorescent potential-sensitive dyes RH-421, RH-237 and RH-160 on the bilayer lipid membrane were studied. It was shown that a dipole potential drop, positive in the hydrophobic part of the membrane, arose due to the dye adsorption. The dye adsorption led to a considerable increase of the rate constant of hydrophobic anion translocation through the membrane, but did not affect their partition coefficient between membrane and water. It implies that the region of the membrane where the potential drops is located deeper than the adsorption plane of hydrophobic ions. The values of boundary potential differences were estimated by two independent methods with unilateral and bilateral application of the dyes to lipid bilayer membranes. The results suggest that RH dye molecules penetrate through the lipid bilayers. The values of zeta-potential in liposomes did not change on dye adsorption. Hence, dye molecules are adsorbed in a form that does not change the surface charge. We estimated the effects of electric field of dye dipole layer on an individual dipole located in the same layer and on ion transport through a membrane protein Na+/K+-ATPase. It turned out that the local electric field of each dye dipole decayed so rapidly that a neighbouring dye molecule did not feel it. It also appeared that RH dyes could have but a minor effect on the electrogenic transport performed by the sodium pump in the examined range of dye concentrations.

Influence of sodium concentration on changes of membrane capacitance associated with the electrogenic ion transport by the Na,K-ATPase

Abstract Electrogenic ion transport by the Na,K-ATPase was investigated in a model system of protein-containing membrane fragments adsorbed to a lipid bilayer. Transient Na+ currents were induced by photorelease of ATP from inactive caged ATP. This process was accompanied by a capacitance change of the membrane system. Two methods were applied to measure capacitances in the frequency range 1 to 6000 Hz. The frequency dependent capacitance increment, ΔC, was of sigmoidal shape and decreased at high frequencies. The midpoint frequency, f0, depended on the ionic strength of the buffer. At 150 mm NaCl f0 was about 200 Hz and decreased to 12 Hz at high ionic strength (1 M). At low frequencies (f≪f0) the capacitance increment became frequency independent. It was, however, dependent on Na+ concentration and on the membrane potential which was generated by the charge transferred. A simple model is presented to analyze the experimental data quantitatively as a function of two parameters, the capacitance of the adsorbed membrane fragments, CP, and the potential of maximum capacitance increment, ψ0. Below 5 mm Na+ a negative capacitance change was detected which may be assigned to electrogenic Na+ binding to cytoplasmic sites. It could be shown that the results obtained by experiments with the presented alternating current method contain the information which is determined by current-relaxation experiments with cell membranes.

pH-Dependent Formation and Disintegration of the Influenza A Virus Protein Scaffold To Provide Tension for Membrane Fusion

ABSTRACT Influenza virus is taken up from a pH-neutral extracellular milieu into an endosome, whose contents then acidify, causing changes in the viral matrix protein (M1) that coats the inner monolayer of the viral lipid envelope. At a pH of ∼6, M1 interacts with the viral ribonucleoprotein (RNP) in a putative priming stage; at this stage, the interactions of the M1 scaffold coating the lipid envelope are intact. The M1 coat disintegrates as acidification continues to a pH of ∼5 to clear a physical path for the viral genome to transit from the viral interior to the cytoplasm. Here we investigated the physicochemical mechanism of M1s pH-dependent disintegration. In neutral media, the adsorption of M1 protein on the lipid bilayer was electrostatic in nature and reversible. The energy of the interaction of M1 molecules with each other in M1 dimers was about 10 times as weak as that of the interaction of M1 molecules with the lipid bilayer. Acidification drives conformational changes in M1 molecules due to changes in the M1 charge, leading to alterations in their electrostatic interactions. Dropping the pH from 7.1 to 6.0 did not disturb the M1 layer; dropping it lower partially desorbed M1 because of increased repulsion between M1 monomers still stuck to the membrane. Lipid vesicles coated with M1 demonstrated pH-dependent rupture of the vesicle membrane, presumably because of the tension generated by this repulsive force. Thus, the disruption of the vesicles coincident with M1 protein scaffold disintegration at pH 5 likely stretches the lipid membrane to the point of rupture, promoting fusion pore widening for RNP release. IMPORTANCE Influenza remains a top killer of human beings throughout the world, in part because of the influenza viruss rapid binding to cells and its uptake into compartments hidden from the immune system. To attack the influenza virus during this time of hiding, we need to understand the physical forces that allow the internalized virus to infect the cell. In particular, we need to know how the protective coat of protein inside the viral surface reacts to the changes in acid that come soon after internalization. We found that acid makes the molecules of the protein coat push each other while they are still stuck to the virus, so that they would like to rip the membrane apart. This ripping force is known to promote membrane fusion, the process by which infection actually occurs.

Membrane Transport of Singlet Oxygen Monitored by Dipole Potential Measurements

The efficiency of photodynamic reactions depends on 1), the penetration depth of the photosensitizer into the membrane and 2), the sidedness of the target. Molecules which are susceptible to singlet oxygen ((1)O(2)) experience less damage when separated from the photosensitizer by the membrane. Since (1)O(2) lifetime in the membrane environment is orders of magnitude longer than the time required for nonexcited oxygen (O(2)) to cross the membrane, this observation suggests that differences between the permeabilities or membrane partition of (1)O(2) and O(2) exist. We investigated this hypothesis by releasing (1)O(2) at one side of a planar membrane while monitoring the kinetics of target damage at the opposite side of the same membrane. Damage to the target, represented by dipole-modifying molecules (phloretin or phlorizin), was indicated by changes in the interleaflet dipole potential difference Deltaphi(b). A simple analytical model allowed estimation of the (1)O(2) interleaflet concentration difference from the rate at which Deltaphi(b) changed. It confirmed that the lower limit of (1)O(2) permeability is approximately 2 cm/s; i.e., it roughly matches O(2) permeability as predicted by Overtons rule. Consequently, the membrane cannot act as a barrier to (1)O(2) diffusion. Differences in the reaction rates at the cytoplasmic and extracellular membrane leaflets may be attributed only to (1)O(2) quenchers inside the membrane.

Membrane Photopotential Generation by Interfacial Differences in the Turnover of a Photodynamic Reaction

The adsorption of a membrane-impermeable photosensitizer to only one membrane leaflet is found to trigger a localized photodynamic reaction; i.e., the amount of carbonyl cyanide m-chlorophenylhydrazone (CCCP) molecules damaged in the leaflet facing the photosensitizer is roughly identical to the total amount of CCCP inactivated. Whereas the latter quantity is assessed from the drop in membrane conductivity G, the former is evaluated from the photopotential phi that is proportional to the interfacial concentration difference of the uncoupler. Localized photodestruction is encountered by CCCP diffusion to the site of photodamage. A simple model that accounts for both photoinhibition and diffusion predicts the dependence of the photopotential on light intensity, buffer capacity, and pH of the medium. It is concluded that only a limited amount of the reactive oxygen species responsible for CCCP photodamage diffuses across the membrane. If the concentration of reactive oxygen species is decreased by addition of NaN(3) or by substituting aqueous oxygen for argon, phi is inhibited. If, in contrast, their life time is increased by substitution of H(2)O for D(2)O, phi increases.

Voltage-sensitive styryl dyes as singlet oxygen targets on the surface of bilayer lipid membrane

Photosensitizers are widely used as photodynamic therapeutic agents killing cancer cells by photooxidation of their components. Development of new effective photosensitive molecules requires profound knowledge of possible targets for reactive oxygen species, especially for its singlet form. Here we studied photooxidation of voltage-sensitive styryl dyes (di-4-ANEPPS, di-8-ANEPPS, RH-421 and RH-237) by singlet oxygen on the surface of bilayer lipid membranes commonly used as cell membrane models. Oxidation was induced by irradiation of a photosensitizer (aluminum phthalocyanine tetrasulfonate) and monitored by the change of dipole potential on the surface of the membrane. We studied the drop of the dipole potential both in the case when the dye molecules were adsorbed on the same side of the lipid bilayer as the photosensitizer (cis-configuration) and in the case when they were adsorbed on the opposite side (trans-configuration). Based on a simple model, we determined the rate of oxidation of the dyes from the kinetics of change of the potential during and after irradiation. This rate is proportional to steady-state concentration of singlet oxygen in the membrane under irradiation. Comparison of the oxidation rates of various dyes reveals that compounds of ANEPPS series are more sensitive to singlet oxygen than RH type dyes, indicating that naphthalene group is primarily responsible for their oxidation.

Electrogenic transport of sodium ions in cytoplasmic and extracellular ion access channels of Na + ,K + -ATPase probed by admittance measurement technique

Electrogenic movements of sodium ions in cytoplasmic and extracellular access channel of the Na+,K+-ATPase have been studied by the admittance measurement technique which allows the detection of small changes of the membrane capacitance and conductance induced by phosphorylation of the ion pump. The measurements were carried out on a model system consisting of a bilayer lipid membrane, to which membrane fragments with ion pumps were adsorbed that contain the ion pumps in high density. Small changes of the membrane capacitance and conductance were induced by a fast release of ATP from caged ATP. The effect was measured at various frequencies and in solutions with different Na+ concentrations. The experimentally observed frequency dependences were explained using a theoretical model assuming that Na+ movement through the cytoplasmic access channel occurs in one step and through the extracellular access channel, in two steps. The phosphorylation of the protein by ATP leads to a block of the cytoplasmic access channel and an opening the extracellular access channel. The disappearance of electrogenic Na+ movements on the cytoplasmic side produces a negative change of capacitance and conductance, while the emergence of extracellular Na+ movements generates a positive change. Fitting the experimental dependences of capacitance and conductance by theoretical curves allowed the determination equilibrium and kinetic parameters of sodium transport in the access channels.

Effect of chaotropic anions on the sodium transport by the Na,K-ATPase

The effect of choline iodide, bromide and chloride on the kinetics of the electrogenic sodium transport by the Na,K-ATPase was investigated in a model system of ATPase-containing membrane fragments adsorbed on the lipid bilayer membrane. The kinetic parameters of Na+ transport were determined from short circuit currents after fast release of ATP from its caged precursor. The falling phase of the current transients could be fitted by a single exponential with the time constant, τ2. Its temperature dependence allowed an estimation of the activation energy of the rate-limiting reaction step, the conformation transition E1/E2. Choline iodide and bromide caused a decrease of the activation energy as well as the overall rate of the process expressed as the pre-exponential factor A of the Arrhenius equation. If choline iodide or bromide were present on the cytoplasmic and extracellular sides of the protein, the temperature dependent changes were more pronounced than when present on the cytoplasmic side only. These results can be explained by an effect of the anions on water structure on the extracellular surface of the protein, where a deep access channel connects the ion-binding sites with the solution. Chloride ions also caused a deceleration of the electrogenic transport, however, in contrast to iodide or bromide, they did not affect the activation energy, and were more effective when added on the cytoplasmic side. This effect can be explained by asymmetric screening of the negative surface charges which leads to a transmembrane electric potential that modifies the ion transfer.

Electrogenic Binding of Ions at the Cytoplasmic Side of the Na + ,K + ATPase

Electrogenic binding of ions from the cytoplasmic side of the Na+,K+-ATPase has been studied by measurements of changes of the membrane capacitance and conductance triggered by a jump of pH or of the sodium-ion concentration in the absence of ATP. The pH jumps were performed in experiments with membrane fragments containing purified Na+,K+-ATPase adsorbed to a bilayer lipid membrane (BLM). Protons were released in a sub-millisecond time range from a photosensitive compound (caged H+) triggered by a UV light flash. The sodium concentration jumps were carried out by a fast solution exchange in experiments with membrane fragments attached to a solid-supported membrane deposited on a gold electrode. The change of the membrane capacitance triggered by the pH jump depended on the sodium-ion concentration. Potassium ions had a similar effect on the capacitance change triggered by a pH jump. The effects of these ions are explained by the their competition with protons in the binding sites on cytoplasmic side of the Na+,K+-ATPase. The approximation of the experimental data by a theoretical model yields the dissociation constants, K, and the cooperativity coefficients, n, of the binding sites for sodium ions (K = 2.7 mM, n = 2) and potassium ions (K = 1.7 mM, n = 2). In the presence of magnesium ions the apparent dissociation constants of sodium increased. A possible reason of the inhibition of sodium-ion binding by magnesium ions can be an electrostatic or conformational effect of magnesium ions bound to a separate site of the Na+,K+-ATPase close to the entrance to the sodium-ion binding sites.

Involvement of protons in the ion transport cycle of Na+,K+-ATPase

The effect of pH on electrogenic sodium transport by the Na+,K+-ATPase has been studied. Experiments were carried out by admittance recording in a model system consisting of a bilayer lipid membrane with adsorbed membrane fragments containing purified Na+,K+-ATPase. Changes in the membrane admittance (capacitance and conductance increments in response to photo-induced release of ATP from caged ATP) were measured as function of AC voltage frequency, sodium ion concentration, and pH. In solutions containing 150 mM Na+, the frequency dependence of capacitance increments was not significantly dependent on pH in the range between 6 and 8. At a low NaCl concentration (3 mM), the capacitance increments at low frequencies decreased with the increasing pH. In the absence of NaCl, the frequency-dependent capacitance increment at low frequencies was similar to that measured in the presence of 3 mM NaCl. These results may be explained by involvement of protons in the Na+,K+-ATPase pump cycle, i.e., electroneutral exchange of sodium ions for protons under physiological conditions, electrogenic transport of sodium ions at high pH, and electrogenic transport of protons at low concentrations (and in the absence) of sodium ions.