The Rates of Interexchange of Ions Across Fixed Charge Membranes in Bi-Ionic Systems

This paper examines the applicability of the Nernst-Planck approach in treating the relationship between the initial rates at which critical ions interexchange across permselective membranes in bi-ionic systems and the rates of self-exchange of these ions across the same membranes. Data are presented for five species of univalent cations with two types of cation permeable membranes, a polystyrene sulfonic acid-collodion matrix membrane, and an oxidized collodion membrane; five species of univalent anions were studied with a protamine-collodion matrix anion permeable membrane. Except with systems involving H⁺ ion, the experimentally found relationships between the rates of interexchange and the rates of self-exchange were in agreement, in most cases within ±5%, with the values calculated from an expression in which interaction between the critical ions in the membrane is not taken into account. In systems with H⁺ ion, the experimental rates of interexchange were from 27% to 40% less than calculated values.     

Permeability properties of unilamellar vesicles containing choline plasmalogens and comparison with other choline glycerophospholipid species

The rates of non-electrolyte and ion diffusion across bilayer membranes consisting of choline plasmologens or of their alkyl and acyl analogs were studied. The influx of [¹⁴C]glucose, ⁸⁶Rb⁺ and ³⁶Cl^? into small unilamellar vesicles made from a semisynthetic choline plasmalogen and from synthetic diacyl, alkylacyl and dialkyl analogs with comparable side chain compositions were measured. Rates of glucose and Rb⁺ diffusion are about equal in alkenylacyl- and diacyl-glycerophosphocholine (GPC) bilayers, but are reduced in dialkyl-GPC membranes; the permeability coefficients correlate with the packing densities of the respective choline glycerophospholipids in monolayers at the air water interface. Rates of chloride diffusion are consistently higher in membranes formed from phospholipids containing alkenyl or alkyl other bonds as compared to the diacyl analogs. Highest rates of Cl^? diffusion are observed with choline plasmalogen vesicles. The phospholipid side chain composition has little influence on Cl^? permeation, but glucose and Rb⁺ diffusion are markedly affected. Incorporation of cholesterol (30 mol%) into choline plasmalogen membranes reduces their solute permeability by approximately 70%. A similar effect is found with the other choline phospholipid analogs. Thus, the choline phospholipid—cholesterol interaction, as far as it is reflected in reduced bilayer permeability, is not influenced by the presence of the alkenylether bond of plasmalogens.     

Failure of the Nernst-Einstein Equation to Correlate Electrical Resistances and Rates of Ionic Self-Exchange across Certain Fixed Charge Membranes

The electrical resistances and rates of self-exchange of univalent critical ions across several types of collodion matrix membranes of high ionic selectivity were studied over a wide range of conditions. The relationship which was observed between these quantities with membranes of a certain type, namely those activated with poly-2-vinyl-N-methyl pyridinium bromide, cannot be explained on the basis of current concepts of the movement of ions across ion exchange membranes. Rates of self-exchange across these membranes were several times greater than those calculated from the electrical resistances of the membranes on the basis of an expression derived by the use of the Nernst-Einstein equation. The magnitude of the discrepancy was greatest at low concentrations of the ambient electrolyte solution and was independent of the species of both critical and noncritical ions. The data obtained with other types of collodion matrix membranes were, at least approximately, in agreement with the predictions based on the Nernst-Einstein equation. Self-exchange rates across the anion permeable protamine collodion membranes, and across the cation permeable polystyrene sulfonic acid collodion membranes, were about 20% less than those calculated from the electrical resistances. The direction and magnitude of these differences, also observed by other investigators, are qualitatively understood as an electroosmotic effect. With cation permeable membranes prepared by the oxidation of preformed collodion membranes, almost exact agreement was obtained between measured and calculated self-exchange rates; the cause of the apparent absence of an electroosmotic effect with these membranes is unknown.     

The effect of plasmolysis and deplasmolysis on the permeability of plant membranes

The overall washing out of ions, especially⁸⁶Rb⁺ (as the tracer for K⁺), from hypocotyl segments of pumpkin (Cucurbita pepo L.) into distilled water or a CaCl₂ solution was studied, during plasmolysis with a saccharose solution and during deplasmolysis. Compartimental analysis was used to evaluate the⁸⁶Rb⁺ washing out kinetics. During plasmolysis, the washing out of⁸⁶Rb⁺ increases, due to two processes whose half-times are lower than those during washing out into the CaCl₂ solution. During deplasmolysis, the permeability of plasmalemma and tonoplast is substantially descreased, leading to washing out of most⁸⁶Rb⁺ from the cells. Plasmolysis differs from a mere decrease in the turgor pressure in the fact that after exchange for a hypotonic solution the membranes are irreversibly damaged. The aim of this work was to monitor the changes in the cell membrane permeability due to a change in the water potential of the cells, especially during plasmolysis and deplasmolysis.     

THE POTENTIOMETRIC ANALYSIS OF MEMBRANE STRUCTURE AND ITS APPLICATION TO LIVING ANIMAL MEMBRANES

1. The electromotive forces which arise, if two electrolyte solutions are separated from each other by a layer of any kind, are discussed. A general equation is derived comprising the known equations for diffusion, partition, and membrane (Donnan) potentials as special cases. 2. A method is proposed to analyse membranes potentiometrically with respect to their cation or anion selectivity, their dissolving power for ions, and their influence on ion mobility (migration velocity). 3. The possibility of analysing a membrane composed of several layers of different permeability is discussed. 4. The investigation of the skin of the belly of Rana temporaria leads to the following results. It is composed of at least four layers of different permeability, one of which is specifically permeable to H ions and is very likely identical with the "basal membrane" situated between the stratum germinativum and the corium. The major part of the resting potential of the skin is located across this membrane and is due to the difference of H⁺ concentrations on both sides of the membrane. 5. Experiments on muscle show that the sarcolemma is specifically permeable to H ions. The injury potential of the muscle is attributed to the difference of H⁺ concentration inside and outside the fibre.     

Contribution of residues in second transmembrane domain of ASIC1a protein to ion selectivity

Acid-sensing ion channels (ASICs) are proton-gated cation-selective channels expressed in the peripheral and central nervous systems. The ion permeation pathway of ASIC1a is defined by residues 426–450 in the second transmembrane (TM2) segment. The gate, formed by the intersection of the TM2 segments, localizes near the extracellular boundary of the plasma membrane. We explored the contribution to ion permeation and selectivity of residues in the TM2 segment of ASIC1a. Studies of accessibility with positively charged methanethiosulfonate reagents suggest that the permeation pathway in the open state constricts below the gate, restricting the passage to large ions. Substitution of residues in the intracellular vestibule at positions 437, 438, 443, or 446 significantly increased the permeability to K⁺ versus Na⁺. ASIC1a shows a selectivity sequence for alkali metals of Na⁺>Li⁺>K⁺≫Rb⁺>Cs⁺. Alanine and cysteine substitutions at position 438 increased, to different extents, the relative permeability to Li⁺, K⁺, Rb⁺, and Cs⁺. For these mutants, ion permeation was not a function of the diameter of the nonhydrated ion, suggesting that Gly-438 encompasses an ion coordination site that is essential for ion selectivity. M437C and A443C mutants showed slightly increased permeability to K⁺, Rb⁺, and Cs⁺, suggesting that substitutions at these positions influence ion discrimination by altering molecular sieving. Our results indicate that ion selectivity is accomplished by the contribution of multiple sites in the pore of ASIC1a.     

Faster-than-anticipated Na/Cl diffusion across lipid bilayers in vesicles

Maintenance of electrochemical potential gradients across lipid membranes is critical for signal transduction and energy generation in biological systems. However, because ions with widely varying membrane permeabilities all contribute to the electrostatic potential, it can be difficult to measure the influence of diffusion of a single ion type across the bilayer. To understand the electrodiffusion of H⁺ across lipid bilayers, we used a pH-sensitive fluorophore to monitor the lumenal pH in vesicles after a stepwise change in the bulk pH. In vesicles containing the ion channel gramicidin, the lumenal pH rapidly approached the external pH. In contrast, the lumen of intact vesicles showed a two stage pH response: an initial rapid change occurred over ~ 1 min, followed by a much slower change over ~ 24 h. We provide a quantitative interpretation of these results based on the Goldman–Hodgkin–Katz ion fluxes discharging the electrical capacitance of the bilayer membrane. This interpretation provides an estimate of the permeability of the membranes to Na⁺ and Cl⁻ ions of ~ 10^− 8 cm/s, which is ~ 3 orders of magnitude faster than previous reports. We discuss possible mechanisms to account for this considerably higher permeability in vesicle membranes.     

A dielectric dispersion technique for measuring the ionic permeability of internal membranes of isolated chloroplasts

Summary A method has been developed in which a chloroplast suspension is placed between electrodes to which a variable AC potential is applied. The dielectric constant of the suspension varies inversely as the square root of frequency within the range 0.5 to 50 MHz. Results are consistent with the view that this dielectric dispersion is due to ion movement across the chloroplast internal membranes, under the influence of the applied potential. The slope of the dispersion depends on the permeability of the membranes, and thus enables the mobility of externally added ions to be calculated. Results imply that the internal membranes of sugar cane chloroplasts are more permeable to K⁺ than Na⁺, and more permeable to Cl^– than CH₃COO^–. Results also confirm the view that Triton X-100 increases the ionic permeability of membranes.     

pH-dependent permeabilization of the plasma membrane of mammalian cells by anthrax protective antigen

Protective antigen (PA) of anthrax toxin forms ion-conductive channels in planar lipid bilayers and liposomes under acidic pH conditions. We show here that PA has a similar permeabilizing action on the plasma membranes of CHO-K1 and three other mammalian cell lines (J774A.1, RAW264.7 and Vero). Changes in membrane permeability were evaluated by measuring the efflux of the K⁺ analogue, ⁸⁶Rb⁺, from prelabelled cells, and the influx of ²²Na⁺. The permeabilizing activity of PA was limited to a proteolytically activated form (PA_N) and was dependent on acidic pH for membrane insertion (optimal at pH 5.0), but not for sustained ion flux. The flux was reduced in the presence of several known channel blockers: tetrabutyl-, tetrapentyl-, and tetrahexylammonium bromides. PA_N facilitated the membrane translocation of anthrax edema factor under the same conditions that induced changes in membrane permeability to ions. These results indicate that PA_N permeabilizes cellular membranes under conditions that are believed to prevail in the endosomal compartment of toxin-sensitive cells; and they provide a basis for more detailed studies of the relationship between channel formation and translocation of toxin effector moieties in vivo.     

Molecular basis of ion permeability in a voltage‐gated sodium channel

Voltage‐gated sodium channels are essential for electrical signalling across cell membranes. They exhibit strong selectivities for sodium ions over other cations, enabling the finely tuned cascade of events associated with action potentials. This paper describes the ion permeability characteristics and the crystal structure of a prokaryotic sodium channel, showing for the first time the detailed locations of sodium ions in the selectivity filter of a sodium channel. Electrostatic calculations based on the structure are consistent with the relative cation permeability ratios (Na⁺ ≈ Li⁺ ≫ K⁺, Ca²⁺, Mg²⁺) measured for these channels. In an E178D selectivity filter mutant constructed to have altered ion selectivities, the sodium ion binding site nearest the extracellular side is missing. Unlike potassium ions in potassium channels, the sodium ions in these channels appear to be hydrated and are associated with side chains of the selectivity filter residues, rather than polypeptide backbones.     

The influence of surface charge on the kinetics of ion-translocation across biological membranes

Rate equations have been developed which describe the concentration dependence for ion-translocation across charged membranes for those cases in which the translocation process can be considered to be formally equivalent with an enzymic process of a Michaelis-Menten type. We have limited ourselves to those cases in which the ion-translocational step through the membrane is electroneutral. In addition it is assumed that the sites on the membrane involved in the ion-translocation process can not move through the membrane when these sites are not occupied by ions.It is shown that in general deviations from Michaelis-Menten kinetics may be expected. In case of monovalent ion-translocation across oppositely charged membranes apparent negative homotrope cooperative effects may occur, whereas for ion-translocation across equally charged membranes apparent positive homotrope cooperative effects may be found. When the bulk aqueous phase also contains polyvalent ions both types of effects may occur both in the case of ion-translocation across oppositely charged membranes as well as with ion-translocation across a membrane of which the sign of the surface charge is the same as that of the ion translocated.Under limited conditions, also apparent single Michaelis-Menten kinetics may be observed. In these cases, however, the apparent K_m generally is no linear function of the concentration of a competing ion. It is shown that even when an ion does not bind to the translocation sites the K_m is affected by increasing concentrations of this ion, a phenomenon which is not expected when the membrane is not charged. The effects of divalent ions, added to the bulk aqueous phase as 1-1-electrolytes, upon the K_m are discussed in connection with in literature reported effects of Ca⁺⁺ upon the rate of uptake of several monovalent ions into plant cells.     

The acrosome reaction of Strongylocentrotus purpuratus sperm. Ion requirements and movements

The acrosome reaction of sperm of the sea urchin, Strongylocentrotus purpuratus, is accompanied by ion movements. When the reaction is induced by the addition of egg jelly to sperm suspended in sea water, there is an acid release and an uptake (or exchange) of calcium ions. Verapamil and D600, drugs which block Ca²⁺ channels, inhibit induction of the acrosome reaction, acid release, and ⁴⁵Ca²⁺ uptake; this inhibition is reduced at higher concentrations of external Ca²⁺. Although acid release correlates temporally with extension of the acrosome filament, ⁴⁵Ca²⁺ uptake continues after the acrosome reaction has been completed. Neither the acrosome reaction nor acid release is inhibited by cyanide, azide, dinitrophenol (DNP), or carbonyl cyanide m-chlorophenylhydrazone (CCCP), whereas these metabolic inhibitors partially inhibit Ca²⁺ uptake. Tetraethylammonium (TEA) chloride, an inhibitor of delayed axonal potassium currents, inhibits the acrosome reaction. An increase in ⁸⁶Rb⁺ permeability accompanies the acrosome reaction, suggesting that movement of K⁺ is an important effector of the reaction. In support of this, the acrosome reaction may be triggered with nigericin, an ionophore that catalyzes the electrically neutral exchange of K⁺ and H⁺ across membranes. Induction of the acrosome reaction with nigericin can occur with either Na⁺ or K⁺ as the predominant external monovalent cation, while with jelly it requires external Na⁺. With nigericin, there is a delay in acid release, Ca²⁺ uptake, and filament extension, all of which follow a transient proton uptake. Taken together, these data suggest that triggering of the acrosome reaction involves linked permeability changes for monovalent and divalent ions.     

The stimulation of diffusion of adenine nucleotides across bimolecular lipid membranes by divalent metal ions

The diffusion rates of [³H] adenine nucleotides across bimolecular lipid membranes were shown to be directly related to their organic/water partition coefficients, the order being ATP > ADP > AMP. Nucleotide diffusion was stimulated by divalent metal ions with the order of stimulation being Cu⁺² ? Zn⁺² > Mg⁺². The ability of a divalent metal ion to stimulate diffusion appears to be related to its ability to bind to the N-7 of the adenine ring. The divalent metal ions increase adenine nucleotide diffusion both by complexing with the nucleotide thus decreasing the charge on the nucleotide and by increasing the permeability of the lipid bilayer.     

Junctional Membrane Uncoupling : Permeability transformations at a cell membrane junction

The permeability of the membrane surfaces where cells are in contact (junctional membranes) in Chironomus salivary glands depends on Ca⁺⁺ and Mg⁺⁺. When the concentration of these ions at the junctional membranes is raised sufficiently, these normally highly permeable membranes seal off; their permeability falls one to three orders, as they approach the nonjunctional membranes in conductance. This permeability transformation is achieved in three ways: (a) by iontophoresis of Ca⁺⁺ into the cell; (b) by entry of Ca⁺⁺ and/or Mg⁺⁺ from the extracellular fluid into the cell through leaks in the cell surface membrane (e.g., injury); or (c) by entry of these ions through leaks arising, probably primarily in the perijunctional insulation, due to trypsin digestion, anisotonicity, alkalinity, or chelation. Ca⁺⁺ and Mg⁺⁺ appear to have three roles in the junctional coupling processes: (a) in the permeability of the junctional membranes; (b) in the permeability of the perijunctional insulation; and (c) a role long known— in the mechanical stability of the cell junction. The two latter roles may well be closely interdependent, but the first is clearly independent of the others.     

Loss of membrane cholesterol influences lysosomal permeability to potassium ions and protons

Cholesterol is an essential component of lysosomal membranes. In this study, we investigated the effects of membrane cholesterol on the permeability of rat liver lysosomes to K⁺ and H⁺, and the organelle stability. Through the measurements of lysosomal β-hexosaminidase free activity, membrane potential, membrane fluidity, intra-lysosomal pH, and lysosomal proton leakage, we established that methyl-β-cyclodextrin (MβCD)-produced loss of membrane cholesterol could increase the lysosomal permeability to both potassium ions and protons, and fluidize the lysosomal membranes. As a result, potassium ions entered the lysosomes through K⁺/H⁺ exchange, which produced osmotic imbalance across the membranes and osmotically destabilized the lysosomes. In addition, treatment of the lysosomes with MβCD caused leakage of the lysosomal protons and raised the intra-lysosomal pH. The results indicate that membrane cholesterol plays important roles in the maintenance of the lysosomal limited permeability to K⁺ and H⁺. Loss of this membrane sterol is critical for the organelle acidification and stability.     

The comparative transport of K+ and Rb+ in normal and malignant rat tissuesin vivo and in liver slices,diaphragm, and tumor slicesin vitro

Summary The selectivity in the steady state uptakes of Rb⁺ and K⁺ has been studied in a number of normal and malignant rat tissues. The selectivity is minimal in erythrocytes and the two fastest-growing of four transplantable tumors, in which there is little discrimination between the two ions, and ranges upwards to a maximum Rb⁺ uptake in liver. In each tissue, the selectivity is independent of Rb⁺ concentration or of K⁺ deficiency (except in skeletal muscle). In liver slicesin vitro, reduction of energy metabolism by lowering the temperature or by the addition of metabolic inhibitors reduces the Rb⁺K⁺ discrimination proportionately much more than K⁺ transport. Diaphragm and slices of a transplantable tumor give similar results. With temperature reduction, there is a logarithmic relation between the Rb⁺K⁺ discrimination ratio and the respiration rate of liver slices. The results are quantitatively accounted for by simultaneous diffusion and metabolically coupled transport across a homogeneous membrane in which Rb⁺ transport is more closely coupled than that of K⁺ to a metabolic flux across the membrane. There is evidence that the tissue differences in Rb⁺K⁺ selectivity originate in the different levels of the coupling metabolic flux in different cell types and thus of the energy expenditure on ion transport. In contrast to the differences in steady state selectivity between Rb⁺ and K⁺, the initial ratio of uptakes of trace⁴³K and⁸⁶Rb, in otherwise steady state conditions, is close to unity in both liver and tumor slices, in agreement with theoretical calculations.     

Study of the neurotoxic complex and its components from the venom of the Bulgarian sand viper Vipera ammodytes ammodytes: Interaction of the acidic component with cations

Addition of alkali metal ions (Li⁺, Na⁺, K⁺, Rb⁺) to the solution of isolated component A of the viper neurotoxic complex was found to pronouncedly change the protein fluorescence properties. The maximal effect takes place at the addition of potassium salts which induce the fluorescence spectral shift toward shorter wavelengths by 13.5 nm. This effect is dependent on the protein concentration and is evidence that alkali ions induce the oligomerization of component A. The oligomerization equilibrium constants are strongly dependent on both the concentration and the kind of alkali ions inducing it. The presence in the solution of Tris strongly inhibits the oligomerization. The process is temperature dependent and the oligomerization is maximal at 35–50 °C. An attempt was made to check the assumption that component A can increase the K⁺ permeability of phospholipid membranes (liposomes). The results confirmed qualitatively this assumption. Possible functional significance of these findings is discussed.     

Pathophysiology of mitochondrial volume homeostasis: Potassium transport and permeability transition

Regulation of mitochondrial volume is a key issue in cellular pathophysiology. Mitochondrial volume and shape changes can occur following regulated fission-fusion events, which are modulated by a complex network of cytosolic and mitochondrial proteins; and through regulation of ion transport across the inner membrane. In this review we will cover mitochondrial volume homeostasis that depends on (i) monovalent cation transport across the inner membrane, a regulated process that couples electrophoretic K⁺ influx on K⁺ channels to K⁺ extrusion through the K⁺-H⁺ exchanger; (ii) the permeability transition, a loss of inner membrane permeability that may be instrumental in triggering cell death. Specific emphasis will be placed on molecular advances on the nature of the transport protein(s) involved, and/or on diseases that depend on mitochondrial volume dysregulation.     

Interactions between ions and the axon plasma membrane: Effects of cations and anions on the axonal cholinergic binding macromolecule of lobster nerves

Summary It has been demonstrated that cations and ions interact directly with the axonal cholinergic binding macromolecule (ACBM) from lobster walking leg nerves. This interaction results in an increased affinity for binding of [³H] nicotine. The action sequence for the enhancement effect is Na⁺>K⁺>Li⁺>Rb⁺>Cs⁺ while the anion sequence is I^–>Br^–>Cl^–>F^–. These results have been interpreted in terms of Eisenman's theory of equilibrium cation specificity in an attempt to acquire information about the ion binding sites on the ACBM. The mechanism of the enhancement of nicotine binding to the ACBM may serve as a model for studying the conformational changes arising from binding of ions to axonal macromolecules.     

CONTRIBUTION TO THE THEORY OF PERMEABILITY OF MEMBRANES FOR ELECTROLYTES

From experiments on such membranes as apple skin, parchment paper membrane, and a membrane of completely dry collodion, results have been obtained which could be interpreted by the assumption that these membranes are less permeable for anions than for cations. In parchment paper there is only a relative diminution of the mobility of the anions, in the apple skin and in the dry collodion membrane there is practically no permeability for anions at all. The theory is developed which explains how the decrease or complete lack of mobility of anions influences the electromotive effects of the membrane and the diffusibility of electrolytes across a membrane. The results of the theory are compared with the experimental results. In membranes impermeable for anions the permeability for cations gives the same order of cations as for the mobilities in a free aqueous solution. But the differences of the mobilities are enormously magnified, e.g. the mobilities of H^• and Li^•, which are in the proportion of about 1:10 in aqueous solution, are in proportion of about 1:900 in the collodion membrane. The general cause for the retardation of ionic mobility within the membrane may be supposed to be the increased friction of the water envelope dragged along by the ion in the capillary canals of the membrane. The difference of the effect on the cations and on the anions may be attributed to the electric charge of the walls of the canals.