Aggregation and fusion of vesicles composed of N-palmitoyl derivatives of membrane phospholipids

N-Acylphosphatidylethanolamines and N-acylphosphatidylserines have been isolated from mammalian cells and have been associated with some tissue degenerative changes, although the relationship between their synthesis and the uncontrolled sequence of events that ends in irreversible tissue damage is not completely established. Our results show that monovalent and divalent cations induce aggregation and fusion of liposomes constituted by N-palmitoylphosphatidylethanolamine (NPPE) and N-palmitoylphosphatidylserine (NPPS). The effectiveness of cations to induce the aggregation of NPPE and NPPS liposomes is Ca²⁺>Mg²⁺>>Na⁺. NPPS liposomes aggregate at lower concentrations of divalent cations than NPPE liposomes, but with sodium NPPE liposomes aggregate to a higher extent than NPPS liposomes. The reaction order for the aggregation processes depends on the lipid and the cation nature and range from 1.04 to 1.64. Dynamic light scattering shows an irreversible increase of the size of the aggregates in the presence of all cations tested. The irreversibility of the aggregation process and the intermixing of bilayer lipids, as studied by resonance energy transfer assay, suggest that fusion, rather than aggregation, occurs. The existence of a real fusion was demonstrated by the coalescence of the aqueous contents of both NPPS and NPPE liposomes in the presence of either monovalent or divalent cations. The different binding sensitivity of Ca²⁺ to NPPS and NPPE liposomes, determined by ş potential measurements, agrees with the results obtained in the aggregation and fusion assays. Our results suggest that the synthesis in vivo of N-acylated phospholipids can introduce important changes in membrane-mediated processes.     

Gel shrinking resulting from uneven distribution of ionic micelles between the inside and the outside of the polymer gel network

The volume change of crosslinked nonionic poly (N‐isopropylacrylamide) (NIPA) polymer gel immersed in tetradecyldimethylaminoxide (C14DMAO) surfactant solutions at 0.1M NaCl, were investigated to distinguish between binding and nonbinding polymer gel/C14DMAO surfactants. Also, the aggregation behavior of C14DMAO surfactants the inside and the outside the polymer hydrogels has been studied through solubilization of Sudan III dye. For the C14DMAO surfactants at the degrees of ionization (α) of 0.5 and 1, they bind to the NIPA gel at low surfactant concentration (C_D) that enhance the gel swelling due mainly to the osmotic pressure contribution from the counter ions (regime I, C_D<10mM). However, the deswelling behavior was observed as the surfactant concentration increases above 10 mM (regime II). The solubilization experiments indicated that the surfactant concentration inside the gel is lower than that outside the gel in the regime II, which may be due to the large micelle size that cannot accommodate the mesh size of the gel. It was suggested that the uneven distribution of the ionic micelles leads to the reduction of the net swelling osmotic pressure of the gel (i.e., the decrease of the gel volume). In the case of the nonionic C14DMAO at α = 0, on the other hand, the deswelling behavior was not clearly observed and the surfactant concentration inside the gel and outside the gel was almost identical even at 30 mM. For the nonionic surfactant, it was also found that the gel volume increases with the surfactant concentration at low surfactant concentration less than 1mM. This may be attribute to the dipole‐dipole repulsion of N‐O headgroups. © 2004 Wiley Periodicals, Inc. J Appl Polym Sci 93: 2001–2006, 2004     

Influence of Extractant Aggregation on the Extraction of Trivalent f‐Element Cations by a Tetraalkyldiglycolamide

Abstract

The influence of nitric acid extraction on the aggregation state of 0.10 M N,N,N′,N′‐tetra‐n‐octyl‐3‐oxapentane‐1,5‐diamide (TODGA) in n‐octane or n‐heptane was studied by small‐angle neutron scattering (SANS) and vapor pressure osmometry (VPO). When the equilibrium concentration of nitric acid in the aqueous phase is less than 0.7 M, TODGA exists as a mixture of monomers and dimers. As the aqueous phase acidity is increased, the extractant molecules form higher aggregates containing up to an average of seven molecules of TODGA. The formation of the larger TODGA aggregates takes place over the same range of aqueous acidities where the extraction of trivalent f‐element cations displays a hyperstoichiometric sixth power nitric acid dependence. This suggests that acid‐driven aggregation of TODGA is responsible for the unusual acid and extractant dependencies observed for the extraction of trivalent metal nitrates with this ligand.     

Separation of VOCs from N2 using poly(ether block amide) membranes

This work deals with the separation of volatile organic compounds (VOCs) from nitrogen streams for organic vapour emission control by poly(ether block amide) membranes. As representative air pollutant VOCs, n‐pentane, n‐hexane, cyclohexane, n‐heptane, methanol, ethanol, n‐propanol, n‐butanol, acetone, dimethyl carbonate, and methyl tert‐butyl ether were used in this study. The separation of both binary VOC/N₂ and multicomponent VOCs/N₂ gas mixtures was carried out, and the membranes exhibited good separation performance. A VOC concentration of more than 90 mol% was achieved at a feed VOC concentration of 5 mol%. It was found that the permeances of the VOCs were mainly dominated by their solubilities in the membrane, whereas the permeance of N₂ was affected by the presence of the VOCs. The permeance of N₂ in the VOC/N₂ mixtures was shown to be higher than pure N₂ permeance due to membrane swelling induced by the VOCs dissolved in the membrane. Nevertheless, theVOC/N₂ selectivity increased with an increase in the feed VOC concentration. Among the VOCs studied, the membrane showed a higher permeance to alcohol VOCs than paraffin VOCs. The effects of feed VOC concentration, temperature, stage cut, and permeate pressure on the separation performance were investigated.     

Polyunsaturation in cell membranes and lipid bilayers and its effects on membrane proteins

The effect of variation of the degree ofcis-unsaturation on cell membrane protein functioning was investigated using a model lipid bilayer system and protein kinase C (PKC). This protein is a key element of signal transduction. Furthermore it is representative of a class of extrinsic membrane proteins that show lipid dependent interactions with cell membranes. To test for dependence of activity on the phospholipid unsaturation, experiments were devised using a vesicle assay system consisting of phosphatidylcholine (PC) and phosphatidylserine (PS) in which the unsaturation was systematically varied. Highly purified PKCα and ε were obtained using the baculovirus-insect cell expression system. It was shown that increased PC unsaturation elevated the activity of PKCα. By contrast, increasing the unsaturation of PSdecreased the activity of PKCα, and to a lesser extent PKCε. This result immediately rules out any single lipid bilayer physical parameter, such as lipid order, underlying the effect. It is proposed that while PC unsaturation effects are explainable on the basis of a contribution to membrane surface curvature stress, the effects of PS unsaturation may be due to specific protein-lipid interactions. Overall, the results indicate that altered phospholipid unsaturation in cell membranes that occurs in certain disease states such as chronic alcoholism, or by dietary manipulations, are likely to have profound effects on signal transduction pathways involving PKC and similar proteins.     

Permeability alterations in unilamellar liposomes due to betaine-type zwitterionic and anionic surfactant mixed systems

The alterations caused by betaine-type zwitterionic and anionic surfactant mixed systems in the permeability of unilamellar liposomes have been investigated. The partition coefficient of these systems, at different molar fractions, between the aqueous phase and the lipid bilayer of liposomes has been determined. These surfactant mixed systems were formed byN-dodecyl-N,N-dimethylbetaine (C₁₂-Bet) and sodium dodecyl sulfate (SDS) in the presence of 20 mM PIPES buffer and 110 mM Na₂SO₄, at pH 7.21. Unilamellar liposomes were prepared from egg phosphatidylcholine and phosphatidic acid (9:1 molar ratio). The release of the fluorescent agent 5-(6)-carboxyfluorescein induced by the systems has been studied at sub-solubilizing concentrations. When the molar fraction of C₁₂-Bet/SDS is about 0.4, the critical micelle concentration values of these systems exhibit a minimum, whereas their partition coefficient between the aqueous phase and lipid bilayer of lipid bilayers shows a maximum. There is a consistent correlation between the partition coefficient and the ability of the different systems of surfactants to modify the permeability of liposomes.     

Destabilizing effects of fructose-1,6-bisphosphate on membrane bilayers

Fructose-1,6-bisphosphate (FBP) is a high-energy glycolytic intermediate that decreases the effects of ischemia; it has been used successfully in organ perfusion and preservation. How the cells utilize external FBP to increase energy production and the mechanism by which the molecule crosses the membrane bilayer are unclear. This study examined the effects of FBP on membrane bilayer permeability, membrane fluidity, phospholipid packing, and membrane potential to determine how FBP crosses the membrane bilayer. Large unilamellar vesicles composed of egg phosphatidylcholine (Egg PC) were made and incubated with 50 mM FBP spiked with ¹⁴C-FBP at 30°C. Uptake of FBP was significant (P<0.05) and dependent on the lipid concentration, suggesting that FBP affects membrane, bilayer permeability. With added calcium (10 mM), FBP uptake by lipid vesicles decreased significantly (P<0.05). Addition of either 5 or 50 mM FBP led to a significant increase (P<0.05) in Egg PC carboxyfluorescein leakage. We hypothesized that the membrane-permeabilizing effects of FBP may be due to a destabilization of the membrane bilayer. Small unilamellar vesicles composed of dipalmitoyl pC (DPPC) were made containing either diphenyl-1,3,5-hexatriene (DPH) or trimethylammmonia-DPH (TMA-DPH) and the effects of FBP on the fluorescence anisotropy (FA) of the fluorescent labels examined. FBP caused a significant decrease in the FA of DPH in the liquid crystalline state of DPPC (P<0.05), had no effect on FA of TMA-DPH in the liquid crystalline state of DPPC, but increased the FA of TMA-DPH in the gel state of DPPC. From phase transition measurements with DPPC/DPH or TMA-DPH, we calculated the slope of the phase transition as an indicator of the cooperativity of the DPPC molecules. FBP significantly decreased the slope, suggesting a decrease in fatty acyl chain interaction (P<0.05). The addition of 50 mM FBP caused a significant decrease (P<0.05) in the liquid crystalline/gel state fluorescence ratio of merocyanine 540, indicating increased head-group packing. To determine what effects these changes would have on cellular membranes, we labeled human endothelial cells with the membrane potential probe 3,3′-dipropylthiacarbocyanine iodide (DiSC₃) and then added FBP. FBP caused a significant, dose-dependent decrease in DiSC₃ fluorescence, indicating membrane depolarization. We suggest that FBP destabilizes membrane bilayers by decreasing fatty acyl chain interaction, leading to significant increases in membrane permeability that allow FBP to diffuse into the cell where it can be used as a glycolytic intermediate.     

Adsorption of metal cations from aqueous solutions onto the pH responsive poly(vinylidene fluoride grafted poly(acrylic acid) (PVDF-PAA) membrane

This study investigated the influence of pH of adsorption medium and co-adsorptive metal cations for the adsorption of potassium (K⁺) and magnesium (Mg²⁺) ions onto poly (vinylidene fluoride) grafted poly(acrylic acid) (PAA-PVDF) membrane. At pH 4.8, the adsorption of potassium and magnesium was minimal, because of nearly non-dissociated carboxylic acid groups of PAA-chains, but adsorption increased with increasing ion concentration. The interaction of the studied cations between PVDF-PAA membranes increased considerably at pH 7.0 the dissociation of carboxylic acid groups of PAA. The addition of ionic substances (calcium (Ca²⁺) and sodium (Na⁺) to the adsorption medium reduced the adsorption of potassium and magnesium onto the membrane, because of co-adsorption. Divalent calcium reduced more effectively than univalent sodium the adsorption of potassium and magnesium onto the membrane. In conclusion, co-adsorbing ions reduced the adsorbed amount of potassium and magnesium ions due to binding competition. The percentual adsorbed values suggest that adsorption affinity of studied ions onto the PVDF-PAA membrane followed the order Na⁺ < K⁺ < Mg²⁺ < Ca²⁺. The effect of metal cations on drug adsorption from biological fluids needs research in the future, because e.g. PVDF-PAA membrane has been used in drug separation processes.     

Intermembrane cholesterol transfer: Role of sterol carrier proteins and phosphatidylserine

The effect of phosphatidylserine and sterol carrier proteins on cholesterol exchange was determined using an assay not requiring separation of donor and acceptor membrane vesicles. Sterol carrier protein-2 (SCP₂, also called nonspecific lipid transfer protein), but not fatty acid binding protein (FABP, also called sterol carrier protein), enhanced the initial rate of sterol exchange between neutral zwitterionic phosphatidylcholine small unilamellar vesicles (SUV) 2.3-fold. Phosphatidylserine at 10 mol% increased the initial rate of spontaneous and of SCP₂-mediated (but not FABP-mediated) sterol exchange by 22% and 44-fold, respectively. The SCP₂ potentiation of sterol transfer was dependent on SCP₂ concentration and on phosphatidylserine concentration. The SCP₂-mediated sterol transfer was inhibited by a variety of cations including KCl, divalent metal ions, and neomycin. The data suggest that SCP₂ increase in activity for sterol transfer may be partly ascribed to charge on the phospholipid. A portion of this work was presented as an abstract: Nemecz, G., Butko, P., and Schroeder, f. (1989)Biophysical Journal 55, 137a.     

Docosahexaenoic Acid Incorporation Is Not Affected by Doxorubicin Chemotherapy in either Whole Cell or Lipid Raft Phospholipids of Breast Cancer Cells in vitro and Tumor Phospholipids in vivo

To better understand how docosahexaenoic acid (DHA) improves the effects of doxorubicin (DOX), we examined DHA ± DOX on changes in whole cell and lipid raft phospholipids (PL) of MDA-MB-231 and MCF-7 breast cancer cells. We sought to confirm whether the relative changes in PL DHA content of MDA-MB-231 cells could be extended to PL from MDA-MB-231 tumors grown in mice fed a DHA supplemented diet ±DOX. Treatment with DHA did not change PL composition yet DOX increased the proportion of phosphatidylserine in MCF-7 cell lipid rafts by two-fold (p < 0.001). Regardless of DOX, the relative percent incorporation of DHA was higher in MDA-MB-231 cells compared to MCF-7 cells in phosphatidylserine, phosphatidylethanolamine, and phosphatidylcholine (whole cell and lipid rafts); and higher in phosphatidylethanolamine vs. phosphatidylcholine (4.4-fold in MCF-7 and 6-fold in MDA-MB-231 cells respectively). DHA treatment increased eicosapentaenoic acid and docosapentaenoic acid in MDA-MB-231 cells but not MCF-7 cells. Increased DHA content in MDA-MB-231 cells, MCF-7 cells, and MDA-MB-231 tumors in all PL moieties (except sphingomyelin) corresponded with reduced arachidonic acid (p < 0.05). Feeding mice 2.8% (w/w of fat) DHA ± DOX increased tumor necrotic regions (p < 0.05). This study established differential incorporation of DHA into whole cell and lipid rafts between human breast cancer cell lines. However, within each cell line, this incorporation was not altered by DOX confirming that DOX does not change membrane lipid composition. Furthermore, our findings indicate that membrane changes observed in vitro are translatable to in vivo changes and that DHA + DOX could contribute to the anticancer effects through increased necrosis.     

The effect of beta blocking drugs on lipid peroxidation in rat heartin vitro

Beta-adrenergic receptor blocking drugs include a structurally related class of drugs that are employed clinically to treat a variety of cardiovascular disorders. Since these drugs exert additional nonspecific effects including membrane stabilization, representative samples including atenolol, dilevolol, labetolol, metoprolol and propranolol were studied to determine their influence on lipid peroxidation. Homogenates or liposomes of adult rat hearts were incubated in the presence of various concentrations of propranolol or equivalent concentrations of dilevolol, labetolol, metoprolol or atenolol. Lipid peroxidation was stimulated with 50 μM FeSO₄, 5 μMt-butyl hydroperoxide (homogenates) or 0.2 mM citrate FeSO₄ (liposomes) plus O₂. Lipid peroxidation, as assessed by both the thiobarbituric acid reaction and chemiluminescence, was reduced in a dose-dependent manner as the propranolol concentration was increased from 1 to 10 mM. The five beta-adrenergic receptor blocking drugs reduced lipid peroxidation both in crude homogenates and in liposomes; their effectiveness was related to their lipophilicity. Dilevolol, propranolol, labetolol and metoprolol at a concentration of 20 mM reduced lipid peroxidation by 45%, 37%, 35% and 28%, respectively. The hydrophilic blocker atenolol was ineffective in reducing lipid peroxidation event at elevated concentrations. Lipophilic beta-blocking drugs apparently are capable of exerting an antioxidant effect in protecting membrane lipids against peroxidation.     

The effect of chelation on the selective transport of alkaline earth metal ions in asymmetric cellulose acetate hyperfiltration membranes. II

The effects of chelation on the transport of calcium and magnesium, both separately and in a variety of admixtures, in a controlled series of asymmetric cellulose acetate membranes were characterized. Ethylenediaminetetraacetic acid (EDTA) and ethylenebis(oxyethylenenitrilo)tetraacetic acid (EGTA) were used as chelating agents for the alkaline earth metal ions. Asymmetric cellulose acetate membranes annealed at 70°, 75°, and 85°C were studied. Chelation of each of these alkaline earth metals ions in aqueous solutions at pH 6, by either EDTA or EGTA, significantly increased the overall hyperfiltration rejections of these metals by all the membranes studied. The increase in rejection varied montonically with the fraction of metal ion complexed. The higher rejection of metal chelates, compared to the rejection of unbound metal ions, was considered to be the result of the significantly larger size of the chelated species. Calculations suggested that selective (or competitive) chelation took place at pH 6 in a mixture of calcium and magnesium ions in the presence of a stoichiometrically limiting amount of chelating agent. Calcium successfully competed for most of the available chelating agent in equimolar aqueous solutions of chelating agent, calcium, and magnesium. The calcium rejection was explained primarily in terms of the effects of chelation per se on the effective size of the formed complex even in feeds comprised of these ternary solute mixtures. The complexation reaction between magnesium and EGTA is, however, so unfavorable at pH 6 that the Mg²⁺ ion remains uncomplexed even in the presence of an equivalent amount of EGTA. The observed increased rejection of magnesium ions, therefore, in ternary systems was explained by electroneutrality criteria and by solute–membrane interactions involving the various calcium species and the membranes.     

Lipid exchanges between dioctadecyldimethylammonium bromide monolayer and vesicles in the subphase

Studies on the interaction of lipid monolayer with bilayer structures, such as vesicles, are relatively scarce in the literature. In order to ascertain whether these structures interact for cationic dioctadecyldimethylammonium bromide (DODAB) monolayers at the aqueous surfaces of 0, 0.05, and 0.5 mmol L⁻¹ DODAB vesicle dispersions, differential scanning calorimetry (DSC) and surface film balance experiments were carried out. DSC results confirmed the presence of unilamellar vesicles in the subphase, while changes in the monolayer surface pressure–area per molecule (π–A) isotherm profile yielded by the presence of DODAB vesicle in the subphase revealed monolayer-vesicle interactions as a result of monomer exchanges between the monolayer and the vesicles with stronger effects at the higher vesicle concentration investigated.     

A Double Prodrug with Improved Membrane Permeability over the Parent Chelator HBED Provides Superior Cytoprotection against Hydrogen Peroxide

The clinical use of N,N′‐bis(2‐hydroxybenzyl)ethylenediamine‐N,N′‐diacetic acid (HBED) has been hindered by its lack of bioavailability. N,N′‐bis(2‐boronic pinacol ester benzyl)ethylenediamine‐N,N′‐diacetic acid methyl, ethyl, and isopropyl esters 7 a – c , respectively, and their dimesylate salts 8 a – c , are double prodrugs that mask the two phenolate and two carboxylate donors of HBED as boronic esters and carboxylate esters, respectively. Their activation by chemical hydrolysis and oxidation, their passive diffusivity, and their cytoprotective capabilities have been investigated here. 8 a – c hydrolyzed in minimum essential medium at 37 °C with half‐lives of 0.69, 0.81, and 2.28 h, respectively. The intermediate formed, 9 [N,N′‐bis(2‐boronic acid benzyl)ethylenediamine‐N,N′‐diacetic acid], then underwent oxidative deboronation by H₂O₂ to give HBED (k=1.82 m ^?1 min^?1). Solubility measurements in mineral oil and in phosphate buffer indicated that 7 a had a better balance between lipid and aqueous solubilities than did HBED. 7 a was also able to passively diffuse across a lipid‐like silicone membrane (log flux=?0.36), whereas HBED‐HCl was not. 8 c provided better protection to retinal cells than did HBED against a lethal dose of H₂O₂ (84 % vs. 28 % protection, respectively, at 44 μm ). These results suggest that the double prodrugs have better membrane permeability than does HBED, and therefore could be therapeutically useful for improving the delivery of HBED.     

Synthesis and properties of hydrophobically modified acrylamide-based polysulfobetaines

Acrylamide-based, hydrophobically modified polysulfobetaines containing 3-[N-(2-methacroyloylethyl)-N,N-dimethylammonio]-propane sulfonate (DMAPS) and varying amounts of the hydrophobic monomer stearyl methylacrylate (SMA) were synthesized by micellar copolymerization. The basic physico-chemical properties of the synthesized copolymers were studied by means of surface tension, dynamic laser light scattering, and rheological measurements. All the copolymers showed surface activity when the copolymer concentration was above 0.07 wt%. The dynamic laser light scattering measurement revealed that both zwitterionic and hydrophobic associations were important in copolymer aggregation. The rheological properties of the copolymers in aqueous solution depended on the content of hydrophobic monomer, the copolymer concentration and the addition of salt, which were characteristic of hydrophobically modified polyacrylamide and acrylamide-based polyzwitterions. The critical aggregation concentration of the copolymers was in the range of 0.07–0.1 wt%.     

Investigation of platelet activation and calcium store release by a topical hemostatic xerogel dressing for improved blood clotting

Adequate topical hemostatic dressings are required as first-line approach for reduction of uncontrolled hemorrhage, a leading cause of mortalities. Platelets play a major role during blood clotting to prevent hemorrhage during injuries. Here, we demonstrate the mechanisms activated through protease activating receptor 1 (PAR1), a platelet membrane protein in response to a porous composite xerogel dressing incorporating SiNPs (size 122 ± 10 nm) and calcium (2.5 mM), characterized by scanning electron microscopy–energy dispersive x-ray spectroscopy and Fourier transform infrared spectroscopy. The composite displayed 13.9-fold improved blood clotting index in comparison to commercial dressing. The composite displayed increased platelet aggregation due to development of well-formed pseudopodia as compared to bare xerogel, SFLLRN (a thrombin mimic), adenosine di-phosphate (a platelet activator), and heparin (a thrombin inhibitor). Further, PAR1 gene was significantly upregulated in model A549 epithelial cell line (1.2-fold) and human platelets (1.4-fold). The composite enhanced calcium release and its extrusion in A549 cells. Upregulation of PAR1 on the platelet surface and calcium release are crucial for platelet shape change and aggregation. The data indicate that xerogel composite containing SiNPs and calcium enhanced blood clotting through activation of PAR1. Such dressings can provide a potential hemostatic solution to reduce blood loss, disability, and mortality during surgery and trauma care.     

Effect of n−3 fatty acid supplementation on lipid peroxidation and protein aggregation in rat erythrocyte membranes

Human erythrocytes in the circulation undergo dynamic oxidative damage involving membrane lipid peroxidation and protein aggregation during aging. The present study was undertaken to determine the effect of n−3 fatty acid supplementation on lipid peroxidation and protein aggregation in the circulation and also the in vitro susceptibility of rat erythrocyte membranes to oxidative damage. Wistar male rats were fed a diet containing n−6 fatty acid-rich safflower oil or n−3 fatty acid-rich fish oil with an equal amount of vitamin E for 6 wk. n−3 Fatty acid content in erythrocyte membranes of rats fed fish oil was significantly higher than that of rats fed safflower oil. The degree of membrane lipid peroxidation and protein aggregation of rats fed fish oil was not significantly higher than that of rats fed safflower oil when the amounts of phospholipid hydroper-oxides, thiobarbituric acid-reactive substances, and detergent-insoluble protein aggregates were measured. When isolated erythrocytes were oxidized under aerobic conditions in the presence of Fe(III), the degree of membrane lipid peroxidation of erythrocytes from rats fed fish oil was increased to a greater extent than that of rats fed safflower oil, whereas the degree of membrane protein aggregation of both groups was increased in a similar extent. Hence, n−3 fatty acid supplementation did not affect lipid peroxidation and protein aggregation in membranes of circulating rat erythrocytes, and the supplementation increased the susceptibility of isolated erythrocytes to lipid peroxidation, but not to protein aggregation, under the aerobic conditions. If a sufficient amount of vitamin E is supplied, n−3 fatty acid supplementation may give no undesirable oxidative effects on rat erythrocytes in the circulation.     

Effect of anionic-lipid-molecule geometry on the structure and properties of liposome-polycation complexes

The influence of anionic amphiphilic compounds that have different geometric shapes and become incorporated into bilayers on the polycation-mixed liposome interaction and the structure and properties of the resulting complexes is analyzed. Phosphatidylserine, cardiolipin, and sodium dodecyl phosphate are used as anionic lipids, and poly(N-ethyl-4-vinylpyridinium bromide) and polylysine are used as polycations. Polycation adsorption on the surfaces of all examined types of liposomes is accompanied by the neutralization of their charge, an increase in the size of particles of the systems, and quenching of fluorescence labels. Liposomes whose membranes contain incorporated cylindrical phosphatidylserine molecules retain their integrity during contact with polycations. The resulting complexes quantitatively dissociate into initial components during an increase in the salt concentration in the surrounding solution. In the case of liposomes with asymmetric anionic lipids, that is, cardiolipin and sodium dodecyl phosphate, the conditions of retaining the membrane integrity and reversible complexation are fulfilled only at relatively low molar fractions of both lipids. The obtained data witness the decisive effect of the geometry of anionic lipid molecules on the stability of complexes formed from mixed liposomes and polycations.     

Laboratory RO and NF processes fouling investigation by residence time distribution curves examination

The fouling phenomena of nanofiltration of calcium sulfate saturated feed solution in the presence of magnesium and carbonates as well as the reverse osmosis of saturated silica feedwater with magnesium chloride content at different pH levels, was investigated by analyzing the membrane residence time distribution curves (RTD) in our laboratory. The fraction of degraded membrane (parameter a), the fraction of active membrane area (parameter b) and the fraction of membrane blocked by impermeable layer (parameter c) as a function of permeate recovery was determined. It was found that not only surface blockage affects permeate efficiency, but also other factors, such as module retentate chamber pressure drop and osmotic pressure increase. The membranes RTD measurements as well as fouling, a, b and c parameters, gathered with ion-selective electrodes (chloride, calcium and cupric ion-selective) and appropriate tracer solutions (sodium chloride, calcium chloride and cupric nitrate) were compared with commonly used conductivity sensor and sodium chloride tracer solution. We found that both the tracer and detector type strongly affects membrane mean residence time and its variance, but at the same time no influence of detector and tracer type on membrane fouling a, b and c parameters was observed.