Influence of the level of cholesteryl sulfate in the solubilization of stratum corneum lipid liposomes by sodium dodecyl sulfate

 The role played by cholesteryl sulfate (Chol-sulf) in the solubilization of liposomes modeling the stratum corneum (SC) lipids by sodium dodecyl sulfate (SDS) was studied. We determined the surfactant-to-lipid molar ratios and the bilayer/aqueous phase surfactant partition coefficients of this interaction by varying the proportion of Chol-sulf, the relative proportions of the others lipids remaining constant. These parameters were determined by monitoring the changes in the static light scattering of the system during solubilization. The fact that the free surfactant concentration was always similar to its critical micelle concentration indicates that the liposome solubilization was mainly ruled by the formation of mixed micelles. The SDS ability to saturate and solubilize SC liposomes decreased as the proportion of Chol-sulf in the bilayers increased until a minimum was reached for a Chol-sulf proportion of about 15%. Inversely, the SDS partitioning into liposomes (or affinity with these bilayers) increased as the proportion of Chol-sulf increased until a maximum was reached at similar Chol-sulf proportions (10–15%). Hence, in these Chol-sulf proportions (similar to that existing in the intercellular lipids, which was 10%) the ability of SDS molecules to interact with liposomes exhibits a minimum despite their enhanced partitioning into liposomes. These effects may be related to the reported dependencies of the level of Chol-sulf on the abnormalities in the skin barrier function and on the SC intercellular cohesion. Received: 12 October 1999 Accepted: 20 January 2000     

Diffusion of sodium dodecyl sulfate micelles in agarose gels

The gradient diffusion of ionic sodium dodecyl sulfate micelles in agarose gel was investigated at moderate concentrations above the CMC. Of particular interest were the effects of micelle, gel, and sodium chloride concentration on the micelle diffusivity. Holographic interferometry was used to measure the gradient diffusion coefficient at three sodium chloride concentrations (0, 0.03, 0.10 M), three gel concentrations (0, 1, 2 wt%), and several surfactant concentrations. Time-resolved fluorescence quenching was used to measure aggregation numbers both in solution and gel. The micelle diffusivity increased linearly with surfactant concentration at the two larger sodium chloride concentrations and all gel concentrations. In general, the strength of this effect increased with decreasing sodium chloride concentration and increased with gel concentration. This behavior is evidence of decreasing micelle-micelle electrostatic interactions with increasing sodium chloride concentrations, and increasing excluded volume effects and hydrodynamic screening with increasing gel concentration, respectively. The only exception was at 0.1M sodium chloride and 2 wt% agarose, which showed a slight reduction in the slope compared to 1 wt% agarose. It was found that the concentration effect is quite strong for charged solutes: at a NaCl concentration of 0.03 M in a 2% agarose gel, in a solution with 3% SDS micelles by volume, the micelle diffusion coefficient is doubled relative to its value in the same gel at infinite dilution. The extrapolated, infinite-dilution diffusion coefficients and the rate at which the micelle diffusivity increased with surfactant concentration were compared with predictions of previously published theories in which the micelles are treated as charged, colloidal spheres and the gel as a Brinkman medium. The experimental data and theoretical predictions were in good agreement.     

Ionic quenching of naphthalene fluorescence in sodium dodecyl sulfate micelles

Micellar effects on luminescense of organic compounds or probes are well established, and here we show that quenching is highly favored in aqueous sodium dodecyl sulfate (SDS) micelles, which concentrate a naphthalene probe and cations of lanthanides, transition metals, and noble metals. Interactions have been studied by steady state and time-resolved fluorescence in examining the fluorescence suppression of naphthalene by metal ions in anionic SDS micelles. The quenching is collisional and correlated with the unit charge and the reduction potential of the metal ion. The rate constants, calculated in terms of local metal ion concentrations, are close to the diffusion control limit in the interior of SDS micelles, where the microscopic viscosity decreases the transfer rate, following the Stokes-Einstein relation.     

Salt effects on solute exchange in sodium dodecyl sulfate micelles

We describe the influence of sodium chloride on the rate of solute exchange in aqueous SDS micelles for a water-insoluble solute, a pyrene-containing triglyceride 1. The initially prepared solutions contained a small fraction of micelles containing two molecules of 1 and a large excess of empty micelles. These solutions showed a measurable excimer emission (of intensity I(E)) that was stable for days to weeks in the absence of added salt. Following additions of salt, I(E) decayed exponentially (rate constant, k(obs)) accompanied by an increase in pyrene monomer emission. Values of k(obs) increased strongly with ionic strength (k(obs) similar [Na(+)](4)). There was no contribution of the empty micelle concentration beyond its contribution to the sodium ion concentration. We conclude that the solute exchange involves spontaneous fragmentation of the SDS micelles into two submicelles, each bearing a molecule of 1, which then grow back to normal micelles through condensation of SDS monomers. We propose a model for the fragmentation process in which large amplitude surface fluctuations "pinch off" a subunit that becomes a submicelle. These fluctuations bring sulfate headgroups into close proximity. Fluctuations leading to fission become important only in the presence of sufficient counterion concentration to reduce the electrostatic repulsion between neighboring headgroups.     

Kinetics of solubilization of n-decane and benzene by micellar solutions of sodium dodecyl sulfate

We observed the diminishing of single microscopic oil drops to study the kinetics of solubilization of n-decane and benzene by micellar solutions of sodium dodecyl sulfate (SDS). Each drop is located in a horizontal glass capillary of inner diameter 0.06 cm filled with a thermostated surfactant solution; the small vertical dimension of the cell prevents the appearance of uncontrollable thermal convections. The experiments show that the radius of an n-decane drop decreases linearly with time, whereas for benzene this dependence is nonlinear. To interpret the data, a kinetic model of solubilization is developed. It accounts for the diffusion and capturing of dissolved oil molecules by the surfactant micelles, as well as for the finite rate of oil dissolution at the oil-water interface. By processing the data, we determined the rate constant of solubilization for a given oil and surfactant. It turns out that the elementary act of catching a dissolved oil molecule by a surfactant micelle occurs under a barrier (rather than diffusion) control. The effective rate of solubilization is greater for the oil, which exhibits a higher equilibrium solubility in pure water (benzene), despite the lower value of the solubilization rate constant for this oil.     

Chlorpromazine and sodium dodecyl sulfate mixed micelles investigated by small angle X-ray scattering

Small-angle X-ray scattering (SAXS) studies are reported on the interaction of chlorpromazine (CPZ) with micelles of anionic surfactant sodium dodecyl sulfate (SDS). Isotropic solutions of SDS (40 and 100 mM) at pH 4.0, 7.0, and 9.0 in the absence and presence of CPZ (2-25 mM) were investigated at the National Laboratory of Synchrotron Light (LNLS, Campinas, Brazil). The data were analyzed through the modeling of the micellar form factor and interference function. The results evidence a micellar shape transformation from prolate ellipsoid to cylinder accompanied by micellar growth and surface charge screening as the molar ratio CPZ : SDS increases in the complex. Small ellipsoids with axial ratio nu=1.5+/-0.1 at 40 mM SDS grow and reassemble into cylinder-like aggregates upon 5 mM drug incorporation (1 CPZ : 8 SDS monomers) with a decrease of the micelle surface charge. At 10 mM CPZ : 40 mM SDS cylindrical micelles are totally screened with an axial ratio nu approximately 2.5. The data also indicate the presence of small prolate ellipsoids (nu=1.7+/-0.1) in solutions of 100 mM SDS (no drug) and micellar growth (nu approximately 2.0 and 4.0) when 10 and 25 mM CPZ are added to the system. In the latter case, the aggregate is also better represented by a cylinder-like form. Therefore, our results demonstrate that the axial ratio and shape evolution of the surfactant : phenothiazine complex are both SDS concentration and drug : SDS molar ratio dependent. The drug location close to the SDS polar headgroup region without disrupting in a significant way both the paraffinic hydrophobic core and the polar shell thickness is inferred. SAXS data made it possible to obtain the shapes and dimensions of CPZ/SDS aggregates.     

Pyrene-assisted synthesis of size-controlled gold nanoparticles in sodium dodecyl sulfate micelles

Gold nanoparticles prepared by chemical reduction in sodium dodecyl sulfate (SDS) solution are size-controlled with the addition of pyrene. Micellar electrokinetic capillary chromatography (MEKC) is applied to the system to examine the size and polydispersity of gold nanoparticles and to show that pyrene has the extraordinary effect in decreasing the size and narrowing the dispersity of gold nanoparticles. The MEKC electropherograms further suggest that pyrene could be oxidized by the aqueous Au(III) complexes first. All the reduced Au complexes were then solubilized in the pyrene-SDS micelles. The growth of gold nanoparticles beyond the embryonic stage was subsequently inhibited by the encapsulating SDS and electrophilic pyrene.     

Exchange mechanisms for sodium dodecyl sulfate micelles: high salt concentration

Solute exchange experiments for the pyrene-labeled triglyceride TG-Py solubilized in sodium dodecyl sulfate (SDS) micelles in the presence and absence of salt show that the "observed" rate constant k(obs) for solute exchange varies by over 6 orders of magnitude as the free sodium ion concentration [Na(+)](aq) is varied between 10 and 850 mM. There is a sharp break in the log-log plot of k(obs) versus [Na(+)](aq) in the range of [Na(+)](aq) = 200 mM, with the exchange rate showing a weaker dependence on [Na(+)](aq) above this concentration. Up to 100 mM added NaCl, this exchange takes place essentially exclusively by a micelle fission mechanism in which each submicelle carries off one of the solutes. At higher salt concentrations, a bimolecular process becomes increasingly important. This fusion process, which involves formation of a transient supermicelle followed by fission back to two normal micelles, becomes the dominant process at high salt concentrations. The fission rate appears to level off for salt concentrations above 300-400 mM. These fission and fusion processes are related in an intimate way to the changes in the size and shape of the SDS micelles with increasing salt concentration.     

Inclusions of methylene blue and phenothiazine by β-cyclodextrin in sodium dodecyl sulfate micelles

The inclusions of methylene blue and phenothiazine by β-cyclodextrin (β-CD) in sodium dodecyl sulfate (SDS) micelles and SDS/n-C₅H₁₁OH mixed micelles are studied by fluorescence spectroscopy. β-CD molecules can include monomers of methylene blue only after they have included SDS at a ratio of 1:1. However, phenothiazine can be included in the β-CD cavities even with β-CD concentrations lower than the total SDS concentration in SDS micelles, but not for solutions with SDS/n-C₅H₁₁OH mixed micelles.     

Spectrophotometric determination of sodium dodecyl sulfate with preconcentration by reversed micelles of triton N-42

Micellar preconcentration has been proposed to improve the procedure of spectrophotometric determination of sodium dodecyl sulfate (SDS). It involves quantitative extraction by reversed micelles of Triton N-42 in n-decane and the subsequent formation of an ion associate with methylene blue and azure A upon destruction of the micellar solution by diluting it with a mixture of chloroform and n-decane in the presence of small concentrations of a dye solution. The absence of losses of 10^?7?10^?5 M SDS upon from 5-to 50-fold preconcentration is confirmed by the standard addition method (RSD = 4–5%); the determination limit of SDS equals 5 × 10^?8 M.     

Structure of pravastatin and its complex with sodium dodecyl sulfate micelles studied by NMR spectroscopy

The aim of this work was to study the mechanisms of interaction between pravastatin and cell membranes using model membranes (sodium dodecyl sulfate micelles) by nuclear magnetic resonance spectroscopy methods. On the basis of the nuclear magnetic resonance experiments, it was established that pravastatin can form intermolecular complexes with sodium dodecyl sulfate micelles by the interaction of its hydrophilic groups with the polar surface of the micelle. Conformational features of pravastatin molecule were also studied. Copyright © 2014 John Wiley & Sons, Ltd.     

Enzymatic determination of some pharmaceuticals in direct and reversed sodium dodecyl sulfate micelles

The properties of horseradish peroxidase in sodium dodecyl sulfate (DDS) reversed micelles in benzene-pentanol-water solutions are studied. The potential of the analytical application of direct and reversed DDS micelles is demonstrated using newly developed methods for the determination of peroxidase substrates (hydrogen peroxide and cystein), inhibitor (sulfanylamide), and activator (imidazole) via the oxidation of o-dianisidine (o-D) with hydrogen peroxide.     

The interaction of isomeric hexanediols with sodium dodecyl sulfate and dodecyltrimethylammonium bromide micelles

The micelle formation process for a typical anionic surfactant, sodium dodecyl sulfate, and a typical cationic surfactant, dodecyltrimethylammonium bromide, has been investigated in a series of mixed solvents consisting of different concentrations of isomeric hexanediols (1,2-hexanediol and 1,6-hexanediol) in water. The critical micelle concentrations and the degrees of counterion dissociation of the mixed micelles were obtained from conductance experiments. Luminescence probing experiments have been used to determine the concentration of micelles in solution and, hence, the micellar aggregation numbers of the surfactants in the mixed solvent systems. The alcohol aggregation numbers were determined by combining the partition coefficients (obtained using NMR paramagnetic relaxation enhancement experiments) with the micellar concentrations from the luminescence probing experiments. All these results are interpreted in terms of the difference in the interaction of the isomeric hexanediols with the surfactant as a function of the position of the hydroxyl groups on the six-carbon chain of the alcohol. Received: 28 June 2000/Accepted: 5 July 2000     

Separation and selectivity of benzophenones in micellar electrokinetic chromatography using sodium dodecyl sulfate micelles or sodium cholate modified mixed micelles

The separation and selectivity of nine benzophenones in micellar electrokinetic chromatography (MEKC) using sodium dodecyl sulfate (SDS) micelles or sodium cholate (SC) modified mixed micelles were investigated in the pH range 6.5-8.0. The results indicate that the combined effects of buffer pH and SC concentration can greatly affect the separation and selectivity of benzophenones, particularly for benzophenones possessing a hydroxyl substituent at the 4-position of the aromatic ring with respect to the carbonyl moiety when using SDS-SC mixed micelles. Better separability can be obtained with SDS-SC mixed micelles than with SDS micelles. Complete separation of nine benzophenones in MEKC can be achieved with an appropriate choice of buffer pH and the concentration of SDS micelles or SC modified mixed micelles. The dependence of the migration order of those benzophenones based on their structures and solute-micelle interactions is discussed.     

Hair protein removal by sodium dodecyl sulfate

The effect of sodium dodecyl sulfate (SDS) on protein loss was studied. Three kinds of human hair were tested by rubbing or immersion in water or immersion in SDS solution, at 25, 40 and 70 degrees C. Under friction, hair treated with SDS solution loses seven times more protein than in water, while by immersion, protein loss is roughly two times higher in SDS than in water. Protein loss increases at higher temperatures. Estimated activation energy values for protein loss by immersion are 69+/-22 kJ mol(-1) for blended brown hair; 40+/-12 kJ mol(-1) for blond hair (tip-end region) and 61+/-4 kJ mol(-1) for blond hair (root-end region) for samples treated in water, while 53+/-8, 7+/-5 and 32+/-8 kJ mol(-1) were the corresponding activation energy values for samples treated in 5% SDS solution. These values indicate that protein loss is mainly a diffusion-controlled process. The more damaged the hair, the lower the activation energy and the higher the protein loss. From these data, it can be estimated that daily care shampooing at room temperature will cause opacity and combing difficulties in 1 year and split ends after 3 years by removal of all cuticle layers.     

Supramolecular complex induced by the binding of sodium dodecyl sulfate to PAMAM dendrimers

Isothermal titration calorimetry (ITC) and dynamic light scattering (DLS) were employed to study the spontaneous supramolecular complexation of amine terminated PAMAM dendrimer (G3[EDA] PAMAM-NH2) induced by the binding of an anionic surfactant, sodium dodecyl sulfate (SDS). At pHor=10, the electrostatic binding ceased because the deprotonated PAMAM dendrimer was uncharged, and hence the surfactant-induced supramolecular assembly could not be formed.     

Thermodynamics of protein denaturation by sodium dodecyl sulfate

The anionic surfactant sodium n-dodecyl sulfate (SDS) plays a variety of roles with regard to protein conformation, depending on its concentration. SDS at low concentrations mostly induces the compaction of protein (folding). Examples of this include: the molten globule state of acid-unfolded cytochrome c, associated with enhancement of the exothermic enthalpy values of isothermal titration calorimetry and a reversible profile by differential scanning calorimetry; the enzyme activation and compaction of Aspergillus niger catalase, and relationship of calorimetric enthalpy (ΔH_cal) to van’t Hoff enthalpy (ΔH_VH), which proves the existence of intermolecular and intramolecular interaction during enzyme activation by SDS; the production of a new energetic domain for human apotransferrin and folded state for histone H1 by SDS. SDS at moderate concentrations below the critical micelle concentration (cmc) is a potent denaturant for protein in solution. Protein denaturation is a key method in thermodynamics and binding site analysis and can be used to enhance our understanding of the protein structure-function relationship. The interaction between protein and surfactant, such as SDS, at the cmc level is a complicated interaction, thermodynamically, that should bring about enthalpy correction through micellar dissociation and micelle dilution.