Admicelle-enhanced synchronous fluorescence spectrometry for the selective determination of polycyclic aromatic hydrocarbons in water

A simple and rapid method for the highly sensitive determination of polycyclic aromatic hydrocarbons (PAHs) in water was developed. Benzo[a]pyrene, benzo[k]fluoranthene, perylene, and pyrene in water were concentrated into sodium dodecyl sulfate (SDS)-alumina admicelles. The collection was performed by adding SDS and alumina particles into the sample solution at pH 2. After gentle mixing, the resulting suspension was passed through a membrane filter to collect the SDS admicelles containing highly concentrated PAHs. The filter was placed on a slide glass and then covered admicellar layer with a fused silica glass plate before setting in a fluorescence spectrometer. Benzo[a]pyrene, benzo[k]fluoranthene, perylene, and pyrene were selectively determined by the synchronous fluorescence scan (SFS) analysis with keeping wavelength intervals between excitation and emission to 98, 35, 29, and 45 nm, respectively. Because of the minimum spectral overlapping, 1-40 ng l⁻¹ of benzo[a]pyrene, benzo[k]fluoranthene, and perylene as well as 10-150 ng l⁻¹ of pyrene were selectively determined with eliminating the interferences of other 12 PAHs. The detection limits were 0.3 ng l⁻¹ for benzo[a]pyrene, benzo[k]fluoranthene, and perylene, and 1 ng l⁻¹ for pyrene. They were 2-3 orders of magnitude lower than the detection limits in normal aqueous micellar solutions. The application to water analysis was studied.     

Swelling of poly(ethylene oxide) gel in aqueous solutions of sodium dodecyl sulfate with added sodium chloride

The swelling behavior of poly(ethylene oxide) (PEO) gels in aqueous solutions of sodium dodecyl sulfate (SDS) with and without NaCl was investigated. In the absence of NaCl, PEO gels with different degrees of cross-linking began to swell from a concentration lower than the critical micelle concentration (cmc) of SDS, then showed sigmoidal enhancements of swelling in a higher SDS concentration region until the degrees of swelling reached maximum values. The SDS concentration at which the swelling began to appear was in reasonable agreement with the critical aggregation concentration (cac) value reported for the aqueous PEO system. For the cases where NaCl was present, the swelling behavior of PEO gel was different from that when NaCl was absent in the following way. The concentrations where the swelling begins to appear, and hence those where the degree of swelling rises steeply, decreased with an increase in NaCl concentration. The ultimate degrees of swelling at higher concentration regions also decreased with an increase in the NaCl concentration. The lowering of the SDS concentrations at which the PEO gel began to swell is in line with the decreases in the cmc of SDS solutions containing NaCl and also with the decreases in the cac of PEO solution. Electronic Publication     

Capillary zone electrophoresis with indirect UV detection: Determination of sodium dodecyl sulfate in simulated stream water

SDS (sodium dodecyl sulfate) has been quantitatively determined by capillary zone electrophoresis using a fused silica capillary and a 5 mM dihydroxybenzoic acid / sodium hydroxide buffer in 5% methanol solution at a pH of 8.1. The ion was detected by indirect UV absorption at 250 nm. Detection range was from 0.8 to 50 mg SDS/L. This rapid method requiring only small sample volumes was developed in support of an aquatic toxicology study in a simulated stream water and is applicable to waters containing common inorganic ions.     

Effects of nonionic surfactant and sodium dodecyl sulfate layers on electroacoustics of hexadecane/water emulsions

Hexadecane-in-water emulsion droplets were formed in a homogeniser in the presence of a mixture of an anionic surfactant (sodium dodecyl sulfate, SDS) and nonionic surfactants of various chain lengths [nonylphenol ethoxylate (C₉φE_N, N=100, 40 and 30) or an alcohol ethoxylate (Brij35)]. The dynamic mobility of the oil droplets was then measured using a flow-through version of an AcoustoSizer. Large changes were observed in the dynamic mobility of the particles formed with the mixed surfactants compared to particles formed with SDS alone. O'Brien's “gel layer” model was employed to interpret the data. The characteristics of the adsorbed layer appeared to be similar whether the nonionic surfactant was adsorbed concurrently with the SDS as the emulsion formed or was merely added afterwards to the emulsion established. The particle size, the charge and the molar fraction of SDS had virtually no effect. The layers formed with the nonionic surfactants decreased in thickness with decreasing molecular weight as expected. Passage through the homogeniser itself had no effect on the properties of the largest nonionic surfactant and, hence, on the adsorption layer formed with it. Received: 4 October 2000 Accepted: 16 October 2000     

Resonance light-scattering method for the determination of BSA and HSA with sodium dodecyl benzene sulfonate or sodium lauryl sulfate

A new resonance light-scattering (RLS) assay of proteins such as bovine serum albumin (BSA) and human serum albumin (HSA) is presented. In the medium of phosphoric acid (pH=2.6), the weak RLS of sodium dodecyl benzene sulfonate (SDBS) or sodium lauryl sulfate (SLS) can be greatly enhanced by proteins, owing to interaction between the protein and the anionic surfactant and formation of an associate. The RLS intensity of the SDBS–protein system is stronger than that of the SLS–protein system under same experimental conditions. It is considered that the synergistic resonance caused by the absorption of both protein and SDBS could produce strong RLS, while absorption of protein only in the SLS system could cause relatively weak RLS. The enhanced intensity of RLS is proportional to the concentration of the protein. If SDBS is used as the probe the linear range is 7.5×10^–9–1.5×10^–5 g mL^–1 for BSA and 1.0×10^–8–1.0×10^–5 g mL^–1 for HSA. The detection limits are 1.8 and 2.8 ng mL^–1, respectively. When SLS is used as the probe the linear range is 2.0×10^–8–1.0×10^–5 g mL^–1 and 2.5×10^–8–1.0×10^–5 g mL^–1 for BSA and HSA, respectively, and the detection limits are 12.8 and 21.6 ng mL^–1, respectively. The biological mimics samples are synthetic concoctions of BSA and HSA with some interferents. In these samples, the concentration of interferents is higher than the concentration normally existing in organisms. The samples were determined satisfactorily.     

A direct calorimetric determination of denaturation enthalpy for lysozyme in sodium dodecyl sulfate

Thermodynamics of the interaction between sodium dodecyl sulfate (SDS) with lysozyme were investigated at pH 7.0 and 27 °C in phosphate buffer by isothermal titration calorimetry. A new method to follow protein denaturation, and the effect of surfactants on the stability of proteins was introduced. The new solvation model was used to reproduce the enthalpies of lysozyme–SDS interaction over the whole range of SDS concentrations. The solvation parameters recovered from the new equation, attributed to the structural change of lysozyme and its biological activity. At low concentrations of SDS, the binding is mainly electrostatic, with some simultaneous interaction of the hydrophobic tail with nearby hydrophobic patches on the lysozyme. These initial interactions presumably cause some protein unfolding and expose additional hydrophobic sites. The enthalpy of denaturation is 160.81 ± 0.02 kJ mol⁻¹ for SDS.     

Thermodynamic and aggregation properties of sodium dodecyl sulfate in aqueous binary mixtures of isomeric butanediols

The effect of aqueous binary mixtures of isomeric butanediols on the micellization of sodium dodecyl sulfate has been investigated. Conductivity and fluorescence techniques were employed to determine the critical micellar concentration, the degree of dissociation of the counterions and the aggregation numbers of the surfactants in these binary blends. Differential conductivity plots were employed to distinguish between the cooperative and the stepwise aggregation process of the surfactant in each solvent system. The mass-action model was employed to calculate the hydrophobic and the electrostatic contributions to the Gibbs energy of micellization as well as the monomer and the counterion concentrations in the postmicellar region. The thermodynamic parameters calculated for each system indicate that the micellization process occurs more readily in the presence of cosolvent owing to the formation of mixed micelles. Received: 5 July 2000 Accepted: 25 July 2000     

Capturing sodium dodecyl sulfate-treated protein antigens by antibody affinity electrophoresis

Modifications to antibody affinity electrophoresis for improved detection of proteins have been developed. The bifunctional linker glutaraldehyde is added to the polyacrylamide gel solution for better incorporation of the bait antibody into a distinct region of a 10% w/v polyacrylamide gel. The addition of glutaraldehyde alleviates the need of an electrophoresis buffer with a specific pH. The protein sample to be analyzed is treated with 2% w/v sodium dodecyl sulfate (SDS) to ensure that they carry a negative charge. The negative charge will allow the proteins to migrate towards the cathode and hence pass through the area embedded with the bait antibody. It is observed that electrophoretic migration of bovine serum albumin (BSA) or protein G ceases upon encounter with anti-BSA whereas proteins ovalbumin, beta-lactoglobulin A, and myoglobin migrate freely. However, the addition of 0.1% w/v SDS in the native gel running buffer disrupts the antibody-antigen bond and neither BSA nor protein G can be captured by anti-BSA.     

Photodegradation of polyaromatic hydrocarbons over thin film of TiO2 nanoparticles; a study of intermediate photoproducts

The photocatalytic degradation of saturated aqueous solution of naphthalene and anthracene was studied over thin films of porous TiO₂ particles on glass substrate, prepared by sol–gel process. Surface morphology and structural features were studied by SEM, TEM and Laser Raman Spectroscopy. These films have been found to be very efficient and the total photomineralisation of these organics to carbon dioxide and water occurs in air-equilibrated solution within 1 h. Concentration changes linearly with the illumination time, and high rate constants are obtained for the degradation of these organics. The pH of the solution changes with the irradiation time due to the formation of intermediate photoproducts, e.g., 5,8-dihydroxynaphthaquinone, and 9,10-anthraquinone, etc. Photodegradation mechanism and the detection of reaction intermediates have been discussed in details.     

Microemulsion polymerization of styrene stabilized by sodium dodecyl sulfate and diethylene glycol monoalkyl ether

The effects of the cosurfactants diethylene glycol monoalkyl ether [C _i H_{2 i +1}O(CH₂CH₂O) _j OH (C _i E _j ; i=4, 6 and j=1, 2)] on the formation of an oil-in-water styrene (ST) microemulsion and the subsequent free radical polymerization were studied. For comparison, the data for the C _i H_{2 i +1}OH (C _i OH; i=4, 6) systems obtained from the literature were also included in this work. Sodium dodecyl sulfate was used as the surfactant. The pseudo three-component phase diagram (macroemulsion, microemulsion and lamellar gel phases) was constructed for each cosurfactant. The primary parameters selected for the polymerization study are the concentrations of cosurfactant and styrene. The number of latex particles nucleated is much smaller than that of the microemulsion droplets initially present in the reaction system. Limited flocculation of the latex particles occurs to some extent during polymerization. Among the cosurfactants investigated, the C₄OH-containing polymerization system is the least stable. By contrast, the diethylene glycol monoalkyl ether group of C _i E _j tends to enhance the latex stability. C _i E _j is more effective in stabilizing the ST microemulsion and the subsequent polymerization in comparison with the C _i OH counterpart. Received: 24 December 1999 Accepted: 9 February 2000     

Determination of lead in the presence of morin-5′-sulfonic acid and sodium dodecyl sulfate by adsorptive stripping voltammetry

A simple and sensitive electroanalytical method is developed for the determination of lead by adsorptive stripping voltammetry (AdSV) in the presence of morin-5′-sulfonic acid (MSA) and sodium dodecyl sulfate (SDS). The Pb-MSA complex accumulates on the surface of a hanging mercury drop electrode (HMDE) and peak current is measured by square wave voltammetry (SWV). The complex is reduced at −0.48 V and peak current increases when low concentrations of SDS are added to the sample solution. The experimental variables pH, MSA concentration (C_MSA); accumulation time (t_acc); accumulation potential (E_acc), and SDS concentration (C_SDS), as well as potential interferences, are investigated. Under the optimized conditions (pH 3.2; C_MSA: 0.5 μmol L⁻¹; t_acc: 60 s; E_acc: −0.35 V, and C_SDS: 20 μmol L⁻¹), peak current is proportional to the concentration of Pb(II) over the 0.1-32.0 μg L⁻¹ range, with a detection limit of 0.04 μg L⁻¹. The relative standard deviation for a solution containing 5.0 μg L⁻¹ of Pb(II) solution was 1.5% for seven successive assays. The method was validated by determining Pb(II) in synthetic sea water (ASTM D665) spiked with ICP multi-element standard solution and in certified reference water (GBW08607). Finally, the method was successfully applied to the determination of Pb(II) in tap water and sea water after UV digestion.     

A systematic investigation into the recovery of radioactively labeled proteins from sodium dodecyl sulfate-polyacrylamide gels

We report the results of a systematic investigation designed to optimize a method for quantifying radioactivity in proteins in sodium dodecyl sulfate-polyacrylamide gels. The method involves dissolving appropriately sized pieces of gel in hydrogen peroxide and heating to 70 degrees C overnight followed by liquid scintillation counting. H(2)O(2) had no effect on the count rates of [(14)C]bovine serum albumin (BSA) when counted in a conventional liquid scintillation system, and the count rates remained stable for several days. Temperatures below 70 degrees C resulted in incomplete extraction of radioactivity from gels containing [(14)C]BSA, but there was also a significant reduction in count rates in samples incubated at 80 degrees C. At 70 degrees C recovery was not affected by the amount of sample loaded onto the gel or by the staining procedure (Coomassie Brilliant Blue or SYPRO Ruby). Recoveries were in the range of 89-94%, and the coefficient of variation for five replicate samples was 5-10%. This method offers a reliable way of measuring the amount of radioactivity in proteins that have been separated by electrophoresis. It may be useful, for example, in quantitative metabolic labeling experiments when it is necessary to know precisely how much tracer has been incorporated into a particular protein.     

Interactions between gelatin and sodium dodecyl sulphate: binding isotherm and solution properties

The interaction between sodium dodecyl sulphate (SDS) and gelatin was studied at pH 4.5 and 6.5 where the gelatin is positively charged (i.e.p. 8). At pH 4.5 a SDS/gelatin concentration range was found where gelatin precipitates. At pH 6.5 the SDS-gelatin complex remains soluble although three SDS concentration domains were distinguished where the SDS-gelatin complex had very different affinities for the solvent. Below C₁ the complex was highly surface active but other measurements (viscosity, potentiometry, protons uptake) did not reveal any particular consequence of binding. Between C₁ and C₂ the molecular size decreased (viscosity lowering) upon charge neutralization and collapse about small SDS aggregates (17 SDS molecules per gelatin molecule). Above C₂ a cooperative binding mechanism lead to the formation of SDS aggregates; the complex stretched out and turned strongly hydrophilic (the viscosity increases, low surface activity). At saturation one gelatin molecule bound about 200 SDS molecules. Above the overlap concentration (about 3 wt%) SDS aggregates formed between several gelatin molecules, the viscosity increased continuously with SDS concentration and the binding ratio was lower than in dilute gelatin solutions. A very good correspondence was found between the different analytical data including turbidity, viscosity, surface tension, protons uptake and direct potentiometric SDS binding measurements.     

Studies of the association of chitosan and alkylated chitosan with oppositely charged sodium dodecyl sulfate

Cationic biopolymer chitosan has many applications in food, cosmetic and pharmaceutical industries. Grafting alkylated chains on its backbone can hydrophobically modify this water-soluble polymer.This paper concerns unmodified chitosan, alkylated chitosan and their interactions with a model anionic surfactant, sodium dodecyl sulfate (SDS). The solvent is pH 4 acetic acid solution. The purpose of this study is to highlight the hydrophobicity brought by the alkylated chains by comparing surface tension measurements and rheological properties of hydrophobically modified polymer (HMP) and chitosan solutions at 25 °C.Interactions of chitosan and HMP with surfactant have also been investigated giving information about surface activity and electrical conductivity of such systems. It results that alkylated chitosan/SDS system is more surface active than chitosan/SDS and it offers new potential applications in pharmaceutical and cosmetic fields because of the formation of amphiphilic complexes.     

Rheological properties of a surfactant-induced gel for the lysozyme–sodium dodecyl sulfate–water system

Rheological properties of isotropic solutions and gel structures of lysozyme–sodium dodecyl sulfate mixtures in water are investigated. Isotropic solutions behave as Newtonian fluids with very low viscosity values. For the lysozyme solutions the intrinsic viscosity and the Huggins coefficient were calculated on the basis of the Mooney equation. Above a certain yield stress value, the viscosity of the gel samples decreases continuously in the whole range of the shear rate. Dynamic rheological experiments show weak gel behavior where the storage modulus and the loss modulus are almost parallel and are frequency-dependent. A belated gel stage with very slow kinetics has been characterized. There is a substantial enhancement of the gel strength by ageing since the belated gel stage manifests a higher yield stress value and a higher storage modulus than the initial gel stage. The gels are stable in the temperature range between 10 and 32 °C.     

Combined sorption/transport of sodium dodecyl sulfate and hydrochloric acid in a blend of cellulose acetate butyrate with cellulose acetate hydrogen phthalate

The transport of hydrochloric acid (0.001-0.1 M) and sodium dodecyl sulfate (0.001-0.1 M) has been measured through a membrane consisting of a blend of cellulose acetate butyrate and cellulose acetate hydrogen phthalate. The cellulose derivative blend is suggested to suffer an alteration in the degree of hydrophobicity when in equilibrium with sodium dodecyl sulfate (SDS) through hemimicelle formation. An increase in surface hydrophobicity of the blend when in equilibrium with SDS solution was observed by fluorescence measurements using the vibronic bands of the probe pyrene, as well as by water desorption kinetics; a decrease of the effective diffusion coefficients from 1.2 × 10⁻¹¹ m² s⁻¹ in the absence of SDS to approximately 2 × 10⁻¹³ m² s⁻¹ in its presence was found. The value obtained for the mutual diffusion coefficient of HCl in the concentration range 0.001-0.1 M (D=4.2×10⁻¹⁴ m² s⁻¹) shows also that the membrane presents hydrophobic features. The flux of SDS in the blend membrane at different pH values shows two distinct permeation rates depending on the cmc. However, from the calculation of permeability coefficients at SDS concentrations below the cmc a clear decrease in P is found, whilst, at concentrations above the cmc the permeability coefficients are nearly constant, only showing a slightly increase. The diffusion coefficients of SDS in the blend increase over the whole SDS concentration range analysed and show an effective diffusion coefficient 2-3 orders of magnitude below the diffusion coefficients of SDS in aqueous solutions. This fact suggests that the only diffusing species are SDS unimers. The presence of HCl in the SDS bulk solution has the effect of increasing the permeability and diffusion coefficients. Mutual analysis of permeation and diffusion coefficients and sorption isotherms shows that, on decreasing the pH, the interactions between SDS and the polymer network decrease. This is also reflected in a clear decrease of the hydrophobic interactions between the diffusing and polymeric species, provoked by a decrease in the unimer-unimer association.     

Detection of coexisting protein conformations in capillary zone electrophoresis subsequent to transient contact with sodium dodecyl sulfate solutions

Non-native conformations of proteins were generated by temporary contact with aqueous solutions of sodium dodecyl sulfate (SDS) and separated from the native state with capillary zone electrophoresis (CZE) in alkaline borate buffer deficient of SDS. Nine proteins at concentrations of 2.0 or 3.0 mg.L(-1) were compared in terms of their susceptibility to SDS. For superoxide dismutase and ferritin the tendency of unfolding was modest with < 25% of the protein being transformed to the non-native state at 10 mmol.L(-1) SDS. Highest susceptibility was observed for albumin, myoglobin (Mb), and hemoglobin with > 75% in the non-native state even at 2.0 mmol.L(-1) SDS. The influence of varying SDS concentrations on the conformational state of Mb was tested. Increasing the SDS concentration, circular dichroism revealed a reduction in alpha-helix, an increase in random coil, and an introduction of beta-sheet, which is absent in native structure. Modifications in the secondary structure were in agreement with distinct changes in the shape of the non-native Mb peak in CZE and make a gradual unfolding/refolding process with several coexisting molten globules instead of two-state transition of conformations most plausible for Mb. CZE was found to contribute to a further understanding of holo-Mb transformation towards a population of non-native conformations (i) by means of calculated peak area ratios of native to non-native states, which showed sigmoid transition, (ii) by detecting the release of the prosthetic heme group, and (iii) by changes in the effective electrophoretic mobility of the Mb-SDS peaks. Reconstituted holo-Mb forms differed in the Soret band around 410 nm, indicating diversity in the conformation of the heme pocket.     

The cooperative binding behavior of sodium dodecyl sulfate to crosslinked chitosan films

The binding behavior of sodium dodecyl sulfate (SDS) to cationic chitosan, in the form of a swollen crosslinked film is described. Chitosan films were crosslinked with epichlorohydrin. Binding isotherms were determined potentiometrically. The binding isotherms of the crosslinked chitosan was compared to the binding isotherms of chitosan in free solution. As expected, a more highly cooperative binding phenomena is observed, than for cationic chitosan in free solution. The collapse of the gel occurs at a binding fraction greater than 0.6. The collapsed cationic chitosan/SDS complex is described. The presence of hydrophobic regions within the chitosan-SDS complex was demonstrated with the oleophilic dyes C.I. Disperse Yellow 23 and C.I. Solvent Green 3. © 1997 John Wiley & Sons, Inc. J Polym Sci A: Polym Chem 35: 3755–3765, 1997     

On-line isotachophoretic preconcentration and gel electrophoretic separation of sodium dodecyl sulfate-proteins on a microchip

A microchip for integrated isotachophoretic (ITP) preconcentration with gel electrophoretic (GE) separation to decrease the detectable concentration of sodium dodecyl sulfate (SDS)-proteins was developed. Each channel of the chip was designed with a long sample injection channel to increase the sample loading and allow stacking the sample into a narrow zone using discontinuous ITP buffers. The pre-concentrated sample was separated in GE mode in sieving polymer solutions. All the analysis steps including injection, preconcentration, and separation of the ITP-GE process were performed continuously, controlled by a high-voltage power source with sequential voltage switching between the analysis steps. Without deteriorating the peak resolution, four SDS-protein analyses with integrated ITP-GE system resulted in a decreased detectable concentration of approximately 40-fold compared to the GE mode only. A good calibration curve for molecular weights of SDS-proteins indicated that the integrated ITP-GE system can be used for qualitative analysis of unknown protein samples.     

Detection of glutathione reductase after electrophoresis on native or sodium dodecyl sulfate polyacrylamide gels

Commercial glutathione reductase (GR) from spinach and yeast (Saccharomyces cerevisiae) were stained on 7.5% native polyacrylamide gel electrophoresis (PAGE) gels or 15% sodium dodecyl sulfate (SDS)-PAGE gels with or without further purification by a 2',5'-ADP Sepharose 4B affinity column. For SDS-PAGE gels, the SDS was removed first by washing twice with 25% isopropanol in 10 mM Tris-HCl (pH 7.9) for 10 min. The gel was then dipped in a 50 mM Tris-HCl buffer (pH 7.9) containing 4.0 mM oxidized glutathione (GSSG), 1.5 mM NADPH, and 2 mM 5,5'-dithiobis(2-nitrobenzoic acid) (DTNB) for 20 min. The GR activity was negatively stained in the dark by a solution containing 1.2 mM 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) and 1.6 mM phenazine methosulfate (PMS) for 5-10 min. The contrast between the clear zone of GR activity and the purple background was found in both native and SDS-PAGE gels. This negative staining method can detect GR as little as 0.064 units and 0.0032 units, respectively, for spinach and yeast sources. Under reduced SDS-PAGE gels, the GR activity band located on 72 kDa for spinach and 51 kDa for yeast. This fast and sensitive method could be used during enzyme purification and for characterization of GR from different sources under different physiological stages or conditions.