Cationic liposomes in mixed didodecyldimethylammonium bromide and dioctadecyldimethylammonium bromide aqueous dispersions studied by differential scanning calorimetry, nile red fluorescence, and turbidity

The thermotropic phase behavior of cationic liposomes in mixtures of two of the most investigated liposome-forming double-chain lipids, dioctadecyldimethylammonium bromide (DODAB) and didodecyldimethylammonium bromide (DDAB), was investigated by differential scanning calorimetry (DSC), turbidity, and Nile Red fluorescence. The dispersions were investigated at 1.0 mM total surfactant concentration and varying DODAB and DDAB concentrations. The gel to liquid-crystalline phase transition temperatures (T-m) of neat DDAB and DODAB in aqueous dispersions are around 16 and 43 degrees C, respectively, and we aim to investigate the T-m behavior for mixtures of these cationic lipids. Overall, DDAB reduces the T-m of DODAB, the transition temperature depending on the DDAB content, but the T-m of DDAB is roughly independent of the DODAB concentration. Both DSC and fluorescence measurements show that, within the mixture, at room temperature (ca. 22 degrees C), the DDAB-rich liposomes are in the liquid-crystalline state, whereas the DODAB-rich liposomes are in the gel state. DSC results point to a higher affinity of DDAB for DODAB liposomes than the reverse, resulting in two populations of mixed DDAB/DODAB liposomes with distinctive phase behavior. Fluorescence measurements also show that the presence of a small amount of DODAB in DDAB-rich liposomes causes a pronounced effect in Nile Red emission, due to the increase in liposome size, as inferred from turbidity results.

L’étude des stratégies de séparations préparatrices de protéines par électrophorèse capillaire

La protéomique est un sujet d'intérêt puisque l'étude des fonctions et des structures de protéines est essentiel à la compréhension du fonctionnement d'un organisme donné. Ce projet se situe dans la catégorie des études structurales, ou plus précisément, la séquence primaire en acides aminés pour l’identification d’une protéine. La détermination des protéines commence par l'extraction d'un mélange protéique issu d'un tissu ou d'un fluide biologique pouvant contenir plus de 1000 protéines différentes. Ensuite, des techniques analytiques comme l’électrophorèse en gel polyacrylamide en deux dimensions (2D-SDS-PAGE), qui visent à séparer ce mélange en fonction du point isoélectrique et de la masse molaire des protéines, sont utilisées pour isoler les protéines et pour permettre leur identification par chromatographie liquide and spectrométrie de masse (MS), typiquement. Ce projet s'inspire de ce processus et propose que l'étape de fractionnement de l'extrait protéique avec la 2D-SDS-PAGE soit remplacé ou supporté par de multiples fractionnements en parallèle par électrophorèse capillaire (CE) quasi-multidimensionnelle. Les fractions obtenues, contenant une protéine seule ou un mélange de protéines moins complexe que l’extrait du départ, pourraient ensuite être soumises à des identifications de protéines par cartographie peptidique et cartographie protéique à l’aide des techniques de séparations analytiques et de la MS. Pour obtenir la carte peptidique d'un échantillon, il est nécessaire de procéder à la protéolyse enzymatique ou chimique des protéines purifiées et de séparer les fragments peptidiques issus de cette digestion. Les cartes peptidiques ainsi générées peuvent ensuite être comparées à des échantillons témoins ou les masses exactes des peptides enzymatiques sont soumises à des moteurs de recherche comme MASCOT™, ce qui permet l’identification des protéines en interrogeant les bases de données génomiques. Les avantages exploitables de la CE, par rapport à la 2D-SDS-PAGE, sont sa haute efficacité de séparation, sa rapidité d'analyse et sa facilité d'automatisation. L’un des défis à surmonter est la faible quantité de masse de protéines disponible après analyses en CE, due partiellement à l'adsorption des protéines sur la paroi du capillaire, mais due majoritairement au faible volume d'échantillon en CE. Pour augmenter ce volume, un capillaire de 75 µm était utilisé. Aussi, le volume de la fraction collectée était diminué de 1000 à 100 µL et les fractions étaient accumulées 10 fois; c’est-à-dire que 10 produits de séparations étaient contenu dans chaque fraction. D'un autre côté, l'adsorption de protéines se traduit par la variation de l'aire d'un pic et du temps de migration d'une protéine donnée ce qui influence la reproductibilité de la séparation, un aspect très important puisque 10 séparations cumulatives sont nécessaires pour la collecte de fractions. De nombreuses approches existent pour diminuer ce problème (e.g. les extrêmes de pH de l’électrolyte de fond, les revêtements dynamique ou permanent du capillaire, etc.), mais dans ce mémoire, les études de revêtement portaient sur le bromure de N,N-didodecyl-N,N-dimethylammonium (DDAB), un surfactant qui forme un revêtement semi-permanent sur la paroi du capillaire. La grande majorité du mémoire visait à obtenir une séparation reproductible d'un mélange protéique standard préparé en laboratoire (contenant l’albumine de sérum de bovin, l'anhydrase carbonique, l’α-lactalbumine et la β-lactoglobulin) par CE avec le revêtement DDAB. Les études portées sur le revêtement montraient qu'il était nécessaire de régénérer le revêtement entre chaque injection du mélange de protéines dans les conditions étudiées : la collecte de 5 fractions de 6 min chacune à travers une séparation de 30 min, suivant le processus de régénération du DDAB, et tout ça répété 10 fois. Cependant, l’analyse en CE-UV et en HPLC-MS des fractions collectées ne montraient pas les protéines attendues puisqu'elles semblaient être en-dessous de la limite de détection. De plus, une analyse en MS montrait que le DDAB s’accumule dans les fractions collectées dû à sa désorption de la paroi du capillaire. Pour confirmer que les efforts pour recueillir une quantité de masse de protéine étaient suffisants, la méthode de CE avec détection par fluorescence induite par laser (CE-LIF) était utilisée pour séparer et collecter la protéine, albumine marquée de fluorescéine isothiocyanate (FITC), sans l'utilisation du revêtement DDAB. Ces analyses montraient que l'albumine-FITC était, en fait, présente dans la fraction collecté. La cartographie peptidique a été ensuite réalisée avec succès en employant l’enzyme chymotrypsine pour la digestion et CE-LIF pour obtenir la carte peptidique.

Kinetic asymmetry in the gel-liquid crystalline state transitions of DDAB vesicles studied by differential scanning calorimetry

Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)

Interação de ácido algínico com surfactantes catiônicos em solução aquosa

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES)

Transição vesícula-micela em misturas de dispersões de vesículas com soluções de micelas

Pós-graduação em Biofísica Molecular - IBILCE

Transição vesícula-micela em mistura aquosa de sais dialquilados de amônio quaternário com Pluronic® F127

Pós-graduação em Biofísica Molecular - IBILCE

Carbendazim e modelos de biomembrana via filmes de Langmuir e Layer-by-Layer: mecanismos de interação e desenvolvimento de sensores

Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq)

AFM and SPR studies of protein adsorption at solid/liquid interface

Membrane-like structure formed by surfactant molecules of didodecyldimethylammonium bromide (DDAB) on both HOPG and gold electrodes were studied with AFM and SPR techniques. The study shows that the thickness of the adsorbed layer of DDAB is strongly dependent on the concentration of the vesicle solution. We have also investigated the adsorption of redox protein, Cytochrome c, on graphite electrode with in situ tapping mode AFM. The protein adsorbs spontaneously onto the electrode covered with an adsorbed phosphate layer and forms a uniform monolayer. The adsorbed protein exhibits a reversible electron transfer at 0.17 V (Ag/AgCI) once the electrode potential has been increased to 0.75V. Using surface plasmon resonance spectroscopy we have measured subtle conformational change in protein, Cyt c, due to electron transfer of a single electron on MPA-coated gold electrode. The electron transfer induced change in the resonant angle is about 0.006 deg., which corresponds to ~ 0.2 A decreases in the thickness. This is consistent with that reduced state is more compact than the oxidized state.

Validation of an HPLC analytical method for determination of pancuronium bromide in pharmaceutical injections

Pancuronium bromide is used with general anesthesia in surgery for muscle relaxation and as an aid to intubation. A high performance liquid chromatographic method was fully validated for the quantitative determination of pancuronium bromide in pharmaceutical injectable solutions. The analytical method was performed on an amino column (Luna 150mm4.6mm, 5m). The mobile phase was composed of acetonitrile:water containing 50mmol L-1 of 1-octane sulfonic acid sodium salt (20:80v/v) with a flow rate of 1.0mL min-1 and ultraviolet (UV) detection at 210nm. The proposed analytical method was compared with that described in the British Pharmacopoeia.

Determination of Vecuronium Bromide in Pharmaceuticals: Development, Validation and Comparative Study of HPLC and CZE Analytical Methods

Vecuronium bromide is a neuromuscular blocking agent used for anesthesia to induce skeletal muscle relaxation. HPLC and CZE analytical methods were developed and validated for the quantitative determination of vecuronium bromide. The HPLC method was achieved on an amino column (Luna 150 x 4.6 mm, 5 mu m) using UV detection at 205 nm. The mobile phase was composed of acetonitrile:water containing 25.0 mmol L(-1) of sodium phosphate monobasic (50:50 v/v), pH 4.6 and flow rate of 1.0 mL min(-1). The CZE method was achieved on an uncoated fused-silica capillary (40.0 cm total length, 31.5 cm effective length and 50 mu m i.d.) using indirect UV detection at 230 nm. The electrolyte comprised 1.0 mmol L(-1) of quinine sulfate dihydrate at pH 3.3 and 8.0% of acetonitrile. The results were used to compare both techniques. No significant differences were observed (p > 0.05).

Use of lignin extracted from different plant sources as standards in the spectrophotometric acetyl bromide lignin method

A nongravimetric acetyl bromide lignin (ABL) method was evaluated to quantify lignin concentration in a variety of plant materials. The traditional approach to lignin quantification required extraction of lignin with acidic dioxane and its isolation from each plant sample to construct a standard curve via spectrophotometric analysis. Lignin concentration was then measured in pre-extracted plant cell walls. However, this presented a methodological complexity because extraction and isolation procedures are lengthy and tedious, particularly if there are many samples involved. This work was targeted to simplify lignin quantification. Our hypothesis was that any lignin, regardless of its botanical origin, could be used to construct a standard curve for the purpose of determining lignin concentration in a variety of plants. To test our hypothesis, lignins were isolated from a range of diverse plants and, along with three commercial lignins, standard curves were built and compared among them. Slopes and intercepts derived from these standard curves were close enough to allow utilization of a mean extinction coefficient in the regression equation to estimate : lignin concentration in any plant, independent of its botanical origin. Lignin quantification by use of a common regression equation obviates the steps of lignin extraction, isolation, and standard curve construction, which substantially expedites the ABL method. Acetyl bromide lignin method is a fast, convenient analytical procedure that may routinely be used to quantify lignin.

Drug use evaluation of ipratropium bromide at two tertiary referral hospitals in Brisbane.

Objective: To assess the appropriateness of ipratropium bromide prescribing in two tertiary referral hospitals. Method: Criteria for optimal use were developed based on current literature and modified after consultation with respiratory physicians and clinical pharmacists. A prospective review of prescribing was performed over a 2-month period to assess conformity to these criteria. Results: Information was collected from 84 patients; 5% were receiving inhalers and 96% nebuliser therapy (one patient used both). 77% of patients (n = 65) had a principal diagnosis of chronic obstructive pulmonary disease, 14% (n = 12) asthma and 8% (n = 7) had neither diagnosis. 75% of patients were using ipratropium outside the guidelines. The major areas where the guidelines were not met were a lack of therapeutic justification, use of inappropriate doses, and use of an inappropriate delivery device. Feedback and educational interventions were designed and delivered based on the data obtained. Conclusions: There was widespread use of ipratropium outside the developed guidelines. Interventions in specific areas could lead to significant improvements in the use of this high cost drug

Reversible Photorheology in Solutions of Cetyltrimethylammonium Bromide, Salicylic Acid, and trans-2,4,4 '-Trihydroxychalcone

We show photorheology in aqueous solutions of weakly entangled wormlike micelles prepared with cetyltrimethylammonium bromide (CTAB), salicylic acid (HSal), and dilute amounts of the photochromic multistate compound trans-2,4,4'-trihydroxychalcone (Ct). Different chemical species of Ct are associated with different colorations and propensities to reside within or outside CTAB micelles. A light-induced transfer between the intra- and intermicellar space is used to alter the mean length of wormlike micelles and hence the rheological properties of the fluid, studied in steady-state shear Bow and in dynamic rheological measurements. Light-induced changes of fluid rheology are reversible by a the relaxation process. at relaxation rates which depend on pH and which are consistent with photochromic reversion rates measured by UV-vis absorption spectroscopy. Parameterizing viscoelostic rheological states by their effective relaxation time tau(c) and corresponding response modulus G(c), we find the light and dark states of the system to fall onto a characteristic state curve defined by comparable experiments conducted without photosensitive components. These reference experiments were prepared with the same concentration of CTAB, but different concentrations of HSal or sodium salicylote (NaSal), and tested at different temperatures.

Reduction of QTc interval dispersion. Potential mechanism of cardiac protection of pyridostigmine bromide

OBJECTIVE: Parasympathetic dysfunction is an independent risk factor in individuals with coronary artery disease, and cholinergic stimulation is a potential therapeutical option. We determined the effects of pyridostigmine bromide, a reversible anticholinesterase agent, on electrocardiographic variables of healthy individuals. METHODS: We carried out a cross-sectional, double blind, randomized, placebo-controlled study. We obtained electrocardiographic tracings in 12 simultaneous leads of 10 healthy young individuals at rest before and after oral administration of 45 mg of pyridostigmine or placebo. RESULTS: Pyridostigmine increased RR intervals (before: 886±27 ms vs after: 1054±37 ms) and decreased QTc dispersion (before: 72±9ms vs after: 45±3ms), without changing other electrocardiographic variables (PR segment, QT interval, QTc, and QT dispersion). CONCLUSION: Bradycardia and the reduction in QTc dispersion induced by pyridostigmine may effectively represent a protective mechanism if these results can be reproduced in individuals with cardiovascular diseases.