Investigation of the influence on conformational transition of DNA induced by cationic lipid vesicles

Recent studies have focused on the structural features of DNA-lipid assemblies. In this paper we take nile blue A (NBA) as a probe molecule to study the influence of the conformational transition of DNA induced by didodecyldimethylammonium bromide (DDAB) cationic vesicles to the interaction between DNA and the probe molecules. We find that upon binding to DNA, a secondary conformational transition of DNA induced by the cationic liposome from the native B-form to the C-form resulted in the change of binding modes of NBA to DNA and different complexes are formed between DNA, DDAB and NBA.     

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 (Tm) of neat DDAB and DODAB in aqueous dispersions are around 16 and 43 degrees C, respectively, and we aim to investigate the Tm behavior for mixtures of these cationic lipids. Overall, DDAB reduces the Tm of DODAB, the transition temperature depending on the DDAB content, but the Tm 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.     

Effects of micelle-to-vesicle transitions on the degree of counterion binding

Effects of micelle-to-vesicle transitions on the degree of counterion binding (beta) were investigated on three systems. For the concentration-dependent micelle-to-vesicle transition in the didodecyldimethylammonium bromide (DDAB)/water system, in the region of coexistent micelles and vesicles, less than 3 mM, the beta values increased significantly with DDAB concentration: beta (0.07 mM)=0.35 and beta (3 mM)=0.93. In the coexistent region, activities of the bromide ion, a(Br), were almost independent of the DDAB concentration, suggesting the pseudo-phase nature of both micelles and vesicles. In the concentration-dependent vesicle-to-lamellar transition region above 5 mM, where multilamellar vesicles were prevailing, on the other hand, the beta values were only little affected by this transition. This suggests that the increase in the layer number of DDAB multilamellar vesicles scarcely affects the beta values. This was also supported by the fact that the destruction of multilamellar vesicles by ultrasonication did not change the beta values. These results strongly suggest that the inner and outer monolayers of DDAB multilamellar vesicles are characterized by similar beta values. The second system, cetyltrimethylammonium bromide (CTAB)/DDAB mixtures, showed composition-dependent transitions depending on the mole fraction of DDAB X(DDAB): spherical micelles (0rodlike micelles (0.2vesicles (0.6相似文献   

The analysis of serum effects on structure,size and toxicity of DDAB–DOPE and DC-Chol–DOPE lipoplexes contributes to explain their different transfection efficiency

The effect of serum on structural properties of dimethyl-dioctadecyl-ammonium bromide (DDAB)–1,2-dioleoyl-sn-glycero-3-phosphoethanolamine (DOPE) liposomes and DDAB–DOPE/DNA lipoplexes has been investigated by energy dispersive X-ray diffraction (EDXD) technique, at different cationic lipid/DNA weight ratios (ρ). The role of serum on the size of lipoplexes has also been studied by dynamic light scattering. Lipoplex transfection efficiency (TE) as a function of ρ, and lipoplex toxicity to C6 rat glioma cells have been evaluated in Dulbecco's Modified Eagle Medium (DMEM) with and without serum. A multi-parametric analysis concerning the role of size, structure and cytotoxicity on transfection efficiency contributes to explain the experimental observation that 3β-[N-(N′,N′-dimethylaminoethane)carbamoyl]-cholesterol (DC-Chol)–DOPE/DNA transfect C6 cells better than DDAB–DOPE/DNA lipoplexes.     

Nanocapsule of cationic liposomes obtained using "in situ" acrylic acid polymerization: stability, surface charge and biocompatibility

In this work, didecyldimethylammonium bromide (DDAB) and 1,2-dioleoyl-sn-glycero-3-phosphatidylethanolamine (DOPE) (2.5:1) were used to prepare liposomes coated with polyacrylic acid (PAA) using "in situ" polymerization with 2.5, 5 and 25 mM of acrylic acid (AA). The PAA concentrations were chosen to achieve partially to fully covered capsules, and the polymerization reaction was observed with real-time monitoring using dynamic light scattering (NanoDLS). The DDAB:DOPE liposomes showed stability in the tested temperature range (25-70°C), whereas the results confirmed the success of the polymerization according to superficial charge (zeta potential of +66.7±1.2 mV) results and AFM images. For the liposomes that were fully coated with PAA (zeta potential of +0.3±3.9 mV), cytotoxicity was independent of the concentration of albumin. Cationic liposomes and nanocapsules of the stable liposomes coated with PAA were obtained by controlling the surface charge, which was the most important factor related to cytotoxicity. Thus, a potential, safe drug nanocarrier was successfully developed in this work.     

Rheological behavior in the didodecyldimethylammonium bromide/water system

The phase behavior in the dilute region of the didodecyldimethylammonium bromide (DDAB)/water system is studied with a battery of techniques. The critical vesicle concentration (cvc), measured by tensiometry, conductimetry, ion-selective-electrode potentiometry and dye solubilization, is similar to the value reported in the literature. Moreover, the combination of surfactant-ion-selective- electrode and bromide-ion-selective-electrode potentiometry indicates that the vesicles are substantially ionized (α ≈ 0.5) in the proximity of the cvc. The transition from small unilamellar vesicles to larger multilamellar liposomes was detected at 0.2 wt% by viscometry, conductimetry and dye solubilization measurements. The rheology of the DDAB/water system was studied as a function of surfactant concentration and temperature. Non- Newtonian behavior, viscoelasticity, yield stresses and time-dependent flow behavior were observed. Maxima and minima in the dynamic moduli and in conductivity are related to structural changes and phase transitions. Moreover, in time-dependent shear flow, the microstructure is modified and the rheological response shifts from thixotropic to antithixotropic or vice versa, depending on the DDAB concentration and the level and duration of the final applied stress. The conductivity behavior in the Lam₁ phase region can be qualitatively explained by the capillary superconductivity theory. This conductivity behavior occurs when the thickness of the aqueous lamella is of the same order of magnitude as the Debye length. Received: 4 January 1999/Accepted in revised form: 1 September 1999     

Complexation of DNA with cationic surfactants as studied by small-angle X-ray scattering

The phase behaviors of the complex formed by didodecyldimethylammonium bromide(DDAB)and cetyltrimethylammonium bromide(CTAB)interacting with three different types of DNAs,salmon testes DNA(~2000 bp),21-bp double-stranded oligonucleotides(oligo-ds DNA),and 21-nt single-stranded oligonucleotides(oligo-ss DNA)were studied by synchrotron small-angle X-ray scattering.It was found that the DNA length and flexibility,together with the positive/negative charge ratio,determined the final structure.At higher charge ratios,the DNA length exhibited negligible effect.Both oligo-ds DNA and salmon DNA formed inverted hexagonal packing of cylinders with CTAB,as well as bilayered lamella with DDAB.However,at lower charge ratios,oligo-ds DNA formed a distorted hexagonal phase with CTAB and a new structure with DDAB,which was different from the behaviors of salmon DNA.The flexible oligo-ss DNA formed rich structures that were subject to environmental disturbance.Kinetic study also indicated that the structures of the complex formed by oligo-ss DNA took much longer to mature than the structures formed by oligo-ds DNA.We attributed this result to the conformational adjustment of oligo-ss DNA in the complex.     

Spontaneous vesicle formation of single chain and double chain cationic surfactant mixtures

The concentration vs composition diagram of aggregate formation of the dodecyltrimethylammonium bromide (DTAB) and didodecyldimethylammonium bromide (DDAB) mixture in aqueous solution at rather dilute region was constructed by analyzing the surface tension, turbidity, and electrical conductivity data and inspected by cryo-TEM images and dynamic light scattering data. Although the aqueous solution of DTAB forms only micelles, the transition from monomer to small aggregates and then to vesicle was found at 0.1 < X2 相似文献   

Alteration in the temperature-dependent content release property of thermosensitive liposomes in plasma

The effect of plasma components on the temperature-dependent content release property of thermosensitive liposomes has been described. Temperature-sensitive liposomes containing mitomycin C (MMC) were prepared from dipalmitoylphosphatidylcholine (DPPC liposomes) and a 7 : 3 mixture of DPPC and dipalmitoylophosphatidylglycerol (DPPC/DPPG liposomes). We defined in this study the difference in the content release between 38 degrees C and 44 degrees C as an index of the temperature-dependent content release efficiency (Delta% release). In the absence of rat plasma, the Delta% release of the DPPC liposomes and the DPPC/DPPG liposomes was 83% and 71%, respectively. However, when the release study was conducted with rat plasma, the Delta% release increased to about 96% for both liposomes. In addition, while the DPPC liposomes were destabilized by rat plasma below the gel-to-liquid crystalline phase transition temperature (T(m)), MMC leakage from the DPPC/DPPG liposomes below T(m) was suppressed by rat plasma. Moreover, the plasma protein binding onto lipid bilayer was concomitant with the gel-to-liquid crystalline phase transition and then enhanced the temperature-dependent release from the DPPC/DPPG liposomes. The possible mechanism of interaction between liposomes and plasma proteins, especially serum albumin, was discussed based on differential scanning calorimetry and protein binding experiments.     

The analysis of serum effects on structure, size and toxicity of DDAB-DOPE and DC-Chol-DOPE lipoplexes contributes to explain their different transfection efficiency

The effect of serum on structural properties of dimethyl-dioctadecyl-ammonium bromide (DDAB)–1,2-dioleoyl-sn-glycero-3-phosphoethanolamine (DOPE) liposomes and DDAB–DOPE/DNA lipoplexes has been investigated by energy dispersive X-ray diffraction (EDXD) technique, at different cationic lipid/DNA weight ratios (ρ). The role of serum on the size of lipoplexes has also been studied by dynamic light scattering. Lipoplex transfection efficiency (TE) as a function of ρ, and lipoplex toxicity to C6 rat glioma cells have been evaluated in Dulbecco's Modified Eagle Medium (DMEM) with and without serum. A multi-parametric analysis concerning the role of size, structure and cytotoxicity on transfection efficiency contributes to explain the experimental observation that 3β-[N-(N′,N′-dimethylaminoethane)carbamoyl]-cholesterol (DC-Chol)–DOPE/DNA transfect C6 cells better than DDAB–DOPE/DNA lipoplexes.     

Sequence-specific binding of DNA to liposomes containing di-alkyl peptide nucleic acid (PNA) amphiphiles

We present a method to covalently attach peptide nucleic acid (PNA) to liposomes by conjugation of PNA peptide to charged amino acids and synthetic di-alkyl lipids ("PNA amphiphile," PNAA) followed by co-extrusion with disteroylphosphatidylcholine (DSPC) and cholesterol. Attachment of four Glu residues and two ethylene oxide spacers to the PNAA was required to confer proper hydration for extrusion and presentation for DNA hybridization. The extent of DNA oligomer binding to 10-mer PNAA liposomes was assessed using capillary zone electrophoresis. Nearly all PNAs on the liposome surface are complexed with a stoichiometric amount of complementary DNA 10-mers after 3-h incubation in pH 8.0 Tris buffer. No binding to PNAA liposomes was observed using DNA 10-mers with a single mismatch. Longer DNA showed a greatly attenuated binding efficiency, likely because of electrostatic repulsion between the PNAA liposome double layer and the DNA backbone. Langmuir isotherms of PNAA:DSPC:chol monolayers indicate miscibility of these components at the compositions used for liposome preparation. PNAA liposomes preserve the high sequence-selectivity of PNAs and emerge as a useful sequence tag for highly sensitive bioanalytical devices.     

牛血红蛋白与双十二烷基二甲基溴化铵相互作用的光谱研究(英文)

运用荧光光谱、紫外-可见吸收光谱和圆二色谱法研究了双十二烷基二甲基溴化铵(DDAB)与牛血红蛋白(Hb)的相互作用。从紫外-可见吸收光谱观察到,随着DDAB的浓度增大,Hb在406nm处的特征吸收峰强度下降,且峰位蓝移,说明DDAB导致血红素辅基微观环境变化。由荧光光谱研究可以得出随着DDAB的浓度增大,Hb在340nm处的荧光强度逐渐增强,说明导致色氨酸荧光淬灭的血红素辅基与色氨酸的距离增大。由Scatchard方程计算了不同温度下该反应的表观结合常数、结合位点数及结合热力学参数,热力学参数的变化表明DDAB与Hb之间以疏水作用力为主。圆二色谱的研究进一步表明DDAB使Hb产生轻微的二级结构改变,α-螺旋含量增加.     

Heme release in myoglobin-DDAB films and its role in electrochemical NO reduction

Electrochemical nitric oxide (NO) reduction by heme groups incorporated in films of didodecyldimethylammonium bromide (DDAB) on pyrolitic graphite was investigated. It is shown that DDAB most likely induces the release of the heme group from myoglobin and therefore myoglobin-DDAB and heme-DDAB films give the same voltammetric responses. This is confirmed by UV/vis spectroscopy showing a clear shift in the Soret band of myoglobin in a DDAB solution. The electrochemical NO reduction on a heme-DDAB film at different pH values reveals the presence of pH-dependent and pH-independent NO reduction pathways. The selectivity of these pathways is probed by combining the rotating ring-disk electrode technique with online electrochemical mass spectroscopy showing that the product of the pH-independent pathway is N2O and the product of the pH-dependent pathway is NH2OH. The preference for one or the other pathway seems to depend on whether a proton or a NO molecule is transferred to a Fe(II)-NO- reaction intermediate and is influenced by pH, NO concentration, and potential.     

Gold nanoparticle multilayer films based on surfactant films as a template: preparation, characterization, and application

Highly ordered gold nanoparticle multilayer films were achieved conveniently using didodecyldimethylammonium bromide (DDAB) films as a template. The template was produced by casting DDAB chloroform solution onto the surface of a (3-aminopropyl)trimethoxysilane-modified indium tin oxide substrate and then evaporating the organic solvent. Gold nanoparticle multilayer films were prepared by soaking the template in 2.6 nm colloidal gold solution for 120 min. The well-ordered superlattice structure of the DDAB template and the gold nanoparticle multilayer films was identified by x-ray diffraction. The characterizations of the gold nanoparticle multilayer films by UV-vis spectroscopy, atomic force microscopy, and cyclic voltammerty were described in detail. The application of the as-prepared gold nanoparticle multilayer films in surface-enhanced Raman spectroscopy (SERS) was investigated by using Rhodamine 6G as a probe molecule. It was found that the colloidal gold nanoparticle multilayer films exhibit remarkable enhancement ability and can be used as SERS substrates.     

Unravelling micellar structure and dynamics in an unusually extensive DDAB/bile salt catanionic solution by rheology and NMR-diffusometry

The mixed didodecyldimethylammonium bromide (DDAB)-sodium taurodeoxycholate (STDC)-(2)H(2)O catanionic system forms a large isotropic (L(1)) phase at 25 degrees C. The evolution of microstructure along different dilution lines has been followed by means of rheology and NMR diffusometry. In general, the L(1) phase is characterised by a weak viscoelasticity and Newtonian response. In the STDC-rich regime (W(s)=[DDAB]/[STDC]=0.2), 5 wt% is an overlapping concentration at which the discrete-to-rodlike micellar transition occurs as indicated from the total surfactant concentration (C(s)) dependency of both zero-shear viscosity (eta(0) approximately C(s)(3.7)) and surfactant self-diffusion (D(s) approximately C(s)(-3.0)). As the surfactant molar ratio (W(s)1) increases, i.e., DDAB concentration increases, and at constant C(s), eta(0) decreases and D(s) increases, indicating the formation of a multiconnected micellar network.     

Structural behaviour of mixed cationic surfactant micelles: a small-angle neutron scattering study

Self-assembly in mixtures of two single-chain cationic surfactants, with different tail lengths (CTAB and DTAB) as well as of a single-chain (DTAB) and a double-chain (DDAB) cationic surfactant, with identical tail lengths, have been investigated with small-angle neutron scattering (SANS) and rationalised in terms of bending elasticity properties. The growth behaviour of micelles with respect to surfactant composition appears completely different in the two surfactant mixtures. DTAB form small oblate spheroidal micelles in presence of [NaBr] = 0.1 M that transform into prolate spheroidal mixed CTAB/DTAB micelles upon adding moderate amounts of CTAB, so as to give a mole fraction y = 0.20 in solution. Most unexpectedly, upon further addition of CTAB the mixed CTAB/DTAB micelles grow with an almost equal rate in both length and width directions to form tablets. In contrast to this behaviour, mixed DDAB/DTAB micelles grow virtually exclusively in the length direction, in presence of [NaBr] = 0.1 M, to form elongated ellipsoidal (tablet-shaped) and subsequently long wormlike micelles as the fraction of DDAB in the micelles increases. Mixed DDAB/DTAB micelles grow to become as long as 2000 Å before an abrupt transition to large bilayer structures occurs. This means that the micelles are much longer at the micelle-to-bilayer transition as compared to the same mixture in absence of added salt. It is found that the point of transition from micelles to bilayers is significantly shifted towards higher fractions of aggregated DTAB as an appreciable amount of salt is added to DDAB/DTAB mixtures, indicating a considerable reduction of the spontaneous curvature with an increasing [NaBr]. By means of deducing the various bending elasticity constants from our experimental results, according to a novel approach by ours, we are able to conclude that the different growth behaviours appear as a consequence of a considerably lower bending rigidity, as well as higher saddle-splay constant, for DDAB/DTAB surfactant mixtures in presence of [NaBr] = 0.1 M, as compared to mixtures of CTAB/DTAB in [NaBr] = 0.1 M and DDAB/DTAB in absence of added salt.     

Interaction of dicarboxylic metalloporphyrins with liposomes. The effect of pH on membrane binding revisited

The acid-base properties of Zn-hematoporphyrin IX (ZnHP) and Zn-mesoporphyrin IX (ZnMP) and the effect of pH on their binding to liposomes have been studied. The ionization constants for the two carboxylate groups of ZnHP were calculated by principal component analysis and are 5.7 +/- 0.1 and 6.9 +/- 0.05. The neutral species and the mono- and dianionic forms all bind to liposomes, but a strong pH effect on the binding constant was observed for both the investigated compounds. We also observed a decrease in the binding of the two anionic species when the membranes carried a negative charge. These results indicate that the porphyrins partition into the membrane with their carboxylic moieties near the lipid-water interface so that their deprotonation, leading to a charged molecule, does not prevent the insertion of the tetrapyrrole ring into the lipid environment of neutral liposomes.     

Cylindrical and Branched Micelles at Low Temperature: A Rheological Study

We investigate the consequence of decreasing the temperature on the rheological behavior of the cylindrical and branched micelles of the ternary system of DDAB (dodecyldimethylammonium bromide)/STDC (sodium taurodeoxycholate)/water system. An isotropic cylindrical micelle-to-hexagonal liquid crystalline phase is optically (as a birefringence) and rheologically (gel like) detected on the STDC rich part at 6°C. On the other hand, branched micellar solution does not show any birefringence upon decreasing the temperature; however, it mainly exhibits disordered-ordered transition under shear. Such transition is more pronounced as the DDAB concentration increases as a consequence of the decrease in the curvature, and hence a sponge phase formation at low temperature.     

Formation of interfacial milk protein complexation to stabilize oil-in-water emulsions against calcium

The interactions between cationic liposomes doped with the anionic nucleolipid 1,2-dipalmitoyl-sn-glycero-3-cytidine diphosphate (DP-Cyt) and deoxyribonucleic acid (DNA) were investigated. Toward this goal, new liposomal and lipoplex formulations characterized by the presence of the anionic amphiphile DP-Cyt were proposed. The effects of incorporation of the cytosine functionalized lipid DP-Cyt into the cationic bilayers were analyzed by means of electrophoretic mobility, dynamic light scattering (DLS) and fluorescence spectroscopy techniques. These approaches allowed us to follow the DNA condensation process and to identify specific electrokinetic characteristics of liposome and DNA-liposome complexes formation. Specifically, DP-Cyt liposomes and DNA were shown to form electrically stable or unstable complexes depending on the charge ratio between the phosphate group of DNA and the cationic lipid. Remarkably, a prominent role for DP-Cyt in enhancing the DNA binding capacity on liposomes was demonstrated. Zeta potential experiments performed on systems with different liposomes/DNA ratio showed that the value of the charge neutralization point is a function of the content of the incorporated DP-Cyt. As a whole, our data demonstrate that the association of cationic DP-Cyt doped liposomes with DNA is driven by both electrostatic interaction and additional specific interactions at the polar head level based on the cytidine nucleobase.     

DNA condensation and its thermal stability influenced by phospholipid bilayer and divalent cations

We studied the effect of divalent alkaline earth metal cations Ca2?, Mg2? and transition metals Co2?, Ni2?, Cu2? and Zn2? on DNA condensation and its protection against thermal denaturation in presence of dioleoylphosphatidylcholine liposomes (DOPC). Experimental results have shown that Ca2? and Mg2? as well as Zn2? mediate DNA condensation. Cu2? causes DNA double helix destabilization, and does not mediate binding between DNA and DOPC liposomes. Co2? and Ni2? can interact with DNA on both ways mentioned above. Static light scattering was use to follow the size of aggregates in DNA condensation process. Phospholipid bilayer and divalent cations protect condensed DNA against thermal destabilization. The highest stabilization effect was found in aggregates with Ca2? and Zn2?, whereas in presence of either Co2? or Ni2? some volume fraction of DNA is denatured.