Non-bilayer formation in the DPPE-DPPG vesicle system induced by deep rough mutant of Salmonella minnesota R595 lipopolysaccharide

The vesicle system consisting of 80 mol% dipalmitoylphosphatidylethanolamine (DPPE) and 20 mol% dipalmitoylphosphatidylglycerol (DPPG) undergoes to structural changes caused by various concentrations of Salmonella minnesota R595 lipopolysaccharide (LPS). The phenomenon was investigated by methods applying small- and wide-angle X-ray scattering (SAXS and WAXS), calorimetry (DSC) and freeze-fracture. In the low LPS concentration regime (investigated at 0.02 LPS/DPPE–DPPG molar ratio) a phase separation was observed. Two kind of domains are formed which are rich and poor in DPPE and in these domains cubic and lamellar structures are present, respectively. Increasing the LPS concentration up to 0.1 LPS/DPPE–DPPG molar ratio the phase separation is more expressed and the temperature domains of the phase transitions are more different. Increasing the temperature chain melting of the lamellar phase occurs first and destruction of the cubic phase is observed later. At high LPS concentration (equimolar ratio of LPS/DPPE–DPPG), where this amphiphilic molecule cannot be considered any more a guest molecule, the cubic structure dominates the phase behaviour of the LPS molecules.     

Distortion of the lamellar arrangement of phospholipids by deep rough mutant lipopolysaccharide from <Emphasis Type="Italic">Salmonella minnesota</Emphasis>

Summary The concentration dependent effects of deep rough mutant lipopolysaccharide (LPS) from Salmonella minnesota (R595) on two different phospholipid model membranes was investigated by differential scanning calorimetry and small-angle X-ray scattering (SAXS). At low concentrations of LPS the well ordered multilamellar arrangement of dipalmitoylphosphatidylcholine (DPPC) vesicles is strongly distorted resulting in a loss of positional correlation of the lipid lamellae and smaller domain sizes within the lamellae. The pre-transition of DPPC was abolished at a LPS/DPPC molar ratio of 0.1:1 and the main or chain melting transition was strongly broadened. Moreover, the enthalpy was significantly decreased and a transition was hardly detected at an equimolar mixture of LPS/DPPC. LPS also affected the lamellar arrangement of a mixture of dipalmitoylphosphatidylethanolamine (DPPE) and dipalmitoylphosphatidylglycerol (DPPG). Furthermore, a phase separation was observed for this phospholipid mixture resulting in DPPE enriched and depleted domains. Similarly to DPPC, only a weak phase transition was observed at the highest LPS concentration used (LPS/DPPE-DPPG 1:1 mol/mol). SAXS measurements showed that for both systems increasing the concentration of LPS resulted in a concomitant increase of the formation of cubic structures, which are predominant at an equimolar mixture of LPS/phospholipid. However, because of the small number of peaks it was not possible to unambiguously identify the space group of the cubic structure, complicated by the coexistence with a lamellar phase, which was particularly detectable for the LPS/DPPC mixture.     

Vesicle systems for mimicking the effects of 2,4-dichlorophenol on cell membranes

The effect of 2,4-dichlorophenol (DCP) on the phosphatidylethanolamine ( --dipalmitoyl-phosphatidylethanolamine (DPPE))/water liposomes was studied in the temperature domains of the gel and liquid crystalline phases at the DCP/DPPE molar ratios of 10⁻¹ and 10⁻³ by using differential scanning calorimetry (DSC) as well as small and wide angle X-ray scattering (SAXS and WAXS). Different character of the transitions between the gel and the liquid crystalline phases was observed in the lipid/water and by DCP-doped systems. The different DCP concentrations caused similar effects in the change of the layer arrangements of the gel phase, while the perturbation of the subcells of this phase was different. In the liquid crystalline phase, the DCP molecules did not affect the layer structure significantly. The calorimetrical behaviour of the systems were rather correlated to the changes of the subcells than to the layer arrangements.     

Dynamic Behaviors and Morphology Change of Anionic Phospholipid DPPG Monolayer Caused by Bovine Serum Albumin at Air-Water Interface

The interaction between bovine serum albumin (BSA) and the anionic 1.2-dipalmitoyl-snglycero- 3-(phospho-rac-(1-glycerol)) (sodium salt) (DPPG) phospholipid at different subphase pH values was investigated at air-water interface through surface pressure measurements and atomic force microscopy (AFM) observation. By analyzing surface pressure-mean molecular area (π-A) isotherms, the limiting molecular area in the closed packing state-the concentration of BSA (A_lim-[BSA]) curves, the compressibility coefficient-surface pressure (C_S^-1-π) curves and the difference value of mean molecular area-the concentration of BSA (ΔA-[BSA]) curves, we obtained that the mean molecular area of DPPG monolayer became much larger when the concentration of BSA in the subphase increased at pH=3 and 5. But the isotherms had no significant change at different amount of BSA at pH=10. In addition, the amount of BSA molecules adsorbed onto the lipid monolayer reached a threshold value when [BSA]>5×10^-8 mol/L for all pHs. From the surface pressure-time (π-t) data, we obtained that desorption and adsorption processes occurred at pH=3, however, there was only desorption process occurring at pH=5 and 10. These results showed that the interaction mechanism between DPPG and BSA molecules was affected by the pH of subphase. BSA molecules were adsorbed onto the DPPG monolayers mainly through the hydrophobic interaction at pH=3 and 5, and the strength of hydrophobic interaction at pH=3 was stronger than the case of pH=5. At pH=10, a weaker hydrophobic interaction and a stronger electrostatic repulsion existed between DPPG and BSA molecules. AFM images revealed that the pH of subphase and [BSA] could affect the morphology features of the monolayers, which was consistent with these curves. The study provides an important experimental basis and theoretical support to understand the interaction between lipid and BSA at the air-water interface.     

Influence of La3+ on the Phase Behavior and the Pluidity of Phospholipid Bilayers

The influence of La³⁺ on the phase behavior and the fluidity of the negatively charged phospholipid dipalmitoylphosphatidylglycerol(DPPG) bilayers was studied by differential scanning calorimetry (DSC) and FT-Raman spectroscopy. La³⁺, induced a phase separation of DPPG bilayers, and formed three peaks. La³⁺ increased the phase transition temperature of the new peaks, broadened the half width of the DSC signal, and stabilized a gel phase relative to a crystalline phase of DPPG bilayers. La³⁺ was shown to increase interchain order and intermolecular ordering of the lipid lattice, and decreased the fluidity of DPPG bilayers.     

Permeabilization and morphological changes in phosphatidylglycerol bilayers induced by an antimicrobial peptide,tachyplesin I

Tachyplesin I, a broad-spectrum antimicrobial peptide fromTachypleus tridentatus has a basic (+7), amphiphilic, and cyclic -sheet structure. We reported (Matsuzaki K. et al. (1991) Biochim. Biophys. Acta 1070:259–264) that 1) the action mechanism of tachyplesin I may be the permeabilization of bacterial membranes, 2) the peptide specifically permeabilizes acidic phospholipid bilayers, and 3) its Trp² residue is located in the hydrophobic region near the surface of the bilayers. In this paper, we found that tachyplesin I dose-dependently induces not only the permeabilization but also aggregation/fusion and micellization of the phosphatidylglycerol large unilamellar vesicles (100 nm in diameter) either in the gel (L--dipalmitoylphosphatidyl-DL-glycerol (DPPG)) or liquid-crystalline (egg yolk L--phosphatidyl-DL-glycerol (egg PG)) phase, as revealed by light scattering and electron micrograph techniques. The solid DPPG vesicles were more susceptible to the peptide. At peptide to lipid molar ratios (P/L) of 1/500 to 1/200, interpeptide interactions formed a pore through which calcein, a fluorescent dye, can leak out of the vesicles. The pore lifetime was longer in the DPPG vesicles. Further addition of the peptide caused aggregation and/or fusion of the vesicles. At a charge-neutralizingP/L ratio of 1/7, the enlarged vesicles disintegrated into small spherical particles (10–20 nm in diameter). The mechanism for these morphological changes will be discussed.     

Solubilization of negatively charged DPPC/DPPG liposomes by bile salts

The interactions of the bile salts sodium cholate (NaC) and sodium deoxycholate (NaDC) in 0.1 M NaCl (pH 7.4) with membranes composed of 1,2-dipalmitoyl-sn-glycero-3-phosphatidylcholine (DPPC), 1,2-dipalmitoyl-sn-glycero-3-phosphatidylglycerol (DPPG) and mixtures of DPPC and DPPG at molar ratios of 3:1 and 1:1 were studied by means of high-sensitivity isothermal titration calorimetry (ITC), dynamic light scattering (DLS), and differential scanning calorimetry (DSC). The partition coefficients and the transfer enthalpies for the incorporation of bile salt molecules into the phospholipid membranes were determined by ITC. The vesicle-to-micelle transition was investigated by ITC, DLS, and DSC. The phase boundaries for the saturation of the vesicles and their complete solubilization established by ITC were in general agreement with DLS data, but systematic differences could be seen due to the difference in detected physical quantities. Electrostatic repulsion effects between the negatively charged bile salt molecules and the negatively charged membrane surfaces are not limiting factors for the vesicle-to-micelle transition. The membrane packing constraints of the phospholipid molecules and the associated spontaneous curvature of the vesicles play the dominant role. DPPG vesicles are transformed by the bile salts into mixed micelles more easily or similarly compared to DPPC vesicles. The saturation of mixed DPPC/DPPG vesicles requires less bile salt, but to induce the solubilization of the liposomes, significantly higher amounts of bile salt are needed compared to the concentrations required for the solubilization of the pure phospholipid systems. The different solubilization behavior of DPPC/DPPG liposomes compared to the pure liposomes could be due to a specific "extraction" of DPPG into the mixed micelles in the coexistence region.     

Alterations in phospholipid bilayers caused by sodium dodecyl sulphate/triton X-100 mixed systems

The mechanisms governing the subsolubilizing and solubilizing interaction of sodium dodecyl sulphate (SDS)/Triton X-100 mixtures and phosphatidylcholine liposomes were investigated. Permeability alterations were detected as a change in 5(6)-carboxy-fluorescein (CF) released from the interior of vesicles and bilayer solubilization as a decrease in the static light-scattered by liposome suspensions. Three parameters were described as the effective surfactant/lipid molar ratios (Re) at which the surfactant system a) resulted in 50% of CF release (Re _50%CF); b) saturated the liposomes (Re _SAT;c) led to a complete solubilization of these structures (Re _SOL). From these parameters the corresponding surfactant partition coefficientsK _50%CF,K _SAT andK _SOL were determined. The free surfactant concentrationsS _W were lower than the mixed surfactant CMCs at subsolubilizing level, whereas they remained similar to these values during saturation and solubilization of bilayers in all cases. Although theRe increased as the mole fraction of the SDS rose (X _SDS), theK parameters showed a maximum atX _SDS values of about 0.6, 0.4 and 0.2 forK _50%CF,K _SAT andK _SOL respectively. Thus, the higher the surfactant contribution in surfactant/lipid system, the lower theX _SDS at which a maximum bilayer/water partitioning of mixed surfactant systems added took place and, consequently, the lower the influence of the SDS in this maximum bilayer/water partitioning.Abbreviations PC Phosphatidylcholine - PIPES piperazine-1,4 bis (2-ethanesulphonic acid) - SDS sodium dodecyl sulphate - X _SDS mole fraction of sodium dodecyl sulphate in the mixed system - CF 5(6)-carboxyfluorescein - Re effective surfactant/lipid molar ratio - Re _50%CF effective surfactant/lipid molar ratio for 50% CF release - Re _SAT effective surfactant/lipid molar ratio for bilayer saturation - Re _SOL effective surfactant/lipid molar ratio for bilayer solubilization - S _W surfactant concentration in the aqueous medium - S _{W, 50%CF} surfactant concentration in the aqueous medium for 50% CF release - S _{W, SAT} surfactant concentration in the aqueous medium for bilayer saturation - S _{W, SOL} surfactant concentration in the aqueous medium for bilayer solubilization - S _B surfactant concentration in the bilayers - K bilayer/aqueous phase surfactant partition coefficient - K _50%CF bilayer/aqueous phase surfactant partition coefficient for 50% CF release - K _SAT bilayer/aqueous phase surfactant partition coefficient for bilayer saturation - K _SOL bilayer/aqueous phase surfactant partition coefficient for bilayer solubilization - PL phospholipid TLC-FID, thin-layer chromatography/flame ionization detection system - PI polydispersity index - CMC critical micellar concentration - r ² regression coefficient     

脂质体免疫传感器的制备及其应用于测定尿液中2,4-D的量

将4种溶质(以10∶10∶1∶1质量比混合的DPPC、胆固醇、DPPG及DPPE)的混合物22mg,溶于4mL氯仿-异丙醚-甲醇(6+6+1)混合溶剂中。向此溶液中加入0.15mol·L-1亚铁氰化钾溶液1mL,于45℃超声涡旋5min使其包埋于脂质体中。将此脂质体包埋的亚铁氰化钾溶液1mL,通过戊二醛(0.7+99.3)溶液2mL的作用,与200μL 2,4-D免抗体溶液(10.53g.L-1)交联。另将自制MWNT′s修饰的石墨电极插入0.05mol·L-1脂质体-抗体-吡咯溶液中,用循环伏安法在0～0.75V电位区间扫描10次,扫描速率为50mV.s-1。由此制成的免疫传感器应用于测定尿样中2,4-D含量,其线性范围为0.05～2.5 mg·L-1之间,检出限(3S/N)为15.4μg·L-1。     

Effect of cholesterol on diffusion in surfactant bilayers

Biological membranes consist of lipid bilayers with liquid-ordered and liquid-disordered phases. It is believed that cholesterol controls the size of the microdomains in the liquid-ordered phase and thereby affects the mobility as well as the permeability of the membrane. We study this process in a model system consisting of the nonionic surfactant C(12)E(5) and water in the lamellar phase. We measure the diffusion of fluorescent probe molecules (rhodamine B) by fluorescence correlation spectroscopy. For different surfactant to water ratios, we measure how the molecular mobility varies with the amount of cholesterol added. We find that a reduction of the diffusion coefficient is already detectable at a molar ratio of 8 mol % cholesterol.     

Influence of lipidation of GBV-C/HGV NS3 (513-522) and (505-514) peptide sequences on its interaction with mono and bilayers

Two decapeptide fragments of the non-structural hepatitis G NS3 protein (GBV-C/HGV), 513-522 (RGRTGRGRSG) and 505-514 (SAELSMQRRG), as well as their palmitoylated derivatives were synthesized. The physico-chemical properties of the peptides were analyzed in both the absence and presence of the zwitterionic 1,2-dipalmitoyl-sn-glycero-3-phosphatidylcholine (DPPC), the negative 1,2-dipalmitoyl-sn-glycero-3-[phospho-rac-(1-glycerol)] (DPPG) and the positive 1,2-dioeloyl-3-trimethylammonium-propane (DOTAP) lipid monolayers. Based on their high hydrophilic properties, neither parent peptide presented surface activity and their incorporation into lipid monolayers was low. In contrast, their palmitoylated derivatives showed concentration-dependent surface activity and could be inserted into lipid monolayers to varying degrees depending on their sequence. Compression isotherms showed that the presence of palmitoylated peptides in the subphase resulted in a molecular arrangement less condensed than that corresponding to the pure phospholipid. In concordance with the monolayer results, differential scanning calorimetry (DSC) demonstrated that the parent peptides did not have any effect on the thermograms, while the palmitoylated derivatives affected the thermotropic properties of DPPC bilayers.     

Condensed lamellar phase in ternary DNA-DLPC-cationic gemini surfactant system: a small-angle synchrotron X-ray diffraction study

We report on a small-angle synchrotron X-ray diffraction study of dilauroylphosphatidylcholine (DLPC) liposomes aggregated with high molecular DNA in the presence of 1,4-butanediammonium-N,N'-dilauryl-N,N,N',N'-tetramethyl gemini surfactant cations (C12GS). The aggregates prepared at the DLPC/C12GS/DNA phosphate group=2:1:1.6 molar ratio in 0.0015 mol x l(-1) NaCl aqueous solution exhibit Bragg reflections due to lamellar lipid bilayer stacking and the Bragg reflection typical of one-dimensional DNA lattice with parallel strands intercalated between lipid bilayers. In this condensed fluid lamellar L(alpha)(c) phase, the interactions between DNA and charged bilayers damp the thermally induced bilayer undulations. The diffraction data obtained with the mixture of DLPC liposomes and DNA (at DNA phosphate group/DLPC=0.8:1 molar ratio) indicate a DNA-lipid interaction in the absence of C12GS.     

Salicylic acid-induced effects in the mixed-lipid (dipalmitoyl phosphatidylcholine-dipalmitoyl phosphatidylethanolamine) model membrane

The effect of the keratolytic drug salicylic acid (SA) on the thermotropic properties and fluidity of the mixed lipid membrane dipalmitoyl phosphatidylcholine (DPPC)-dipalmitoyl phosphatidylethanolamine (DPPE) had been studied using DSC, (1H and 31P) NMR, SAXS, and dynamic light scattering. The membrane was in multilamellar vesicular (MLV) and unilamellar vesicular (ULV) form with SA/(DPPC+DPPE) molar ratios, R(m), in the range from 0 to 0.5. It was found that the mechanism of interaction of SA with the lipid mixture exhibited similar patterns in both ULV and MLV. Both the NMR and DSC studies indicated that the drug molecules were probably localized in the lipid-water interfacial region neighboring the lipid headgroups or the glycerol moiety. The presence of the drug increased the fluidity of the membrane and the acyl chain order. However, studies on MLV showed that the presence of the drug in high concentration (R(m)0.2), caused destabilization of the DPPC-DPPE mixture, as indicated by the appearance of two endothermic transitions. DSC studies indicated that prolonged equilibration of the membrane led to reduced interaction between the lipid headgroups and the SA molecules. This reduced interaction could be due to the sequestering of the drug molecules into the lipid-water interfacial region, out of proximity to the polar headgroup or glycerol moiety. Effect of inclusion of cholesterol in the membrane systems was also studied.     

Single Lipid Bilayers Constructed on Polymer Cushion Studied by Sum Frequency Generation Vibrational Spectroscopy

Planar solid supported single lipid bilayers on mica, glass, or other inorganic surfaces have been widely used as models for cell membranes. To more closely mimic the cell membrane environment, soft hydrophilic polymer cushions were introduced between the hard inorganic substrate and the lipid bilayer to completely avoid the possible substrate-lipid interactions. In this article, sum frequency generation (SFG) vibrational spectroscopy was used to examine and compare single lipid bilayers assembled on the CaF(2) prism surface and on poly (L-lactic acid) (PLLA) cushion. By using asymmetric lipid bilayers composed of a hydrogenated 1,2-dipalmitoyl-sn-glycerol-3-phosphoglycerol (DPPG) leaflet and a deuterated 1,2-dipalmitoyl-(d62)-sn-glycerol-3-phosphoglycerol (d-DPPG) leaflet, it was shown that the DPPG lipid bilayers deposited on the CaF(2) and PLLA surfaces have similar structures. SFG has also been applied to investigate molecular interactions between an antimicrobial peptide Cecropin P(1) (CP1) and the lipid bilayers on the above two different surfaces. Similar results were again obtained. This research demonstrated that the hydrophilic PLLA cushion can serve as an excellent substrate to support single lipid bilayers. We believe that it can be an important cell membrane model for future studies on transmembrane proteins, for which the possible inorganic substrate-bilayer interactions may affect the protein structure or function.     

Lateral and vertical nanophase separation in Langmuir-Blodgett films of phospholipids and semifluorinated alkanes

It has recently been found that monodisperse surface micelles (hemimicelles) were formed in Langmuir monolayers of the semifluorinated alkane C8F17C16H33 (F8H16) after transfer onto silicon wafers. Grazing incidence X-ray diffraction studies have demonstrated that compression of mixed Langmuir monolayers made from combinations of dipalmitoyl phosphatidylethanolamine (DPPE) and diblock F8H16 in various molar ratios resulted in the complete expulsion of the diblock molecule at high surface pressure. F8H16 then formed a second layer on top of a DPPE-only monolayer, demonstrating a novel type of reversible, pressure-induced, vertical phase separation. Using atomic force microscopy and X-ray reflectivity, we show now that mixed DPPE/F8H16 (1:1.3) Langmuir-Blodgett films transferred onto silicon wafers below 10 mN m(-1) are laterally phase separated and consist of domains of F8H16 surface micelles in coexistence with a monolayer of DPPE. The density of the network of F8H16 surface micelles increases when the surface pressure of transfer increases. Around 10 mN m(-1), the F8H16 surface micelles start to glide on the DPPE monolayer, progressively overlying it, until total coverage is achieved.     

Phase behavior and the partitioning of caveolin-1 scaffolding domain peptides in model lipid bilayers

The membrane binding and model lipid raft interaction of synthetic peptides derived from the caveolin scaffolding domain (CSD) of the protein caveolin-1 have been investigated. CSD peptides bind preferentially to liquid-disordered domains in model lipid bilayers composed of cholesterol and an equimolar ratio of dioleoylphosphatidylcholine (DOPC) and brain sphingomyelin. Three caveolin-1 peptides were studied: the scaffolding domain (residues 83-101), a water-insoluble construct containing residues 89-101, and a water-soluble construct containing residues 89-101. Confocal and fluorescence microscopy investigation shows that the caveolin-1 peptides bind to the more fluid cholesterol-poor phase. The binding of the water-soluble peptide to lipid bilayers was measured using fluorescence correlation spectroscopy (FCS). We measured molar partition coefficients of 10(4) M(-1) between the soluble peptide and phase-separated lipid bilayers and 10(3) M(-1) between the soluble peptide and bilayers with a single liquid phase. Partial phase diagrams for our phase-separating lipid mixture with added caveolin-1 peptides were measured using fluorescence microscopy. The water-soluble peptide did not change the phase morphology or the miscibility transition in giant unilamellar vesicles (GUVs); however, the water-insoluble and full-length CSD peptides lowered the liquid-liquid melting temperature.     

Facile synthesis and intrinsic conductivity of novel pyrrole copolymer nanoparticles with inherent self-stability

Intrinsically self-stabilized nanoparticles of a copolymer from 4-sulfonic diphenylamine (SD) and pyrrole (PY) were facilely synthesized in HCl solution at 10 degrees C by a chemically oxidative polymerization. The critical reaction parameters such as SD/PY ratio, polymerization time, and oxidant species were studied to significantly optimize the polymerization yield, size, conductivity, and solubility of the final copolymer particles. The molecular structure, size, size distribution, and morphology of the particles were analyzed by IR spectroscopy, laser particle-size analysis (LPA), atomic force microscopy, and transmission electron microscopy (TEM). It was found that the polymerization yield of the SD/PY (50/50) copolymers increased dramatically in the initial 2 h of polymerization and then slowly enlarged in the subsequent 22 h. However, the copolymerization yield for the polymerization time of 24 h exhibited a nonlinear dependence on the SD/PY molar ratio, i.e., a maximum at 10/90 and a minimum at 80/20. The number-average diameter, Dn, of the copolymer particles strongly depended on the SD/PY ratio, decreasing rapidly from 6402 to 291 nm as the SD/PY molar ratio changed from 30/70 to 50/50, whereas the polydispersity index, PDI = Dw/Dn (where Dw is the weight-average diameter), surprisingly maintained very small values, decreasing slightly from 1.21 to 1.08. The SD/PY (80/20) copolymer particles prepared with (NH4)2S2O8 as the oxidant had the smallest size of ca. 10 nm by TEM and the lowest Dw/Dn value of 1.03 by LPA, whereas the copolymer particles prepared with FeCl3 as the oxidant exhibited the second smallest size of ca. 20 nm by TEM and the highest conductivity. The conductivity of the SD/PY (50/50) copolymers rose first and then decreased with increasing polymerization time from 10 min to 24 h, exhibiting a maximum (0.217 S/cm) at 12 h. It is of interest that the copolymer particles with SD/PY molar ratios in the range between 50/50 and 80/20 surprisingly exhibited the smallest size, the narrowest size distribution, and the highest conductivity at the same time. In particular, the copolymer nanoparticles exhibited high purity, clean surfaces, good self-stability, high conductivity, and strong chemoresistance that were very important to nanomaterial processibility and application. The obtained copolymers were partially soluble in concentrated H2SO4, demonstrating a new direction for synthesizing a soluble pyrrole copolymer.     

髓鞘碱性蛋白对细胞膜脂质分子DPPC、DPPE单层膜影响机理研究

本文通过Langmuir单层膜的表面压力-平均分子面积(π-A)曲线的测定与分析,分别对髓鞘碱性蛋白(MBP)与细胞膜中不同头部基团脂质分子二棕榈酰基磷脂胆碱(DPPC)和二棕榈酰基磷脂酰乙醇胺(DPPE)在空气/液体界面上的相互作用过程进行了系统研究.实验结果表明:(1)当界面上脂质含量一定时,亚相中随着MBP浓度的增大,DPPC、DPPE单层膜的等温线向平均分子面积较大的方向移动;(2)在单层膜表面压力为10 mN/m时,一个MBP分子分别结合140±3个DPPC分子和100±3个DPPE分子,随着表面压力增大,当MBP分子分别与两种磷脂分子相互作用时,MBP插入到磷脂单层界面的个数逐渐减少;(3)随着蛋白质浓度的增加,脂分子形成的单层膜变得较为疏松,且MBP分子易于插入到分子头部较小的DPPE单层膜中;(4)蛋白质的存在使DPPC单层膜的表面压力逐渐减小,且蛋白质浓度越大表面压力降低越多,DPPC被MBP带入到亚相中越多;(5)对于DPPE单层膜,蛋白质通过与DPPE相互作用插入到界面膜中,引起表面压力增大,且蛋白质浓度越高,压力变化量越大.     

A QUANTITATIVE COMPARISON OF CHLOROPHYLL BILAYERS FORMED WITH AND WITHOUT SOLVENT

Abstract Bimolecular lipid membranes are formed from solutions containing lecithin and chlorophyll- a (chl- a ) in various molar ratios. Both the Mueller-Ruding technique as well as the solvent free, Montal-Mueller technique are used to form bilayers. In both methods, increasing the chl concentration produces greater photosensitivity. The photocurrent/area is about an order of magnitude higher in bilayers formed with the solvent free method, under similar conditions. From the quantum yield calculations, it appears that the higher photocurrent/area obtained with the Montal-Mueller membranes cannot be explained solely due to the greater concentration of pigment molecules in the solvent free system. The possible role of chl—chl interactions are considered.     

Lateral heterogeneity of dipalmitoylphosphatidylethanolamine-cholesterol Langmuir-Blodgett films investigated with imaging time-of-flight secondary ion mass spectrometry and atomic force microscopy

To better understand the influence of cholesterol (CH) on dipalmitoylphosphatidylethanolamine (DPPE), Langmuir-Blodgett (LB) model membranes of DPPE with varying amounts of cholesterol were imaged by time-of-flight secondary ion mass spectrometry (ToF-SIMS) and atomic force microscopy (AFM). Cholesterol has a condensing effect on DPPE that at low cholesterol concentrations results in lateral heterogeneity of the LB monolayer. At 4:1 DPPE/CH, islands of DPPE/CH phase exist with a connected DPPE phase. As the concentration of cholesterol is increased, the percolation threshold is crossed and the DPPE/CH phase islands connect to separate the DPPE phase (2:1 DPPE/CH). Finally, at 50 mol % cholesterol a single homogeneous DPPE/CH phase LB monolayer exists. ToF-SIMS of the DPPE/CH phase provides a lower ion signal for the characteristic lipid fragments and substrate apparently owing to the higher molecular density induced by cholesterol. AFM data indicate that the DPPE/CH phase is lower in height than the DPPE phase. As phosphatidylethanolamine is predominant in the inner lipid leaflet of cellular membranes, this work has implications for the understanding of cholesterol domains in the inner leaflet of cells.