Infrared spectroscopy analysis of mixed DPPC/fibrinogen layer behavior at the air/liquid interface under a continuous compression-expansion condition

The mixed layer behavior of dipalmitoyl phosphatidylcholine (DPPC) with fibrinogen at continuously compressed-expanded air/liquid interfaces was analyzed in situ by infrared reflection-absorption spectroscopy (IRRAS). The reflectance-absorbance (RA) intensities and/or wavenumbers of nu(a)-CH2 and amide I bands for a mixed DPPC/fibrinogen layer at the interface were obtained directly by an infrared spectrometer with a monolayer/grazing angle accessory and a removable Langmuir trough. The nu(a)-CH2 RA intensity-area hysteresis curves of a DPPC monolayer indicate a significant loss of free DPPC molecules at the interface during the first compression stage, which is also supported by the corresponding nu(a)-CH2 wavenumber-area hysteresis curves. For a mixed DPPC/fibrinogen layer at the interface, the amide I RA intensity-area hysteresis curves suggest that the fibrinogen molecules were expelled from the interface upon compression, apparently because of the presence of insoluble DPPC molecules. The squeeze-out of fibrinogen evidently removed a pronounced amount of DPPC from the interface, as judged from the corresponding nu(a)-CH2 intensity and wavenumber data. Moreover, significant adsorption of fibrinogen was found during the subsequent interface expansion stage. With the in situ IRRAS analysis of the mixed layer behavior at the interface, the induced loss of DPPC by fibrinogen expulsion from the compressed interface and the dominant adsorption of fibrinogen to the expanded interface were clearly demonstrated.     

Competitive adsorption of fibrinogen and dipalmitoylphosphatidylcholine at the air/aqueous interface

The competitive adsorption of fibrinogen (FB) and DPPC at the air/aqueous interface, in phosphate buffer saline at 25 degrees C, was studied with tensiometry, infrared reflection absorption spectroscopy (IRRAS), and ellipsometry. For FB/DPPC mixtures with 750 ppm (0.075 wt%) FB and 1000 ppm (0.10 wt%) DPPC, the tension behavior was found to be similar to that of FB when alone, even with DPPC and FB being at the interface. Thus, FB interferes with adsorption of DPPC and inhibits its surface tension lowering ability. When FB protein is introduced in the solution after a DPPC monolayer has formed, the adsorption of FB is inhibited by the DPPC monolayer. When a DPPC monolayer is spread onto a solution with a preadsorbed FB layer, the DPPC monolayer excludes FB from the surface and controls the tension behavior with little inhibition by FB. When a DPPC dispersion is introduced with the Trurnit method, or sprayed dropwise, onto an aqueous FB/DPPC surfaces, the DPPC layer formed on the surface prevents the adsorption of FB and dominates the surface tension behavior. These results have implications in controlling the inhibition of lung surfactant tension behavior by serum proteins, when they leak at the alveolar lining layer, and in developing surfactant replacement therapies for alveolar respiratory diseases.     

Roles of gamma-Globulin in the Dynamic Interfacial Behavior of Mixed Dipalmitoyl Phosphatidylcholine/gamma-Globulin Monolayers at Air/Liquid Interfaces

This study investigated the roles of gamma-globulin in the dynamic interfacial behavior of dipalmitoyl phosphatidylcholine (DPPC)/gamma-globulin monolayers at air/liquid interfaces at 25 degrees C. The surface tension behavior demonstrated that gamma-globulin had a large adsorption time scale. Moreover, the surface pressure-area hysteresis behavior of adsorbed gamma-globulin monolayers suggested that no significant desorption occurred during the compression stage, and the respreading of gamma-globulin molecules at the interface during the expansion stage was slow. From the hysteresis behavior of adsorbed gamma-globulin monolayers with spread DPPC molecules, it was found that gamma-globulin molecules were expelled from the interface as DPPC molecules were in a condensed state. The squeeze-out of gamma-globulin molecules seemed to induce the loss of DPPC molecules at the interface with the extent depending on the initial gamma-globulin surface concentration. Furthermore, the expelled gamma-globulin molecules re-entered the monolayer and participated in the surface pressure increase during the following expansion stage. The exclusion of gamma-globulin associated with the removal of DPPC during monolayer compression and the re-entry of gamma-globulin during subsequent monolayer expansion represented a mechanism for DPPC depletion and gamma-globulin enrichment at the interface, which may explain the inhibitory effect of certain proteins on the surface activity of DPPC. Copyright 2000 Academic Press.     

Adsorption of bovine serum albumin at the air/water interface and its effect on the formation of DPPC surface film

The adsorption of bovine serum albumin (BSA) at the air/water interface and its effect on the transport of dipalmitoylphosphatidylcholine (DPPC) to form a surface film were studied with tensiometry, infrared reflection absorption spectroscopy (IRRAS), and ellipsometry. For 1, 10, 100, and 1000 ppm BSA solutions, the steady-state tension ranges from 55 to 50 mN m⁻¹. At pulsating area (at 20 cycles min⁻¹), both the minimum and maximum tensions decrease with increasing bulk concentration. Even though the steady-state tension is similar for 100 and 1000 ppm BSA, IRRAS and ellipsometry results indicate that the adsorbed density is higher for 1000 ppm BSA. For 1000 ppm/1000 ppm BSA/DPPC mixture, the tension behavior was found to be similar to that of 1000 ppm BSA when alone. Results from IRRAS and ellipsometry also demonstrate that BSA is the dominant adsorbed component at the air/water interface. Thus, at 1000 ppm, by adsorbing fast and possibly irreversibly, BSA interferes with the transport and adsorption of DPPC and inhibits its ability to lower the surface tension. However, when DPPC is introduced via a spread monolayer mechanism, DPPC expels partly or completely the adsorbed BSA monolayer and then controls the tension behavior with little or no inhibition by BSA. Thus, the competitive adsorption of DPPC and BSA depends strongly on the path or mechanism of introducing DPPC to the surface and involves path-dependent nonequilibrium adsorption phenomena.     

Interaction of Dipalmitoyl Phosphatidylcholine with n‐Hexadecanol in Monolayer and Liposome

The monolayer collapse behavior of n‐hexadecanol/dipalmitoyl phosphatidylcholine (DPPC) was investigated in this study at the air/water interface at 37 °C. Surface pressure variations with time for the mixed monolayers of DPPC with 20 mol% and 50 mol% n‐hexadecanol at corresponding collapse points were recorded by a Langmuir trough system. In addition, the interaction of n‐hexadecanol with a pure DPPC monolayer was identified by fluorescence microscopy (FM). The results demonstrated distinct differences between these systems; according to our observation, the higher the ratio of n‐hexadecanol to DPPC, the more nucleation domains can be induced. The FM images demonstrated that pronounced domain formation was associated with a longer relaxation time of the collapsed DPPC and DPPC/n‐hexadecanol monolayers, and the presence of n‐hexadecanol appeared to enhance the relaxation processes. The liposome was prepared by the thin‐film hydration method. The average diameter of DPPC and DPPC/n‐hexadecanol liposomes was investigated by dynamic light scattering. It is shown that the diameter of DPPC liposome with n‐hexadecanol is smaller than pure DPPC liposome at the initial state. After 24 hours, DPPC/n‐hexadecanol liposome became larger than pure DPPC liposome and lasted for the next four days. The effects of a greater ratio of n‐hexadecanol did not play an important role in DPPC liposome formation based on our dynamic light scattering analysis. Our result demonstrated that n‐hexadecanol might affect the DPPC liposome stability. The increased ratio of n‐hexadecanol in DPPC liposomes could only a play a minor role in DPPC liposome fusion.     

Effects of cholesterol component on molecular interactions between paclitaxel and phospholipid within the lipid monolayer at the air-water interface

Cholesterol is a main component of the cell membrane and could have significant effects on drug-cell membrane interactions and thus the therapeutic efficacy of the drug. It also plays an important role in liposomal formulation of drugs for controlled and targeted delivery. In this research, Langmuir film technique, atomic force microscopy (AFM) and Fourier transform infrared spectroscopy (FTIR) are employed for a systematic investigation on the effects of cholesterol component on the molecular interactions between a prototype antineoplastic drug (paclitaxel) and 1,2-dipalmitoyl-sn-glycerol-3-phosphocholine (DPPC) within the cell membrane by using the lipid monolayer at the air-water interface as a model of the lipid bilayer membrane and the biological cell membrane. Analysis of the measured surface pressure (pi) versus molecular area (a) isotherms of the mixed DPPC/paclitaxel/cholesterol monolayers at various molar ratios shows that DPPC, paclitaxel and cholesterol can form a non-ideal miscible system at the air-water interface. Cholesterol enhances the intermolecular forces between paclitaxel and DPPC, produces an area-condensing effect and thus makes the mixed monolayer more stable. Investigation of paclitaxel penetration into the mixed DPPC/cholesterol monolayer shows that the existence of cholesterol in the DPPC monolayer can considerably restrict the drug penetration into the monolayer, which may have clinical significance for diseases of high cholesterol. FTIR and AFM investigation on the mixed monolayer deposited on solid surface confirmed the obtained results.     

Preparation and structure evolution of bowknot-like calcium carbonate particles in the presence of poly(sodium 4-styrene sulfate)

We determined how glucose or insulin interacts with a phospholipid monolayer at the air/water interface and explained these mechanisms from a physico-chemical point of view. The 1,2-dipalmitoyl-2-sn-glycero-3-phosphatidylcholine (DPPC) monolayer at an air/water interface acted as a model membrane, which allowed the effect of the molecular packing density in the monolayer on the interactions to be determined. The interaction of glucose, insulin, and a mixture of glucose and insulin to the DPPC monolayer were investigated via surface pressure-area per molecule Langmuir isotherms and fluorescence microscopy. Glucose adsorbed to the underside of the DPPC monolayer, while insulin was able to penetrate through the monolayer when the phospholipid molecules were not densely packed. The presence of a mixture of insulin and glucose affected the molecular packing in the DPPC monolayer differently than the pure insulin or glucose solutions, and the glucose-insulin mixture was seen to be able to penetrate through the monolayer. These results indicated that glucose and insulin interact with one another, giving a material that may then transported through a pore in the monolayer or through the spaces between the molecules of the monolayer.     

Thermodynamic characteristics and Langmuir-Blodgett deposition behavior of mixed DPPA/DPPC monolayers at air/liquid interfaces

The role of dipalmitoylphosphatic acid (DPPA) as a transfer promoter to enhance the Langmuir-Blodgett (LB) deposition of a dipalmitoylphosphatidylcholine (DPPC) monolayer at air/liquid interfaces was investigated, and the effects of Ca2+ ions in the subphase were discussed. The miscibility of the two components at air/liquid interfaces was evaluated by surface pressure-area per molecule isotherms, thermodynamic analysis, and by the direct observation of Brewster angle microscopy (BAM). Multilayer LB deposition behavior of the mixed DPPA/DPPC monolayers was then studied by transferring the monolayers onto hydrophilic glass plates at a surface pressure of 30 mN/m. The results showed that the two components, DPPA and DPPC, were miscible in a monolayer on both subphases of pure water and 0.2 mM CaCl2 solution. However, an exception occurs between X(DPPA)=0.2 and 0.5 at air/CaCl2-solution interface, where a partially miscible monolayer with phase separation may occur. Negative deviations in the excess area analysis were found for the mixed monolayer system, indicating the existence of attractive interactions between DPPA and DPPC molecules in the monolayers. The monolayers were stable at the surface pressure of 30 mN/m for the following LB deposition as evaluated from the area relaxation behavior. It was found that the presence of Ca2+ ions had a stabilization effect for DPPA-rich monolayers, probably due to the association of negatively charged DPPA molecules with Ca2+ ions. Moreover, the Ca2+ ions may enhance the adhesion of DPPA polar groups to a glass surface and the interactions between DPPA polar groups in the multilayer LB film structure. As a result, Y-type multilayer LB films containing DPPC could be fabricated from the mixed DPPA/DPPC monolayers with the presence of Ca2+ ions.     

Vitamin D(2) modulates melittin-membrane interactions

In the present work, mutual interaction of melittin, a pore forming hemolytic toxin from bee venom, and vitamin D(2), an antioxidant steroid, with dipalmitoyl phosphatidylcholine (DPPC) multilamellar liposomes has been investigated. Turbidity and Fourier transform infrared (FTIR) spectroscopic measurements, in combination with thermodynamic calculations, were used to monitor the modulating effect of vitamin D(2) on a melittin-DPPC membrane system. The results indicate that melittin on its own decreases the main phase transition to lower temperatures and also dramatically decreases the stability of the membrane. It has an overall disordering effect on the phospholipid membrane structures. Inclusion of vitamin D(2) at low concentrations (3, 6 mol%) into melittin containing DPPC liposomes slightly shifts the main phase transition to lower temperatures. High concentration of vitamin D(2) (9 mol%) has a more dramatic effect in shifting the main phase transition to lower temperature. It also causes a significant broadening in the phase transition curve. The present study also demonstrates that, with the addition of vitamin D(2) into melittin-DPPC system, absorbance value in turbidity study and the frequency of the CH(2) stretching band in FTIR study changes in a manner that are consistent with a reduction in the membrane perturbing effect of melittin on DPPC liposomes. Vitamin D(2) diminishes the disordering effect of melittin on DPPC lipids and produces a more ordered membrane system. These results were confirmed with thermodynamic calculations.     

New protocols for preparing dipalmitoylphosphatidylcholine dispersions and controlling surface tension and competitive adsorption with albumin at the air/aqueous interface

The adsorption behavior of dipalmitoylphosphatidylcholine (DPPC), which is the major component of lung surfactant, at the air/aqueous interface and the competitive adsorption with bovine serum albumin (BSA) were studied with tensiometry, infrared reflection absorption spectroscopy (IRRAS), and ellipsometry. Dynamic surface tensions lower than 1 mN/m were observed for DPPC dispersions, with mostly vesicles, prepared with new protocols, involving extensive sonication above 50 °C. The lipid adsorbs faster and more extensively for DPPC dispersions with vesicles than with liposomes. For DPPC dispersions by a certain preparation procedure at T > T_c, when lipid particles were observed on the surface, dynamic surface tensions as low as 1 mN/m were measured. Moreover, IRRAS intensities and ellipsometric δΔ values were found to be much higher than the values for other DPPC dispersions or spread DPPC monolayers, suggesting that a larger amount of liposomes or vesicles adsorb on the surface. For DPPC/BSA mixtures, the tension behavior is controlled primarily by BSA, which prevents the formation of a dense DPPC monolayer. When BSA is injected into the subphase with a spread DPPC monolayer or into a DPPC dispersion with preadsorbed layers, little or no BSA adsorbs and the DPPC layer remains on the surface. When a DPPC monolayer is spread on a BSA solution at 0.1 wt% at 25 °C, then DPPC lipid can displace the adsorbed BSA molecules. The lack of BSA adsorption, and the expulsion of BSA by DPPC monolayer is probably due to the strong hydrophilicity of the lipid polar headgroup. When a DPPC dispersion is introduced with Trurnit's method or when dispersion drops are sprayed onto the surface of a DPPC/BSA mixture, the surface tension becomes lower and is controlled by DPPC, which can prevent the adsorption of BSA. The results may be important in understanding inhibition of lung surfactants by serum proteins and in designing efficient protocols of surfactant preparation and administration.     

Action mechanism of water soluble ethanol on phospholipid monolayers using a quartz crystal oscillator

Interaction between phospholipid monolayers (dihexadecyl phosphate: DHP, dipalmitoyl phosphatidyl choline: DPPC) and water soluble ethanol has been studied using quartz crystal microbalance (QCM) method and quartz crystal impedance (QCI) method. The quartz crystal oscillator was attached horizontally on the DHP and DPPC monolayers that were formed on the water surface. At low concentration, increased ethanol concentration decreased the frequency for QCM and increased the resistance for QCI. Both frequency and resistance approached asymptotically to a saturation value. A further increase in ethanol concentration induced a sudden and discontinuous linear change (a decrease in frequency and an increase in resistance). Based on these results, we propose the following action mechanism of ethanol on phospholipid monolayers: at low concentration, the ethanol hydrates adsorb into the monolayer/water interface and saturate on the interface. The monolayer viscosity also increases with the adsorption of hydrates. A further increase in concentration causes multilayer formation of hydrates and/or penetration of hydrates into the monolayer core. The viscosity of the interfacial layer (monolayer and interfacial structured water) changes dramatically according to the action of ethanol hydrates.     

Insertion mechanism of a poly(ethylene oxide)-poly(butylene oxide) block copolymer into a DPPC monolayer

Interactions between amphiphilic block copolymers and lipids are of medical interest for applications such as drug delivery and the restoration of damaged cell membranes. A series of monodisperse poly(ethylene oxide)-poly(butylene oxide) (EOBO) block copolymers were obtained with two ratios of hydrophilic/hydrophobic block lengths. We have explored the surface activity of EOBO at a clean interface and under 1,2-dipalmitoyl-sn-glycero-3-phosphocholine (DPPC) monolayers as a simple cell membrane model. At the same subphase concentration, EOBO achieved higher equilibrium surface pressures under DPPC compared to a bare interface, and the surface activity was improved with longer poly(butylene oxide) blocks. Further investigation of the DPPC/EOBO monolayers showed that combined films exhibited similar surface rheology compared to pure DPPC at the same surface pressures. DPPC/EOBO phase separation was observed in fluorescently doped monolayers, and within the liquid-expanded liquid-condensed coexistence region for DPPC, EOBO did not drastically alter the liquid-condensed domain shapes. Grazing incidence X-ray diffraction (GIXD) and X-ray reflectivity (XRR) quantitatively confirmed that the lattice spacings and tilt of DPPC in lipid-rich regions of the monolayer were nearly equivalent to those of a pure DPPC monolayer at the same surface pressures.     

Cratylia mollis lectin at the air–aqueous solution interface: adsorption and lectin–lipid interactions

The interfacial behaviour of Cratylia mollis (Cra) at the air/water interface and its penetrant ability into spread phospholipid monolayers (Lipoid E80 and Epicuron 200) has been monitored by surface tension measurements. The first-order rate constants defining adsorption and rearrangement obtained from surface tension kinetics data reveal that Cra is a rather stable protein which exhibits characteristic protein adsorption patterns in which the breaking points separating diffusion–penetration and rearrangement profiles could have been easily distinguished. The penetration of Cra into Lipoid E80 and Epicuron 200 phospholipid monolayers has been inferred in terms of penetration pressure increments (ΔΠ) versus time relationships. The data clearly showed that penetrant ability of the lectin was, to a large extent, dependent on monolayer compressibilities. Thus, for Lipoid E80, which contained a rather high percentage of phosphatidylethanolamine (DPPE) in the mixture with phosphatidylcholine (DPPC), penetration of Cra at the high monolayer compression (20 mN m⁻¹) was lower than that observed for Epicuron 200, which did not contain DPPE. Indeed, in the middle of the Π-A isotherm, DPPE was markedly less compressible than DPPC. However, at the low monolayer surface coverage (3 mN m⁻¹), the rates of Cra penetration into both Lipoid E80 and Epicuron 200, although much higher for the latter at the beginning of adsorption, yielded similar limiting values of ΔΠ. This has been attributed to the occurrence of a hydrophobic interaction between the lectin and hydrophobic phospholipid chains that have the same length for both Lipoid E80 and Epicuron 200.     

On the interaction of dipalmitoyl phosphatidylcholine with normal long-chain alcohols in a mixed monolayer: a thermodynamic study

This study investigated the mixed monolayer behavior of dipalmitoyl phosphatidylcholine (DPPC) with normal long-chain alcohols at the air/water interface. Surface pressure–area isotherms of mixed DPPC/C₁₈OH and DPPC/C₂₀OH monolayers at 37°C were obtained and compared with previous results for the mixed DPPC/C₁₆OH system. The negative deviations from additivity of the areas and the variation of the collapse pressure with composition imply that DPPC and long-chain alcohols were miscible and formed non-ideal monolayers at the interface. At lower surface pressures, it seems that the attractive intermolecular force was dominant in molecular packing in the mixed monolayers. At higher surface pressures, the data suggest that the molecular packing in mixed DPPC/C₁₆OH monolayers may be favored by the packing efficiency or geometric accommodation. Furthermore, negative values of excess free energy of mixing were obtained and became significant as the hydrocarbon chain length of alcohols increased, which indicates there were attractive interactions between DPPC and long-chain alcohols. In each free energy of mixing–composition curve, there was only one minimum and thus a phase separation did not exist for mixed DPPC/long-chain alcohol monolayers.     

Interaction of ovalbumin with phospholipids Langmuir-Blodgett film

Interaction of native ovalbumin (OVA) with 1,2-dipalmitoyl-sn-glycero-3-phosphocholine (DPPC) Langmuir-Blodgett monolayer has been studied at the air-water interface. A compressibility study shows the positive association with DPPC. Adsorption kinetics shows that the protein adsorption is a one-step process and the amount of protein adsorbed depends on the concentration of protein at the water subphase. Incorporation of protein into the DPPC layer is surface-pressure dependent. The compressibility study indicates that the DPPC-OVA interaction is hydrophobic in nature and structural reorganization is eminent to adjust the hydrophobic mismatch between DPPC acyl chains and OVA hydrophobic moieties. At higher pressure, OVA tends to squeeze out from the DPPC monolayer. A nanometer scale FE-SEM image confirms this observation. Globular aggregates of protein of dimension 60-80 nm were observed in DPPC-OVA supported film. Steady-state fluorescence spectroscopy suggests that the tryptophan residues of OVA are main emitting species. The blue shift of tryptophan fluorescence in supported film may be due to the tryptophan molecule of protein exposed to the hydrophobic air phase.     

磷脂酰胆碱LB单分子膜诱导下KDP晶体取向生长的研究

有机超薄膜诱导晶体生长是在化学、物理与生物多门学科相互交融的基础上发展起来的新兴学科 ,并逐渐成为仿生合成的重要分支 [1] .目前的研究重点主要集中于以有机化合物 LB膜作为模板剂诱导生物矿化材料上 [2～ 5] .磷脂 LB膜是生物膜的简化模型体系 [6 ] ,用它作模板剂将使该领域的研究进一步接近生物体系 .对晶体而言 ,修饰晶体材料的特征对于改善和测定材料的光学性能至关重要 [2 ] ,但目前有关上述领域的研究几乎均是空白 .KH2 PO4 ( KDP)晶体是性能优良的非线性光学材料 [7] ,本文首次以磷脂分子 LB膜作为模板剂诱导 KDP的晶化…     

Patterning of magnetic bimetallic coordination nanoparticles of Prussian blue derivatives by the Langmuir-Blodgett technique

We report a novel method to prepare patterns of nanoparticles over large areas of the substrate. This method is based on the adsorption of the negatively charged nanoparticles dispersed in an aqueous subphase onto a monolayer of the phospholipid dipalmitoyl-l-α-phosphatidylcholine (DPPC) at the air-water interface. It has been used to prepare patterns of nanoparticles of Prussian blue analogues (PBA) of different size (K(0.25)Ni[Fe(CN)(6)](0.75) (NiFe), K(0.25)Ni[Cr(CN)(6)](0.75) (NiCr), K(0.25)Ni[Co(CN)(6)](0.75) (NiCo), Cs(0.4)Co[Cr(CN)(6)](0.8) (CsCoCr), and Cs(0.4)Co[Fe(CN)(6)](0.9) (CsCoFe)). The behavior of DPPC monolayer at the air-water interface in the presence of the subphase of PBA nanoparticles has been studied by the compression isotherms and Brewster angle microscopy (BAM) images. Atomic force microscopy (AFM) of the transferred films on mica substrates shows that patterns of the nanoparticles are observed for a 10(-4) M concentration of the subphase, based on the nanoparticle precursors, at surface pressures between 1 and 6 mN/m and transfer velocities from 10 to 80 mm/min. Vertical, horizontal, or tilted fringes of the nanoparticles with respect to the transfer direction can be obtained depending on the transfer velocity and surface pressure.     

Annexin A1 interaction with a zwitterionic phospholipid monolayer: a fluorescence microscopy study

We present the results of a fluorescence microscopy study of the interaction of annexin A1 with dipalmitoylphosphatidylcholine (DPPC) monolayers as a function of the lipid monolayer phase and the pH of the aqueous subphase. We show that annexin A1-DPPC interaction depends strongly on the domain structure of the DPPC monolayer and only weakly on the subphase pH. Annexin A1 is found to be line active, with preferential adsorption at phase boundaries. Also, annexin A1 is found to form networks in the presence of a domain structure in the monolayer. Our results point toward an important contribution of the unique N-terminal domain to the organization of the protein at the interface.     

Miscibility behavior of dipalmitoylphosphatidylcholine with a single-chain partially fluorinated amphiphile in Langmuir monolayers

Surface pressure-area, surface potential-area, and dipole moment-area isotherms were obtained for monolayers made from a partially fluorinated surfactant, (perfluorooctyl)undecyldimorpholinophosphate (F8H11DMP), dipalmitoylphosphatidylcholine (DPPC), and their combinations. Monolayers, spread on a 0.15 M NaCl subphase, were investigated at the air/water interface by the Wilhelmy method, ionizing electrode method, and fluorescence microscopy. Surface potentials were analyzed using the three-layer model proposed by Demchak and Fort. The contribution of the dimorpholinophosphate polar head group of F8H11DMP to the vertical component of the dipole moment was estimated to be 4.99 D. The linear variation of the phase transition pressure as a function of F8H11DMP molar fraction (X(F8H11DMP)) demonstrated that DPPC and F8H11DMP are miscible in the monolayer. This result was confirmed by deviations from the additivity rule observed when plotting the molecular areas and the surface potentials as a function of X(F8H11DMP) over the whole range of surface pressures investigated. Assuming a regular surface mixture, the Joos equation, which was used for the analysis of the collapse pressure of mixed monolayers, allowed calculation of the interaction parameter (xi=-1.3) and the energy of interaction (Delta epsilon =537 Jmol(-1)) between DPPC and F8H11DMP. The miscibility of DPPC and F8H11DMP within the monolayer was also supported by fluorescence microscopy. Examination of the observed flower-like patterns showed that F8H11DMP favors dissolution of the ordered LC phase domains of DPPC, a feature that may be key to the use of phospholipid preparations as lung surfactants.     

Effects of lipid chain unsaturation and headgroup type on molecular interactions between paclitaxel and phospholipid within model biomembrane

Molecular interactions between paclitaxel, an anticancer drug, and phospholipids of various chain unsaturations and headgroup types were investigated in the present study by Langmuir film balance and differential scanning calorimetry. Both the lipid monolayer at the air-water interface and the lipid bilayer vesicles (liposomes) were employed as model cell membranes. It was found that, regardless of the difference in molecular structure of the lipid chains and headgroup, the drug can form nonideal, miscible systems with the lipids at the air-water interface over a wide range of paclitaxel mole fractions. The interaction between paclitaxel and phospholipid within the monolayer was dependent on the molecular area of the lipids at the interface and can be explained by intermolecular forces or geometric accommodation. Paclitaxel is more likely to form thermodynamically stable systems with 1,2-dipalmitoyl-sn-glycerol-3-phosphocholine (DPPC) and 1,2-dielaidoyl-sn-glycero-3-phosphocholine (DEPC) than with 1,2-dipalmitoyl-sn-glycero-3-phosphoethanolamine (DPPE) and 1,2-distearoyl-sn-glycero-3-phosphocholine (DSPC). Investigation of the drug penetration into the lipid monolayer showed that DPPC and DEPC have higher incorporation abilities for the drug than DPPE and DSPC. A similar trend was also evidenced by DSC investigation with liposomes. While little change of DSC profiles was observed for the DPPE/paclitaxel and DSPC/paclitaxel liposomes, paclitaxel caused noticeable changes in the thermographs of DPPC and DEPC liposomes. Paclitaxel was found to cause broadening of the main phase transition without significant change in the peak melting temperature of the DPPC bilayers, which demonstrates that paclitaxel was localized in the outer hydrophobic cooperative zone of the bilayer, i.e., in the region of the C1-C8 carbon atoms of the acyl chain or binding at the polar headgroup site of the lipids. However, it may penetrate into the deeper hydrophobic zone of the DEPC bilayers. These findings provide useful information for liposomal formulation of anticancer drugs as well as for understanding drug-cell membrane interactions.