Polar headgroup

In 1997, a Chinese research group [78] used the colloidal solution of 70-nm-sized carboxylated latex particles as a subphase and spread mixtures of cationic and other surfactants at the air-solution interface. If the pH was sufficiently low (1.5-3.0), the electrostatic interaction between the polar headgroups of the monolayer and the surface groups of the latex particles was strong enough to attract the latex to the surface. A fairly densely packed array of particles could be obtained if a 2 1 mixture of octadecylamine and stearic acid was spread at the interface. The particle films could be transferred onto solid substrates using the LB technique. The structure was studied using transmission electron microscopy. 

It has been proposed that the a-tocopheroxyl radical can be recycled back to tocopherol by ascorbate producing the ascorbyl radical (Packer etal., 1979 Scarpa et al., 1984). The location of a-tocopherol, with its phytyl tail in the membrane parallel to the fatty acyl chains of the phospholipids and its phenolic hydroxyl group at the memisrane-water interface near the polar headgroups of the phospholipid bilayer, enables ascorbate to donate hydrogen atoms to the tocopheroxyl radical. The suitability for ascorbate and tocopherol as chain-breaking antioxidants is exemplified (Buettner,... 

This work also shows that the time constants for the ionic surfactant micelle solutions are twice as fast as the TX solution time constant. Differences between the Stern layers of the micelles appear to be the charge of the surfactant polar headgroups and the presence of counterions. However, these differences do not account for the observed dynamics. Since the polar headgroups and counterions should interfact more strongly with the water molecules, the water motion at the interface should be slower. This view is supported by recent investigations where systematic variation of surfactant counter-... 

In the past few years, a range of solvation dynamics experiments have been demonstrated for reverse micellar systems. Reverse micelles form when a polar solvent is sequestered by surfactant molecules in a continuous nonpolar solvent. The interaction of the surfactant polar headgroups with the polar solvent can result in the formation of a well-defined solvent pool. Many different kinds of surfactants have been used to form reverse micelles. However, the structure and dynamics of reverse micelles created with Aerosol-OT (AOT) have been most frequently studied. AOT reverse micelles are monodisperse, spherical water droplets [32]. The micellar size is directly related to the water volume-to-surfactant surface area ratio defined as the molar ratio of water to AOT,... 

Zone I is the hydrophilic part of the bilayer. It includes the polar headgroup consisting of positively charged choline ammonium group and negatively charged phosphate... 

In the Hn phase and in the inverted micellar cubic phase, the water associated with the polar headgroups is trapped inside a ring structure and is not in rapid exchange with bulk water [18]. In a bicontinuous cubic phase, however, there is a continuous network of aqueous channels. 

An important extension of lipid-solute interaction components [20] to membrane partitioning is provided by solute molecular structure. Spacing between polar and nonpolar regions (Fig. 8) within a solute molecule may result in significant distortion of the KpDm product across the membrane polar headgroup/lipid core interface [21], Such interactions may be responsible for deviations from projected transport predictions based on simple partitioning theory translating to deviations from predicted absorption kinetics [1],... 

Considering only the lipid phase as the transport pathway for the peptide, as the solute enters and diffuses across the membrane it will encounter a number of different microenvironments. The first is the aqueous membrane interface (Fig. 23). In this region, the hydrated polar headgroups of the membrane phospholipids separate the aqueous phase from the apolar membrane interior. It has been shown that this region is capable of satisfying up to 70% of the hydrophobic effect... 

Shimooka, T., Shibata, A. and Terada, H. (1992). The local anesthetic tetracaine destabilizes membrane structure by interaction with polar headgroups of phospholipids, Biochim. Biophys. Acta, 1104, 261-268. 

Surfactant molecules (also called amphiphiles or detergents) combine a polar or ionic head and a non-polar tail within the same molecule. The non-polar part, which is typically made up of one or more alkyl chains, causes these compounds to be sparingly soluble in water, whereas the polar or ionic part interacts strongly with water. Upon increasing the concentration of the amphiphilic compound in water, the solubility limit will be reached at a certain point and phase separation will set in. Due to the efficient interactions between the polar headgroups and the surrounding water molecules, a complete phase separation is usually unfavourable. Instead, the process halts in an intermediate stage... 

Comfurius, P., Smeets, E.F., Willems, G.M., Bevers, E.M., and Zwaal,R.F.A., 1994, Assembly of the prothrombinase complex on the hpid vesicles dependent on the stereochemical configuration of polar headgroup of phosphatidylserine. Biochemistry 33 10319-10324. 

Glycerophosphollpid a complex lipid based on glycerol, containing two fatty acids, and a polar headgroup an important constituent of biological membranes. 

Modification typically takes advantage of electrostatic interactions between charges on the surface of the macromolecules and the polar headgroups of surfactants. We reasoned that the host-guest interactions at the nanoparticle-solution interface investigated in this work could be used for similar purposes. (From Liu et ah, 2001)... 

The interactions obviously differed between the lipid bilayers and the natural membranes. Furthermore, cholesterol slightly hinders the drug partitioning into the liquid-crystalline bilayers, in agreement with several previous reports, and the drug molecules interact electrostatically with membrane proteins at the hydrophilic interface adjacent to the polar headgroups of the phospholipid molecules (7). 

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