Structural properties of model membranes in interaction with the leishmanicidal compound miltefosine

Leishmaniasis is a complex of diseases part of the neglected tropical diseases caused by several species of the genus Leishmania. It reaches a large part of the poorest people in the world and its visceral form, which is fatal if left untreated, has been spread around big cities, increasing the number of people at risk of infection. Among the used drugs for the treatment, there is the synthetic lipid analogue hexadecylphosphocholine (miltefosine), orally administrated, which acts in the cell membranes and can induce apoptosis like death, but its mechanism of action is not totally clear. The first interactions site of this drug is the cell membrane, and it is important to know its mechanism of interaction. In this work we explore properties of several membrane models with different compositions, taking into account the existent knowledge about the composition of the Leishmania plasma membrane. Therefore, the model membranes were giant and large unilamellar vesicles (GUVs and LUVs), formed from pure phospholipids, binary mixtures of phospholipids and cholesterol and ternary mixtures with ceramide, a sterol present in the Leishmania membranes. The interaction with miltefosine was studied in different intervals of drug concentration. The main techniques used were the steady-state and time-resolved fluorescence spectroscopy, fluorescence correlation spectroscopy, confocal and fluorescence microscopy and fluorescence lifetime imaging. The interaction depends on i) the molar ratio of drug and lipids; ii) the real concentration of the drug, if it is below or above the critical micelle concentration (CMC); iii) the composition of the model membrane and the lipid phase of the bilayer. In concentration below the CMC, miltefosine has an effect of bilayer fluidization, mainly when it is in a more ordered phase, but this effect is less pronounced in cholesterol presence, because this compound protects the bilayers from the drug effect. In vesicles from ternary mixtures of phospholipid, cholesterol and ceramide in high concentration, there is no phase separation, and the presence of 10 mol% of miltefosine promotes ceramide domains formation; in vesicles in which ceramide is in low concentration, forming domains, the phase separation is less evident with miltefosine addition. In high concentration ratio miltefosine/lipids, but below CMC, it is observed a decrease in vesicles size with drug/lipids aggregates formation from portion of the bilayer. In concentrations above the CMC, drastic effects occur, with solubilization of bigger portions of the membrane bilayer, and the effects occur in lower times for higher drug concentration. Therefore, generally, cholesterol protects bilayer from the effect of miltefosine, but the drug has a pronounced effect in model membranes of ternary mixtures containing ceramide. The effects vary with miltefosine concentration, increasing the bilayer fluidity in lower drug/lipid ratio, solubilization of small portions of the bilayer and decrease of vesicles size in higher ratios, but still below CMC, and above CMC, formation of aggregates of the drug with portions of bilayer lipids, and membrane fragmentation. (AU)