Influence of a Fluorescent Probe on the Nanostructure of Phospholipid Membranes: Dipalmitoylphosphatidylcholine Interfacial Monolayers

Abstract

Monolayers of dipalmitoylphosphatidylcholine (DPPC), both in the absence and in the presence of 1% (mol/mol) of a fluorescent phospholipid probe, have been spread at the air−liquid interface of a surface balance, compressed up to pressures in the liquid-expanded/liquid-condensed plateau of the isotherm, transferred onto mica supports, and analyzed by scanning force microscopy (SFM). Supported DPPC films showed micrometer-sized condensed domains with morphology and size that were entirely analogous to those observed in situ at the air−liquid interface by epifluorescence microscopy. The analysis by SFM, however, allowed the study and comparison of monolayers in the absence and in the presence of the fluorescent marker. This analysis revealed that the presence of dye reduced by 10−20% the total amount of the liquid-condensed phase in the DPPC films. The presence of the dye also decreased the mechanical stability of the film and increased the time required for the monolayer to equilibrate. The resolution of SFM permitted the determination that the structures of both the liquid-expanded and the liquid-condensed regions of DPPC films were heterogeneous at the nanometer scale. Liquid-condensed DPPC microdomains contained nanoholes covering 4−8% of their area whereas 60−80% of the surface detected as liquid-expanded by fluorescence microscopy consisted of a condensed-like framework of nanodomains. The total area, the shape of the nanodomains, and their interconnectivity were affected by the presence of the probe, suggesting that care must be taken when studying the structure, especially at the nanometer scale, and properties of model lipid films in the presence of extrinsic probes.