Or ManuscriptProg Lipid Res. Author manuscript; available in PMC 2017 April 01.Carquin

April 24, 2018

Or ManuscriptProg Lipid Res. Author manuscript; available in PMC 2017 April 01.Carquin et al.Page2. Lateral organization of lipids into submicrometric MG-132 chemical information domains2.1. Evidence in artificial systems and highly-specialized biological membranes Model membrane systems have aided in understanding the lipid organization of cell membranes. Planar supported bilayers [41], giant unilamellar vesicles (GUVs) made from lipid mixtures [17, 42-44] as well as giant PM vesicles (GPMVs) [15, 16, 18, 45, 46] and PM spheres (PMS), distinct PM preparations segregated from the cytoskeleton and cytoplasmic content [15, 47], have provided elegant views to visualize membrane domains (Fig. 1). Planar supported bilayers represent model systems for exploring lipid domains by fluorescence microscopy or AFM (Section 3.2.4). The main advantage of planar supported bilayers to GUVs was for a long time related to their capacity to form asymmetric bilayers. However, a method to produce asymmetric GUVs was recently developed and validated by London and coll. [48]. Such vesicles exhibit asymmetric lipid distribution and size ( 15-30m in diameter) comparable to those of cell membranes, allowing thereby detailed microscopic analyses. The ability to control the membrane composition of GUVs is advantageous because it enables understanding the functional roles of specific lipids in the formation of domains. However, GUVs are less useful to extrapolate observations to systems with higher lipid compositional complexity such as the PM. Striking differences in lipid or protein partitioning can even be found between GUVs and GPMVs [49]. For more information on model membranes, please read [50]. Lateral membrane heterogeneity, with domains reaching several micrometers in diameter, is present in all of these model systems (Fig. 1). The shape is a Pan-RAS-IN-1MedChemExpress Pan-RAS-IN-1 particular feature of these domains reflecting differential phase coexistence and, hence, distinct lipid composition. Ld, Lo and solid-ordered phases (So; often called gel phase) are the most common phases found in artificial and biological membranes (for a review, see [35, 43]). Irregular shapes are observed in gel phases and usually found in pure systems of lipids with high melting temperature (Tm) but generally poor in cholesterol [18, 44] (Fig. 1c,d). This contrasts with the smooth regular boundaries observed in liquid-phase coexistence [16, 17, 43, 47] (Fig. 1a,b,e). To appreciate the possible phase states that can simultaneously exist in a membrane at thermodynamic equilibrium, one must consider the phase diagrams [51]. Each lipid species has an intrinsic temperature for physical transition from a solid- to a liquid-phase, known as the Tm. Below the Tm, membrane lipids are in solid- or gel-state structures. When the temperature is raised above the Tm, the conformation of acyl chains changes, resulting into an increase of their disorder with more gauche conformation and, consequently, decreased packing. The Gibbs phase rule, which can only be applied if the lipid phases separate macroscopically, states that the number of de-mixed entities (P) for a system at equilibrium is correlated with the number of chemically independent components (C) by the following equation: P= C-F+2, where F is the number of independently variable intensive properties, such as temperature, pressure and mole fractions of phase components. Applying the Gibbs phase rule to a two-component system with a fixed composition and a fixed pressure, three phases can coexist a.Or ManuscriptProg Lipid Res. Author manuscript; available in PMC 2017 April 01.Carquin et al.Page2. Lateral organization of lipids into submicrometric domains2.1. Evidence in artificial systems and highly-specialized biological membranes Model membrane systems have aided in understanding the lipid organization of cell membranes. Planar supported bilayers [41], giant unilamellar vesicles (GUVs) made from lipid mixtures [17, 42-44] as well as giant PM vesicles (GPMVs) [15, 16, 18, 45, 46] and PM spheres (PMS), distinct PM preparations segregated from the cytoskeleton and cytoplasmic content [15, 47], have provided elegant views to visualize membrane domains (Fig. 1). Planar supported bilayers represent model systems for exploring lipid domains by fluorescence microscopy or AFM (Section 3.2.4). The main advantage of planar supported bilayers to GUVs was for a long time related to their capacity to form asymmetric bilayers. However, a method to produce asymmetric GUVs was recently developed and validated by London and coll. [48]. Such vesicles exhibit asymmetric lipid distribution and size ( 15-30m in diameter) comparable to those of cell membranes, allowing thereby detailed microscopic analyses. The ability to control the membrane composition of GUVs is advantageous because it enables understanding the functional roles of specific lipids in the formation of domains. However, GUVs are less useful to extrapolate observations to systems with higher lipid compositional complexity such as the PM. Striking differences in lipid or protein partitioning can even be found between GUVs and GPMVs [49]. For more information on model membranes, please read [50]. Lateral membrane heterogeneity, with domains reaching several micrometers in diameter, is present in all of these model systems (Fig. 1). The shape is a particular feature of these domains reflecting differential phase coexistence and, hence, distinct lipid composition. Ld, Lo and solid-ordered phases (So; often called gel phase) are the most common phases found in artificial and biological membranes (for a review, see [35, 43]). Irregular shapes are observed in gel phases and usually found in pure systems of lipids with high melting temperature (Tm) but generally poor in cholesterol [18, 44] (Fig. 1c,d). This contrasts with the smooth regular boundaries observed in liquid-phase coexistence [16, 17, 43, 47] (Fig. 1a,b,e). To appreciate the possible phase states that can simultaneously exist in a membrane at thermodynamic equilibrium, one must consider the phase diagrams [51]. Each lipid species has an intrinsic temperature for physical transition from a solid- to a liquid-phase, known as the Tm. Below the Tm, membrane lipids are in solid- or gel-state structures. When the temperature is raised above the Tm, the conformation of acyl chains changes, resulting into an increase of their disorder with more gauche conformation and, consequently, decreased packing. The Gibbs phase rule, which can only be applied if the lipid phases separate macroscopically, states that the number of de-mixed entities (P) for a system at equilibrium is correlated with the number of chemically independent components (C) by the following equation: P= C-F+2, where F is the number of independently variable intensive properties, such as temperature, pressure and mole fractions of phase components. Applying the Gibbs phase rule to a two-component system with a fixed composition and a fixed pressure, three phases can coexist a.