Specificity of Intramembrane Protein–Lipid Interactions

Our concept of biological membranes has markedly changed, from the fluid mosaic model to the current model that lipids and proteins have the ability to separate into microdomains, differing in their protein and lipid compositions. Since the breakthrough in crystallizing membrane proteins, the most powerful method to define lipid-binding sites on proteins has been X-ray and electron crystallography. More recently, chemical biology approaches have been developed to analyze protein–lipid interactions. Such methods have the advantage of providing highly specific cellular probes. With the advent of novel tools to study functions of individual lipid species in membranes together with structural analysis and simulations at the atomistic resolution, a growing number of specific protein–lipid complexes are defined and their functions explored. In the present article, we discuss the various modes of intramembrane protein–lipid interactions in cellular membranes, including examples for both annular and nonannular bound lipids. Furthermore, we will discuss possible functional roles of such specific protein–lipid interactions as well as roles of lipids as chaperones in protein folding and transport.Our concept of biological membranes has markedly changed in the last two decades, from the fluid mosaic model (Singer and Nicolson 1972), in which the membrane was thought to be formed by a homogenous lipid fluid phase with proteins embedded, to the current model that lipids and proteins are not homogenously distributed, but have the ability to separate into microdomains, differing in their protein and lipid compositions. A well established example of domains are lipid rafts (see Box 1 for definitions). Raft domains are described as dynamic domain structures enriched in cholesterol, sphingolipids, and membrane proteins (Brown and London 1998; Simons and Ikonen 1997) that have an important role in different cellular processes (Lingwood and Simons 2010). Formation of domains within cellular membranes has been extensively investigated over the past years leading to various models that differ in the primary forces involved in the formation and the recruitment of surrounding membrane components into such domains.

BOX 1.

Definitions

Annular Lipids/Lipid Shell

An annular lipid shell is formed when selected lipid classes or molecular species bind preferentially to the hydrophobic and/or hydrophilic surfaces of a membrane protein. Per definition these lipids show markedly reduced residence times at the protein–lipid interface as compared to bulk lipids.

Bulk Lipids

Lipids within the membrane that diffuse rapidly in the bilayer plane and show a low residence time at the protein–lipid interface following random collisions. Typical diffusion coefficients for bulk lipids in a liquid disordered phase are in the range of D_L = 7×10⁻¹² m²/sec (DOPC) (Filippov et al. 2003).

Hydrophobic Mismatch

A term to describe any deviation from the compatibility of the hydrophobic surface of membrane proteins (their TMDs) to the vertically and laterally encountered hydrophobic surfaces of the lipid bilayer in biological membranes. In the case of a hydrophobic mismatch, the resulting energy penalty may cause the recruitment of a suitable local lipid environment, the deformation of the membrane and/or in conformational changes of the protein to achieve a status of hydrophobic match (for advanced reading, see Killian 1998).

Lateral Pressure Field/Profile of Membranes

Biological membranes can be considered as the “solvent” for membrane proteins that are embedded in them. The lateral pressure profile (Ω(z)) describes the force or pressure that is exerted by the membrane on the matter residing inside it. This pressure is modulated by different extents of lipid–lipid interactions and asymmetries across and within the bilayer, which in turn results in varying lateral pressures that may locally correspond to several hundreds of atmospheres.

Lipid Rafts

Sterol and sphingolipid-dependent microdomains that form a network of lipid–lipid, protein–protein, and protein–lipid interactions; involved in the compartmentalization of processes such as signaling within biological membranes.

Liquid-Disordered Phase (I_d)

A predominantly fluid phase of lipids, characterized by a high degree of mobility (cis-gauche flexibility of acyl chains; lateral diffusion) and a high content of short and/or unsaturated fatty acyl chains.

Liquid-Ordered Phase (I_o)

A liquid crystalline phase (that displays physical properties of both liquids and of solid crystals), characterized by a high degree of acyl chain order (“packing”), a reduced lateral mobility of lipid and protein molecules, and a reduction in the elasticity of the membrane as a result of specific interactions between sterols and phospholipids containing long, saturated acyl chains and/or glycosphingolipids.

Microdomains

Membrane compartments of distinct lipid and protein composition that may modulate the enzymatic functions of membrane proteins.

Molecular Lipid Species

Individual members of a lipid class that differ in their fatty acid composition.

Nonannular Lipids

Lipids that specifically interact with membrane proteins are neither bulk lipids, nor do they belong to the shell/annulus of lipids that surround the membrane protein. These nonannular lipids often reside within membrane protein complexes, in which they may fulfill diverse functions ranging from structural building blocks to allosteric effectors of enzymatic activity (see text). Nonannular lipids bind to distinct hydrophobic sites of membrane proteins or membrane protein complexes.According to one model, membrane domains can form by specific protein–protein interactions (Douglass and Vale 2005). This model is based on single-molecule microscopy experiments. In these studies, single fluorophores were chemically attached to specific proteins, and the dynamics of individual proteins was tracked by monitoring the fluorescent probe. In this kind of set up, a dynamic behavior of lipids is not assessed. Here, proteins involved in signaling processes are trapped within interconnected microdomains created by specific protein–protein interactions, probably involving additional scaffolding proteins. The proteins of such domains can exchange with the surrounding membrane area at individual kinetics, some components are immobile over minutes, and others can diffuse rapidly.Another model emphasizes the importance of lipid–lipid interactions, initiating the formation of subdomains of defined lipid compositions. Transmembrane proteins then can be attracted to such subdomains via various specific interactions with lipids. The resulting lipid–protein complexes then eventually coalesce to form larger lipid–protein assemblies (Anderson and Jacobson 2002).The idea of lipid-dependent domain formation is inherent to the biophysical properties and therefore to the complex lipid composition of cellular membranes that include up to a thousand lipids that vary in structure (van Meer et al. 2008). This wide range of lipid species has been proposed to facilitate the “solvation” of membrane proteins. Taken into account the sum of lipid species present in a cellular membrane, it is important to understand the different interactions and affinities within the bilayer between different lipids. Molecular dynamics simulations have been successfully employed to investigate lipid interactions between different lipid species and found specific interactions of various lipid classes and molecular species (Hofsass et al. 2003; Niemela et al. 2004, 2006, 2009; Pandit et al. 2004; Zaraiskaya and Jeffrey 2005; Bhide et al. 2007). These results are supported and expanded by recent data from our group that suggest a specific order of interactions of sphingomyelin species with cholesterol in membranes (A.M. Ernst, F. Wieland, and B. Brügger, unpubl.). At low cholesterol concentrations, some sphingomyelin species preferentially interact with cholesterol, whereas others prefer their kin. At higher cholesterol concentrations, all sphingomyelin species investigated display an increased affinity for the sterol. These findings open the possibility of differentiated pathways of self-assembly of microdomains, dependent on molecular lipid species.In the present article the various modes of intramembrane protein–lipid interactions in cellular membranes (Fig. 1) will be discussed. This includes possible functional roles of such specific protein–lipid interactions.Open in a separate windowFigure 1.Intramembrane protein–lipid interactions within a cell membrane. (A) Bulk lipids; (B) annular lipids; (C) nonannular lipids/lipid ligands. For details see text.     

Propensity of lignin to associate: light scattering photometry study with native lignins

Many studies of lignins in solution invoke association and aggregation phenomena to explain their solution behavior (e.g., reprecipitation onto pulp fibers, condensation, etc.). Following their colloidal (apparent) molecular weights in solution as a function of time allows us to explore observable dissociation phenomena. These measurements were carried out using multiple angle laser light scattering (MALLS) photometry in the static mode. The challenges and opportunities of measuring the specific refractive index increment (dn/dC) of lignin solutions and determining the kinetics of the dissociation process were thus investigated. Hardwood and softwood representative lignins were isolated, and method for their full dissolution in THF was further developed, which then lead to accurate dn/dC values being obtained as a function of time. When coupled to additional work using light scattering static measurements and Zimm plots for the same solutions, this effort offers insight into the aggregation and ensuing dissociative events that operate within the lignin macromolecules.     

Fishing for lectins from diverse sequence libraries by yeast surface display - an exploratory study

The establishment of a robust technology platform for the expression cloning of carbohydrate-binding proteins remains a key challenge in glycomics. Here we explore the utility of using yeast surface display (YSD) technology in the interaction-based lectin cloning from complete cDNA libraries. This should pave the way for more detailed studies of protein-carbohydrate interactions. To evaluate the performance of this system, lectins representing three different subfamilies (galectins, siglecs, and C-type lectins) were successfully displayed on the surface of Saccharomyces cerevisiae and Pichia pastoris as a-agglutinin and/or alpha-agglutinin fusions. The predicted carbohydrate-binding activity could be detected for three out of five lectins tested (galectin-1, galectin-3, and siaoadhesin). For galectin-4 and E-selectin, no specific carbohydrate-binding activity could be detected. We also demonstrate that proteins with carbohydrate affinity can be specifically isolated from complex metazoan cDNA libraries through multiple rounds of FACS sorting, employing multivalent, fluorescent-labeled polyacrylamide-based glycoconjugates.     

Ca2+ signal summation and NFATc1 nuclear translocation in sympathetic ganglion neurons during repetitive action potentials

NFATc-mediated gene expression constitutes a critical step during neuronal development and synaptic plasticity. Although considerable information is available regarding the activation and functionality of specific NFATc isoforms, in neurons little is known about how sensitive NFAT nuclear translocation is to specific patterns of electrical activity. Here we used high-speed fluo-4 confocal imaging to monitor action potential (AP)-induced cytosolic Ca2+ transients in rat sympathetic neurons. We have recorded phasic and repetitive AP patterns, and corresponding Ca2+ transients initiated by either long (100-800 ms) current-clamp pulses, or single brief (2 ms) electrical field stimulation. We address the functional consequences of these AP and Ca2+ transient patterns, by using an adenoviral construct to express NFATc1-CFP and evaluate NFATc1-CFP nuclear translocation in response to specific patterns of electrical activity. Ten Hertz trains stimulation induced nuclear translocation of NFATc1, whereas 1 Hz trains did not. However, 1 Hz train stimulation did result in NFATc1 translocation in the presence of 2 mM Ba2+, which inhibits M-currents and promotes repetitive firing and the accompanying small (approximately 0.6 DeltaF/F0) repetitive and summating Ca2+ transients. Our results demonstrate that M-current inhibition-mediated spike frequency facilitation enhances cytosolic Ca2+ signals and NFATc1 nuclear translocation during trains of low frequency electrical stimulation.     

Isolation and characterization of a thermostable beta-xylosidase in the thermophilic bacterium Geobacillus pallidus

The isolation, purification, biochemical and biophysical characterization of the first reported beta-xylosidase from Geobacillus pallidus are described. The protein has an optimum pH close to 8 and an optimum temperature of 70 degrees C. These biochemical properties agree with those obtained by spectroscopic techniques, namely, circular dichroism (CD), infrared (FTIR) and fluorescence measurements. Thermal denaturation, followed by CD and FTIR, showed an apparent thermal denaturation midpoint close to 80 degrees C. The protein was probably a hydrated trimer in solution with, an elongated shape, as shown by gel filtration experiments. FTIR deconvolution spectra indicated that the protein contains a high percentage of alpha-helix (44%) and beta-sheet (40%). The sequencing of the N terminus and the biochemical features indicate that this new member of beta-xylosidases belongs to the GH52 family. Since there are no reported structural studies of any member of this family, our studies provide the first clue for the full conformational characterization of this protein family.     

Canine Recombinant Adenovirus Vector Induces an Immunogenicity-Related Gene Expression Profile in Skin-Migrated CD11b+ -Type DCs

Gene expression profiling of the blood cell response induced early after vaccination has previously been demonstrated to predict the immunogenicity of vaccines. In this study, we evaluated whether the analysis of the gene expression profile of skin-migrated dendritic cells (DCs) could be informative for the in vitro prediction of immunogenicity of vaccine, using canine adenovirus serotype 2 (CAV2) as vaccine vector. CAV2 has been shown to induce immunity to transgenes in several species including sheep and is an interesting alternative to human adenovirus-based vectors, based on the safety records of the parental strain in dogs and the lack of pre-existing immunity in non-host species. Skin-migrated DCs were collected from pseudo-afferent lymph in sheep. Both the CD11b⁺ -type and CD103⁺ -type skin-migrated DCs were transduced by CAV2. An analysis of the global gene response to CAV2 in the two skin DC subsets showed that the gene response in CD11b⁺ -type DCs was far higher and broader than in the CD103⁺ -type DCs. A newly released integrative analytic tool from Ingenuity systems revealed that the CAV2-modulated genes in the CD11b⁺ -type DCs clustered in several activated immunogenicity-related functions, such as immune response, immune cell trafficking and inflammation. Thus gene profiling in skin-migrated DC in vitro indicates that the CD11b⁺ DC type is more responsive to CAV2 than the CD103⁺ DC type, and provides valuable information to help in evaluating and possibly improving viral vector vaccine effectiveness.