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Binding of a fluorescent lipid amphiphile to albumin and its transfer to lipid bilayer membranes
Authors:Abreu Magda S C  Estronca Luís M B B  Moreno Maria João  Vaz Winchil L C
Affiliation:Departamento de Química, Universidade de Coimbra, Portugal.
Abstract:
Kinetics and thermodynamics of the binding of a fluorescent lipid amphiphile, Rhodamine Green(TM)-tetradecylamide (RG-C(14:0)), to bovine serum albumin were characterized in an equilibrium titration and by stopped-flow fluorimetry. The binding equilibrium of RG-C(14:0) to albumin was then used to reduce its concentration in the aqueous phase to a value below its critical micelle concentration. Under these conditions, the only two species of RG-C(14:0) in the system were the monomer in aqueous solution in equilibrium with the protein-bound species. After previous determination of the kinetic and thermodynamic parameters for association of RG-C(14:0) with albumin, the kinetics of insertion of the amphiphile into and desorption off lipid bilayer membranes in different phases (solid, liquid-ordered, and liquid-disordered phases, presented as large unilamellar vesicles) were studied by stopped-flow fluorimetry at 30 degrees C. Insertion and desorption rate constants for association of the RG-C(14:0) monomer with the lipid bilayers were used to obtain lipid/water equilibrium partition coefficients for this fluorescent amphiphile. The direct measurement of these partition coefficients is shown to provide a new method for the indirect determination of the equilibrium partition coefficient of similar molecules between two defined lipid phases if they coexist in the same membrane.
Keywords:BSA, bovine serum albumin   CAC, critical aggregation concentration, used here synonymously with solubility product or critical micelle concentration   FLA, fluorescent lipid amphiphile(s)   Ka, equilibrium binding constant for FLA to protein   KP(L/W), equilibrium partition coefficient for partitioning of FLA between a membrane and aqueous phase   KP(L1/L2), equilibrium partition coefficient for partitioning of FLA between two lipid phases   LUV, large unilamellar vesicles with an average diameter of 0.1 μm   POPC, 1-palmitoyl-2-oleoylphosphatidyl choline   RG-C14:0, Rhodamine Green™-carboxylic acid tetradecylamide   SpM, Egg yolk sphingomyelin   TMRITC, Tetramethylrhodamine isothiocyanate (isomer R)   TMR-BSA, BSA labeled covalently with TMRITC at an average molar labeling ratio of 1
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