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Cationized albumin-biocoatings for the immobilization of lipid vesicles
Author(s) -
Sandra Ritz,
Klaus Eisele,
Jan Dorn,
Shaohua Ding,
Doris Vollmer,
Sabine Pütz,
Tanja Weil,
EvaKathrin Sinner
Publication year - 2010
Publication title -
biointerphases
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.633
H-Index - 45
eISSN - 1934-8630
pISSN - 1559-4106
DOI - 10.1116/1.3494039
Subject(s) - vesicle , chemistry , zeta potential , membrane , bovine serum albumin , lipid bilayer , colloidal gold , dynamic light scattering , fluorescence microscope , surface plasmon resonance , biophysics , fluorescence , chromatography , nanotechnology , nanoparticle , materials science , biochemistry , physics , quantum mechanics , biology
Tethered lipid membranes or immobilized lipid vesicles are frequently used as biomimetic systems. In this article, the authors presented a suitable method for efficient immobilization of lipid vesicles onto a broad range of surfaces, enabling analysis by quantitative methods even under rigid, mechanical conditions-bare surfaces such as hydrophilic glass surfaces as well as hydrophobic polymer slides or metal surfaces such as gold. The immobilization of vesicles was based on the electrostatic interaction of zwitterionic or negatively charged lipid vesicles with two types of cationic chemically modified bovine serum albumin (cBSA) blood plasma proteins (cBSA-113 and cBSA-147). Quantitative analysis of protein adsorption was performed as the cBSA coatings were characterized by atomic force microscopy, surface zeta potential measurement, fluorescence microscopy, and surface plasmon spectroscopy, revealing a maximal surface coverage 270-280 ng/cm(2) for 0.02 mg/ml cBSA on gold. Small unilamellar vesicles as well as giant unilamellar vesicles (GUVs) were readily immobilized (∼15 min) on cBSA coated surfaces. GUVs with 5-10 mol% negatively charged 1,2,-dipalmitoyl-sn-glycero-3-phosphoglycerol remained stable in liquid for at least 5 weeks.

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