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Rapid methods for the characterization of unilamellar phospholipid vesicles. Application to studies on fatty acid donor and acceptor properties of membranes and fatty acid binding proteins
Authors:M Reers  R Elbracht  H Rüdel  F Spener
Institution:Institut für Biochemie, Universität Münster, Domagkstrasse 85, D-4400, Münster F.R.G.
Abstract:Vesicles having diameters from 20 to 200 nm were prepared from egg-yolk phosphatidylcholine (PC) and were separated as well as analyzed by methods that can be carried out with standard laboratory equipment. Gel-chromatography on Sephacryl S 1000 was adapted for expeditious size analysis of vesicles as well as for isolation of vesicle populations having a narrow range of diameters. The internal volume of vesicles was derived from enzymic tests for PC and for glucose encapsulated. Size analysis and enzymic determinations provided a convenient check for the lamellarity of membranes produced.Fatty acids and fatty acid binding proteins (FABPs) must interact in vivo in the presence of cellular membranes. As a model, interactions between unilamellar vesicles, anthroyloxypalmitic acid (A16:0) and FABPs were studied with the aid of gel-chromatographic methods elaborated and of fluorescence spectroscopy. FABP from bovine heart donated A16:0 to membranes, whereas FABP from bovine liver removed this fatty acid from vesicle membranes. The results revealed characteristic differences between cardiac and hepatic FABPs with regard to binding a fatty acid.
Keywords:phospholipid vesicles  gel-chromatography  internal volume  fluorescence spectroscopy  anthroyloxypalmitic acid  fatty acid binding protein  A16:0  anthroyloxypalmitic acid  BSA  bovine serum albumin  FABP  fatty acid binding protein  HG  heptyl glucoside  MLV  multilamellar vesicles  OG  octyl glucoside  PC  phosphatidylcholine  RFI  relative fluorescence intensity  SC  sodium cholate  SDC  sodium deoxycholate
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