"Preparation of asymmetric phospholipid vesicles for use as cell membra" by Milka Doktorova, Frederick A. Heberle et al.

Chemistry and Biochemistry Publications

Title

Preparation of asymmetric phospholipid vesicles for use as cell membrane models

Authors

Milka Doktorova, Weill Cornell Medicine
Frederick A. Heberle, Oak Ridge National Laboratory
Barbara Eicher, Karl-Franzens-Universitat Graz
Robert F. Standaert, Oak Ridge National Laboratory
John Katsaras, Oak Ridge National Laboratory
Erwin London, Stony Brook University
Georg Pabst, Karl-Franzens-Universitat Graz
Drew Marquardt, University of Windsor

Document Type

Article

Publication Date

9-1-2018

Publication Title

Nature Protocols

Volume

Issue

First Page

2086

Last Page

2101

Abstract

© 2018, The Author(s). Freely suspended liposomes are widely used as model membranes for studying lipid–lipid and protein–lipid interactions. Liposomes prepared by conventional methods have chemically identical bilayer leaflets. By contrast, living cells actively maintain different lipid compositions in the two leaflets of the plasma membrane, resulting in asymmetric membrane properties that are critical for normal cell function. Here, we present a protocol for the preparation of unilamellar asymmetric phospholipid vesicles that better mimic biological membranes. Asymmetry is generated by methyl-β-cyclodextrin-catalyzed exchange of the outer leaflet lipids between vesicle pools of differing lipid composition. Lipid destined for the outer leaflet of the asymmetric vesicles is provided by heavy-donor multilamellar vesicles containing a dense sucrose core. Donor lipid is exchanged into extruded unilamellar acceptor vesicles that lack the sucrose core, facilitating the post-exchange separation of the donor and acceptor pools by centrifugation because of differences in vesicle size and density. We present two complementary assays allowing quantification of each leaflet’s lipid composition: the overall lipid composition is determined by gas chromatography–mass spectrometry, whereas the lipid distribution between the two leaflets is determined by NMR, using the lanthanide shift reagent Pr 3+ . The preparation protocol and the chromatographic assay can be applied to any type of phospholipid bilayer, whereas the NMR assay is specific to lipids with choline-containing headgroups, such as phosphatidylcholine and sphingomyelin. In ~12 h, the protocol can produce a large yield of asymmetric vesicles (up to 20 mg) suitable for a wide range of biophysical studies.

DOI

10.1038/s41596-018-0033-6

Recommended Citation

Doktorova, Milka; Heberle, Frederick A.; Eicher, Barbara; Standaert, Robert F.; Katsaras, John; London, Erwin; Pabst, Georg; and Marquardt, Drew. (2018). Preparation of asymmetric phospholipid vesicles for use as cell membrane models. Nature Protocols, 13 (9), 2086-2101.
https://scholar.uwindsor.ca/chemistrybiochemistrypub/160

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