Plasma Membrane Plasticity of Xenopus laevis Oocyte Imaged with Atomic Force Microscopy

爪蟾 脂质双层 生物物理学 膜蛋白 细胞质 双层 化学 外周膜蛋白 细胞生物学 生物 生物化学 整体膜蛋白 基因
作者
Hermann Schillers,Timm Danker,Hans‐Joachim Schnittler,Florian Läng,Hans Oberleithner
出处
期刊:Cellular Physiology and Biochemistry [Cell Physiol Biochem Press GmbH and Co KG]
卷期号:10 (1-2): 99-107 被引量:31
标识
DOI:10.1159/000016339
摘要

Proteins are known to form functional clusters in plasma membranes. In order to identify individual proteins within clusters we developed a method to visualize by atomic force microscopy (AFM) the cytoplasmic surface of native plasma membrane, excised from Xenopus laevis oocyte and spread on poly-L-lysine coated glass. After removal of the vitelline membrane intact oocytes were brought in contact with coated glass and then rolled off. Inside-out oriented plasma membrane patches left at the glass surface were first identified with the lipid fluorescent marker FM1-43 and then scanned by AFM. Membrane patches exhibiting the typical phospholipid bilayer height of 5 nm showed multiple proteins, protruding from the inner surface of the membrane, with heights of 5 to 20 nm. Modelling plasma membrane proteins as spherical structures embedded in the lipid bilayer and protruding into the cytoplasm allowed an estimation of the respective molecular masses. Proteins ranged from 35 to 2,000 kDa with a peak value of 280 kDa. The most frequently found membrane protein structure (40/μm2) had a total height of 10 nm and an estimated molecular mass of 280 kDa. Membrane proteins were found firmly attached to the poly-L-lysine coated glass surface while the lipid bilayer was found highly mobile. We detected protein structures with distinguishable subunits of still unknown identity. Since X. laevis oocyte is a generally accepted expression system for foreign proteins, this method could turn out to be useful to structurally identify specific proteins in their native environment at the molecular level.
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