Structure and function at the lipid–protein interface of a pentameric ligand-gated ion channel

Structure and function at the lipid–protein interface of a pentameric ligand-gated ion channel

Although it has long been proposed that membrane proteins may contain tightly bound lipids, their identity, the structure of their binding sites, and their functional and structural relevance have remained elusive. To some extent, this is because tightly bound lipids are often located at the periphe...

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Published in:Proceedings of the National Academy of Sciences - PNAS Vol. 118; no. 23; pp. 1 - 9
Main Authors: Kumar, Pramod, Cymes, Gisela D., Grosman, Claudio
Format: Journal Article
Language:English
Published: Washington National Academy of Sciences 08-06-2021
Subjects:
Binding sites
Biological Sciences
Cardiolipin
Channel gating
E coli
Electron microscopy
Ion channels
Ion channels (ligand-gated)
Lecithin
Ligands
Lipid bilayers
Lipid composition
Lipids
Membrane proteins
Membranes
Phosphatidylcholine
Phospholipids
Proteins
Solubilization
Structure-function relationships
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Summary:Although it has long been proposed that membrane proteins may contain tightly bound lipids, their identity, the structure of their binding sites, and their functional and structural relevance have remained elusive. To some extent, this is because tightly bound lipids are often located at the periphery of proteins, where the quality of density maps is usually poorer, and because they may be outcompeted by detergent molecules used during standard purification procedures. As a step toward characterizing natively bound lipids in the superfamily of pentameric ligand-gated ion channels (pLGICs), we applied single-particle cryogenic electron microscopy to fragments of native membrane obtained in the complete absence of detergent-solubilization steps. Because of the heterogeneous lipid composition of membranes in the secretory pathway of eukaryotic cells, we chose to study a bacterial pLGIC (ELIC) expressed in Escherichia coli’s inner membrane. We obtained a three-dimensional reconstruction of unliganded ELIC (2.5-Å resolution) that shows clear evidence for two types of tightly bound lipid at the protein–bulk-membrane interface. One of them was consistentwith a “regular” diacylated phospholipid, in the cytoplasmic leaflet, whereas the other one was consistent with the tetra-acylated structure of cardiolipin, in the periplasmic leaflet. Upon reconstitution in E. coli polar-lipid bilayers, ELIC retained the functional properties characteristic of members of this superfamily, and thus, the fitted atomic model is expected to represent the (long-debated) unliganded-closed, “resting” conformation of this ion channel. Notably, the addition of cardiolipin to phosphatidylcholine membranes restored the ion-channel activity that is largely lost in phosphatidylcholine-only bilayers.
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Author contributions: P.K., G.D.C., and C.G. designed research; P.K. and G.D.C. performed research; P.K., G.D.C., and C.G. analyzed data; and P.K., G.D.C., and C.G. wrote the paper.
Edited by Richard W. Aldrich, The University of Texas at Austin, Austin, TX, and approved April 30, 2021 (received for review January 5, 2021)
ISSN:0027-8424
1091-6490
DOI:10.1073/pnas.2100164118