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A novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution

Membrane proteins have a range of crucial biological functions and are the target of about 60% of all prescribed drugs. For most studies, they need to be extracted out of the lipid-bilayer, e.g. by detergent solubilisation, leading to the loss of native lipids, which may disturb important protein-li...

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Autores principales: Cecchetti, Cristina, Strauss, Jannik, Stohrer, Claudia, Naylor, Claire, Pryor, Edward, Hobbs, Jeanette, Tanley, Simon, Goldman, Adrian, Byrne, Bernadette
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2021
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8274869/
https://www.ncbi.nlm.nih.gov/pubmed/34252116
http://dx.doi.org/10.1371/journal.pone.0254118
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author Cecchetti, Cristina
Strauss, Jannik
Stohrer, Claudia
Naylor, Claire
Pryor, Edward
Hobbs, Jeanette
Tanley, Simon
Goldman, Adrian
Byrne, Bernadette
author_facet Cecchetti, Cristina
Strauss, Jannik
Stohrer, Claudia
Naylor, Claire
Pryor, Edward
Hobbs, Jeanette
Tanley, Simon
Goldman, Adrian
Byrne, Bernadette
author_sort Cecchetti, Cristina
collection PubMed
description Membrane proteins have a range of crucial biological functions and are the target of about 60% of all prescribed drugs. For most studies, they need to be extracted out of the lipid-bilayer, e.g. by detergent solubilisation, leading to the loss of native lipids, which may disturb important protein-lipid/bilayer interactions and thus functional and structural integrity. Relipidation of membrane proteins has proven extremely successful for studying challenging targets, but the identification of suitable lipids can be expensive and laborious. Therefore, we developed a screen to aid the high-throughput identification of beneficial lipids. The screen covers a large lipid space and was designed to be suitable for a range of stability assessment methods. Here, we demonstrate its use as a tool for identifying stabilising lipids for three membrane proteins: a bacterial pyrophosphatase (Tm-PPase), a fungal purine transporter (UapA) and a human GPCR (A(2A)R). A(2A)R is stabilised by cholesteryl hemisuccinate, a lipid well known to stabilise GPCRs, validating the approach. Additionally, our screen also identified a range of new lipids which stabilised our test proteins, providing a starting point for further investigation and demonstrating its value as a novel tool for membrane protein research. The pre-dispensed screen will be made commercially available to the scientific community in future and has a number of potential applications in the field.
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spelling pubmed-82748692021-07-27 A novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution Cecchetti, Cristina Strauss, Jannik Stohrer, Claudia Naylor, Claire Pryor, Edward Hobbs, Jeanette Tanley, Simon Goldman, Adrian Byrne, Bernadette PLoS One Research Article Membrane proteins have a range of crucial biological functions and are the target of about 60% of all prescribed drugs. For most studies, they need to be extracted out of the lipid-bilayer, e.g. by detergent solubilisation, leading to the loss of native lipids, which may disturb important protein-lipid/bilayer interactions and thus functional and structural integrity. Relipidation of membrane proteins has proven extremely successful for studying challenging targets, but the identification of suitable lipids can be expensive and laborious. Therefore, we developed a screen to aid the high-throughput identification of beneficial lipids. The screen covers a large lipid space and was designed to be suitable for a range of stability assessment methods. Here, we demonstrate its use as a tool for identifying stabilising lipids for three membrane proteins: a bacterial pyrophosphatase (Tm-PPase), a fungal purine transporter (UapA) and a human GPCR (A(2A)R). A(2A)R is stabilised by cholesteryl hemisuccinate, a lipid well known to stabilise GPCRs, validating the approach. Additionally, our screen also identified a range of new lipids which stabilised our test proteins, providing a starting point for further investigation and demonstrating its value as a novel tool for membrane protein research. The pre-dispensed screen will be made commercially available to the scientific community in future and has a number of potential applications in the field. Public Library of Science 2021-07-12 /pmc/articles/PMC8274869/ /pubmed/34252116 http://dx.doi.org/10.1371/journal.pone.0254118 Text en © 2021 Cecchetti et al https://creativecommons.org/licenses/by/4.0/This is an open access article distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Cecchetti, Cristina
Strauss, Jannik
Stohrer, Claudia
Naylor, Claire
Pryor, Edward
Hobbs, Jeanette
Tanley, Simon
Goldman, Adrian
Byrne, Bernadette
A novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution
title A novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution
title_full A novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution
title_fullStr A novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution
title_full_unstemmed A novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution
title_short A novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution
title_sort novel high-throughput screen for identifying lipids that stabilise membrane proteins in detergent based solution
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8274869/
https://www.ncbi.nlm.nih.gov/pubmed/34252116
http://dx.doi.org/10.1371/journal.pone.0254118
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