4.8 Article

A Mass-Spectrometry-Based Approach to Distinguish Annular and Specific Lipid Binding to Membrane Proteins

Journal

ANGEWANDTE CHEMIE-INTERNATIONAL EDITION
Volume 59, Issue 9, Pages 3523-3528

Publisher

WILEY-V C H VERLAG GMBH
DOI: 10.1002/anie.201914411

Keywords

lipid binding; membrane protein structure; molecular dynamics; native mass spectrometry

Funding

  1. Ingvar Carlsson Award from Swedish Foundation for Strategic Research
  2. VR starting grant
  3. KI-StratNeuro starting grant
  4. VR grant [2013_08807]
  5. Wellcome Trust [104633/Z/14/Z]
  6. ERC Advanced Grant ENABLE [641317]
  7. MRC Programme Grant [MR/N020413/1]
  8. Wellcome [208361/Z/17/Z]
  9. MRC [MR/S009213/1]
  10. BBSRC [BB/P01948X/1, BB/R002517/1 BB/S003339/1]
  11. EPSRC [EP/P020232/1, EP/R029407/1]
  12. KI faculty
  13. BBSRC [BB/S003339/1, BB/P01948X/1, BB/R002517/1] Funding Source: UKRI
  14. EPSRC [EP/R029407/1] Funding Source: UKRI
  15. MRC [MR/N020413/1] Funding Source: UKRI
  16. European Research Council (ERC) [641317] Funding Source: European Research Council (ERC)

Ask authors/readers for more resources

Membrane proteins engage in a variety of contacts with their surrounding lipids, but distinguishing between specifically bound lipids, and non-specific, annular interactions is a challenging problem. Applying native mass spectrometry to three membrane protein complexes with different lipid-binding properties, we explore the ability of detergents to compete with lipids bound in different environments. We show that lipids in annular positions on the presenilin homologue protease are subject to constant exchange with detergent. By contrast, detergent-resistant lipids bound at the dimer interface in the leucine transporter show decreased k(off) rates in molecular dynamics simulations. Turning to the lipid flippase MurJ, we find that addition of the natural substrate lipid-II results in the formation of a 1:1 protein-lipid complex, where the lipid cannot be displaced by detergent from the highly protected active site. In summary, we distinguish annular from non-annular lipids based on their exchange rates in solution.

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