Membrane Interactions of the Mason-Pfizer Monkey Virus Matrix Protein and Its Budding Deficient Mutants
Language English Country Netherlands Media print-electronic
Document type Journal Article, Research Support, Non-U.S. Gov't
PubMed
27725181
DOI
10.1016/j.jmb.2016.10.010
PII: S0022-2836(16)30425-9
Knihovny.cz E-resources
- Keywords
- Mason-Pfizer monkey virus, budding, liposome binding, matrix protein, membrane interaction,
- MeSH
- Cell Membrane metabolism MeSH
- Phospholipids metabolism MeSH
- Liposomes metabolism MeSH
- Magnetic Resonance Spectroscopy MeSH
- Mason-Pfizer monkey virus physiology MeSH
- Fatty Acids metabolism MeSH
- Mutation, Missense MeSH
- Mutant Proteins chemistry metabolism MeSH
- Viral Matrix Proteins chemistry metabolism MeSH
- Virus Release * MeSH
- Protein Binding MeSH
- Publication type
- Journal Article MeSH
- Research Support, Non-U.S. Gov't MeSH
- Names of Substances
- Phospholipids MeSH
- Liposomes MeSH
- Fatty Acids MeSH
- Mutant Proteins MeSH
- Viral Matrix Proteins MeSH
Matrix proteins (MAs) play a key role in the transport of retroviral proteins inside infected cells and in the interaction with cellular membranes. In most retroviruses, retroviral MAs are N-terminally myristoylated. This modification serves as a membrane targeting signal and also as an anchor for membrane interaction. The aim of this work was to characterize the interactions anchoring retroviral MA at the plasma membrane of infected cell. To address this issue, we compared the structures and membrane affinity of the Mason-Pfizer monkey virus (M-PMV) wild-type MA with its two budding deficient double mutants, that is, T41I/T78I and Y28F/Y67F. The structures of the mutants were determined using solution NMR spectroscopy, and their interactions with water-soluble phospholipids were studied. Water-soluble phospholipids are widely used models for studying membrane interactions by solution NMR spectroscopy. However, this approach might lead to artificial results due to unnatural hydrophobic interactions. Therefore, we used a new approach based on the measurement of the loss of the 1H NMR signal intensity of the protein sample induced by the addition of the liposomes containing phospholipids with naturally long fatty acids. HIV-1 MA was used as a positive control because its ability to interact with liposomes has already been described. We found that in contrast to HIV-1, the M-PMV MA interacted with the liposomes differently and much weaker. In our invivo experiments, the M-PMV MA did not co-localize with lipid rafts. Therefore, we concluded that M-PMV might adopt a different membrane binding mechanism than HIV-1.
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