Stalk Domain of the Dynamin-like MxA GTPase Protein Mediates Membrane Binding and Liposome Tubulation via the Unstructured L4 Loop
Autor: | Alexander von der Malsburg, Inbal Abutbul-Ionita, Otto Haller, Dganit Danino, Georg Kochs |
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Rok vydání: | 2011 |
Předmět: |
Dynamins
Myxovirus Resistance Proteins G protein Membrane lipids GTPase Biology Guanosine triphosphate Biochemistry Protein Structure Secondary Membrane Lipids Structure-Activity Relationship chemistry.chemical_compound GTP-binding protein regulators GTP-Binding Proteins Humans Structure–activity relationship Protein Structure Quaternary Molecular Biology Dynamin Liposome Hydrolysis Cryoelectron Microscopy Membranes Artificial Cell Biology Protein Structure Tertiary chemistry Mutation Protein Structure and Folding Biophysics Guanosine Triphosphate Protein Multimerization |
Zdroj: | Journal of Biological Chemistry. 286:37858-37865 |
ISSN: | 0021-9258 |
DOI: | 10.1074/jbc.m111.249037 |
Popis: | The human MxA protein is an interferon-induced large GTPase with antiviral activity against a wide range of viruses, including influenza viruses. Recent structural data demonstrated that MxA oligomerizes into multimeric filamentous or ring-like structures by virtue of its stalk domain. Here, we show that negatively charged lipid membranes support MxA self-assembly. Like dynamin, MxA assembled around spherical liposomes inducing liposome tubulation. Cryo-transmission electron microscopy revealed that MxA oligomers around liposomes have a “T-bar” shape similar to dynamin. Moreover, biochemical assays indicated that the unstructured L4 loop of the MxA stalk serves as the lipid-binding moiety, and mutational analysis of L4 revealed that a stretch of four lysine residues is critical for binding. The orientation of the MxA molecule within the membrane-associated oligomer is in agreement with the proposed topology of MxA oligomers based on crystallographic data. Although oligomerization of wild-type MxA around liposomes led to the creation of helically decorated tubes similar to those formed by dynamin, this lipid interaction did not stimulate GTPase activity, in sharp contrast to the assembly-stimulated nucleotide hydrolysis observed with dynamin. Moreover, MxA readily self-assembles into rings at physiological conditions, as opposed to dynamin which self-assembles only at low salt conditions or onto lipids. Thus, the present results indicate that the oligomeric structures formed by MxA critically differ from those of dynamin. |
Databáze: | OpenAIRE |
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