Actin filament assembly and disassembly are vital for cell functions. MICAL Redox enzymes are important post-translational effectors of actin that stereo-specifically oxidize actin's M44 and M47 residues to induce cellular F-actin disassembly. Here we show that Mical-oxidized (Mox) actin can undergo extremely fast (84 subunits/s) disassembly, which depends on F-actin's nucleotide-bound state. Using near-atomic resolution cryoEM reconstruction and single filament TIRF microscopy we identify two dynamic and structural states of Mox-actin. Modeling actin's D-loop region based on our 3.9âà cryoEM reconstruction suggests that oxidation by Mical reorients the side chain of M44 and induces a new intermolecular interaction of actin residue M47 (M47-O-T351). Site-directed mutagenesis reveals that this interaction promotes Mox-actin instability. Moreover, we find that Mical oxidation of actin allows for cofilin-mediated severing even in the presence of inorganic phosphate. Thus, in conjunction with cofilin, Mical oxidation of actin promotes F-actin disassembly independent of the nucleotide-bound state.
Catastrophic disassembly of actin filaments via Mical-mediated oxidation.
Mical介导的氧化作用导致肌动蛋白丝发生灾难性解体
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作者:Grintsevich Elena E, Ge Peng, Sawaya Michael R, Yesilyurt Hunkar Gizem, Terman Jonathan R, Zhou Z Hong, Reisler Emil
| 期刊: | Nature Communications | 影响因子: | 15.700 |
| 时间: | 2017 | 起止号: | 2017 Dec 19; 8(1):2183 |
| doi: | 10.1038/s41467-017-02357-8 | 研究方向: | 免疫/内分泌 |
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