Vital cellular processes, from cell growth to synaptic transmission, rely on membrane-bounded carriers and vesicles to transport molecular cargo to and from specific intracellular compartments throughout the cell. Compartment-specific proteins are required for the final step, membrane fission, which releases the transport carrier from the intracellular compartment. The role of fission proteins, especially at intracellular locations and in non-neuronal cells, while informed by the dynamin-1 paradigm, remains to be resolved. In this study, we introduce a highly sensitive approach for the identification and analysis of membrane fission machinery, called burst analysis spectroscopy (BAS). BAS is a single particle, free-solution approach, well suited for quantitative measurements of membrane dynamics. Here, we use BAS to analyze membrane fission induced by the potent, fission-active ENTH domain of epsin. Using this method, we obtained temperature-dependent, time-resolved measurements of liposome size and concentration changes, even at sub-micromolar concentration of the epsin ENTH domain. We also uncovered, at 37°C, fission activity for the full-length epsin protein, supporting the argument that the membrane-fission activity observed with the ENTH domain represents a native function of the full-length epsin protein.
Single particle fluorescence burst analysis of epsin induced membrane fission.
利用单颗粒荧光爆发分析Epsin诱导的膜裂变
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作者:Brooks Arielle, Shoup Daniel, Kustigian Lauren, Puchalla Jason, Carr Chavela M, Rye Hays S
| 期刊: | PLoS One | 影响因子: | 2.600 |
| 时间: | 2015 | 起止号: | 2015 Mar 23; 10(3):e0119563 |
| doi: | 10.1371/journal.pone.0119563 | 研究方向: | 其它 |
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