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Structural dataset from microsecond-long simulations of yeast mitofusin Fzo1 in the context of membrane docking

机译:膜对接背景下酵母线粒体融合蛋白Fzo1的微秒长模拟结构数据集

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摘要

In this work we present a novel set of possible auto-oligomerisation states of yeast protein Fzo1 in the context of membrane docking. The dataset reports atomistic models and trajectories derived from a molecular dynamics study of the yeast mitofusin Fzo1, residues 101–855. The initial modelling was followed by coarse-grained molecular dynamics simulation to evaluate the stability and the dynamics of each structural model in a solvated membrane environment. Simulations were run for 1 μs and collected with GROMACS v5.0.4 using the martini v2.1 force field. For each structural model, the dataset comprises the production phase under semi-isotropic condition at 1 bar, 310 K and 150 mn NaCl. The integration step is 20 fs and coordinates have been saved every 1 ns. Each trajectory is associated with a ready-available visualization state for the VMD software. These structural detailed informations are a ready-available platform to plan integrative studies on the mitofusin Fzo1 and will aid the community to further elucidate the mitochondrial tethering process during membrane fusion. This dataset is based on the publication “Physics-based oligomeric models of the yeast mitofusin Fzo1 at the molecular scale in the context of membrane docking.” (Brandner and De Vecchis et al., 2019)”.
机译:在这项工作中,我们在膜对接的背景下提出了一套新的酵母蛋白Fzo1可能的自动寡聚状态。该数据集报告了原子模型和轨迹,这些分子模型和轨迹来自酵母线粒体融合蛋白Fzo1(残基101-855)的分子动力学研究。在初始建模之后,进行粗粒度的分子动力学模拟,以评估溶剂化膜环境中每个结构模型的稳定性和动力学。模拟运行1μs,并使用martini v2.1力场通过GROMACS v5.0.4进行收集。对于每个结构模型,数据集包括在1 bar,310 K和1.5亿NaCl的半各向同性条件下的生产阶段。积分步骤为20 fs,每1 ns保存一次坐标。每个轨迹都与VMD软件的可用可视化状态相关联。这些详细的结构信息是计划对线粒体Fzo1进行整合研究的现成平台,将有助于社区进一步阐明膜融合过程中的线粒体束缚过程。该数据集基于出版物“膜对接情况下分子水平的酵母线粒体融合蛋白Fzo1的基于物理的寡聚模型”。 (Brandner and De Vecchis et al。,2019)”。

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