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首页> 外文期刊>Angewandte Chemie >Dynamics of Synthetic Membraneless Organelles in Microfluidic Droplets
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Dynamics of Synthetic Membraneless Organelles in Microfluidic Droplets

机译:微流体液滴合成膜细胞器的动态

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摘要

Cells can form membraneless organelles by liquid-liquid phase separation. As these organelles are highly dynamic, it is crucial to understand the kinetics of these phase transitions. Here, we use droplet-based microfluidics to mix reagents by chaotic advection and observe nucleation, growth, and coarsening in volumes comparable to cells (pL) and on timescales of seconds. We apply this platform to analyze the dynamics of synthetic organelles formed by the DEAD-box ATPase Dhh1 and RNA, which are associated with the formation of processing bodies in yeast. We show that the timescale of phase separation decreases linearly as the volume of the compartment increases. Moreover, the synthetic organelles coarsen into one single droplet via gravity-induced coalescence, which can be arrested by introducing a hydrogel matrix that mimics the cytoskeleton. This approach is an attractive platform to investigate the dynamics of compartmentalization in artificial cells.
机译:细胞可以通过液 - 液相分离形成膜无细胞器。 由于这些细胞器具有高度动态,因此了解这些相变的动力学至关重要。 在此,我们使用基于液滴的微流体通过混沌平流混合试剂,并观察与细胞(PL)相当的体积和秒的核肉中的成核,生长和粗化。 我们应用该平台来分析死箱ATPaseDHH1和RNA形成的合成细胞器的动态,与酵母中的加工体的形成相关。 我们表明,随着隔室的体积增加,相分离的时间尺度线性降低。 此外,合成细胞器通过重力诱导的聚结成于重力诱导的聚结,可以通过引入模拟细胞骨架的水凝胶基质来阻止。 这种方法是一种有吸引力的平台,用于研究人造细胞中的舱室化的动态。

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