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Connecting the dots across time: reconstruction of single-cell signalling trajectories using time-stamped data

机译:将点连接到时间:使用时间戳数据重建单个小区信令轨迹

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Single-cell responses are shaped by the geometry of signalling kinetic trajectories carved in a multidimensional space spanned by signalling protein abundances. It is, however, challenging to assay a large number (more than?3) of signalling species in live-cell imaging, which makes it difficult to probe single-cell signalling kinetic trajectories in large dimensions. Flow and mass cytometry techniques can measure a large number (4 to more than 40) of signalling species but are unable to track single cells. Thus, cytometry experiments provide detailed time-stamped snapshots of single-cell signalling kinetics. Is it possible to use the time-stamped cytometry data to reconstruct single-cell signalling trajectories? Borrowing concepts of conserved and slow variables from non-equilibrium statistical physics we develop an approach to reconstruct signalling trajectories using snapshot data by creating new variables that remain invariant or vary slowly during the signalling kinetics. We apply this approach to reconstruct trajectories using snapshot data obtained from in silico simulations, live-cell imaging measurements, and, synthetic flow cytometry datasets. The application of invariants and slow variables to reconstruct trajectories provides a radically different way to track objects using snapshot data. The approach is likely to have implications for solving matching problems in a wide range of disciplines.
机译:单电池响应由信号传导动力学轨迹的几何形状成形,所述信号传导动力学轨迹通过信号传导蛋白质丰富跨越的多维空间。然而,挑战在实时细胞成像中测定大量(超过Δ3)的信号传导物种,这使得难以在大尺寸中探测单细胞信号传导动力学轨迹。流动和质量细胞术技术可以测量信号传导物种的大量(4至40多个),但不能跟踪单个细胞。因此,细胞测定术实验提供单细胞信号传导动力学的详细时间戳快照。是否可以使用时间戳的细胞计数数据来重建单个小区信令轨迹?借用来自非均衡统计物理学的保守和缓慢变量的概念,我们通过创建在信令动力学期间使用快照数据来使用快照数据重建信号传导轨迹的方法。我们应用这种方法来使用从Silico模拟,实时细胞成像测量和合成流式细胞仪数据集中获得的快照数据进行重建轨迹。不变性和慢变量重建轨迹的应用提供了一种使用快照数据跟踪对象的根本不同的方式。该方法可能有助于解决广泛的学科中的匹配问题。

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