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Instantaneous cell migration velocity may be ill-defined

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 Publication date 2018
  fields Physics
and research's language is English




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Cell crawling is critical to biological development, homeostasis and disease. In many cases, cell trajectories are quasi-random-walk. In vitro assays on flat surfaces often described such quasi-random-walk cell trajectories as approximations to a solution of a Langevin process. However, experiments show quasi-diffusive behavior at small timescales, indicating that instantaneous velocity and velocity autocorrelations are not well-defined. We propose to characterize mean-squared cell displacement using a modified Furth equation with three temporal and spatial regimes: short- and long-time/range diffusion and intermediate time/range ballistic motion. This analysis collapses mean-squared displacements of previously published experimental data onto a single-parameter family of curves, allowing direct comparison between movement in different cell types, and between experiments and numerical simulations. Our method also show that robust cell-motility quantification requires an experiment with a maximum interval between images of a few percent of the cell-motion persistence time or less, and a duration of a few orders-of-magnitude longer than the cell-motion persistence time or more.



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Key to collective cell migration is the ability of cells to rearrange their position with respect to their neighbors. Recent theory and experiments demonstrated that cellular rearrangements are facilitated by cell shape, with cells having more elongated shapes and greater perimeters more easily sliding past their neighbors within the cell layer. Though it is thought that cell perimeter is controlled primarily by cortical tension and adhesion at each cells periphery, experimental testing of this hypothesis has produced conflicting results. Here we studied collective cell migration in an epithelial monolayer by measuring forces, cell perimeters, and motion, and found all three to decrease with either increased cell density or inhibition of cell contraction. In contrast to previous understanding, the data suggest that cell shape and rearrangements are controlled not by cortical tension or adhesion at the cell periphery but rather by the stress fibers that produce tractions at the cell-substrate interface. This finding is confirmed by an experiment showing that increasing tractions reverses the effect of density on cell shape and rearrangements. Our study therefore reduces the focus on the cell periphery by establishing cell-substrate traction as a major physical factor controlling cell shape and motion in collective cell migration.
86 - Yanping Liu 2020
Cell migration, which can be significantly affected by intracellular signaling pathways (ICSP) and extracellular matrix (ECM), plays a crucial role in many physiological and pathological processes. The efficiency of cell migration, which is typically modeled as a persistent random walk (PRW), depends on two critical motility parameters, i.e., migration speed and persistence. It is generally very challenging to efficiently and accurately extract these key dynamics parameters from noisy experimental data. Here, we employ the normalized Shannon entropy to quantify the deviation of cell migration dynamics from that of diffusive/ballistic motion as well as to derive the persistence of cell migration based on the Fourier power spectrum of migration velocities. Moreover, we introduce the time-varying Shannon entropy based on the wavelet power spectrum of cellular dynamics and demonstrate its superior utility to characterize the time-dependent persistence of cell migration, which is typically resulted from complex and time-varying intra or extra-cellular mechanisms. We employ our approach to analyze trajectory data of in vitro cell migration regulated by distinct intracellular and extracellular mechanisms, exhibiting a rich spectrum of dynamic characteristics. Our analysis indicates that the combination of Shannon entropy and wavelet transform offers a simple and efficient tool to estimate the persistence of cell migration, which may also reflect the real-time effects of ICSP-ECM to some extent.
Cell migration plays essential roles in development, wound healing, diseases, and in the maintenance of a complex body. Experiments in collective cell migration generally measure quantities such as cell displacement and velocity. The observed short-time diffusion regime for mean square displacement in single-cell migration experiments on flat surfaces calls into question the definition of cell velocity and the measurement protocol. Theoretical results in stochastic modeling for single-cell migration have shown that this fast diffusive regime is explained by a white noise acting on displacement on the direction perpendicular to the migrating cell polarization axis (not on velocity). The prediction is that only the component of velocity parallel to the polarization axis is a well-defined quantity, with a robust measurement protocol. Here, we ask whether we can find a definition of a migrating-cell polarization that is able to predict the cells subsequent displacement, based on measurements of its shape. Supported by experimental evidence that cell nucleus lags behind the cell center of mass in a migrating cell, we propose a robust parametrization for cell migration where the distance between cell nucleus and the cells center of mass defines cell shape polarization. We tested the proposed methods by applying to a simulation model for three-dimensional cells performed in the CompuCell3D environment, previously shown to reproduce biological cells kinematics migrating on a flat surface.
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