confluent cell
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2021 ◽  
Author(s):  
Guanming Zhang ◽  
Julia Mary Yeomans

We use a computational phase-field model together with analytical analysis to study how inter-cellular active forces can mediate individual cell morphology and collective motion in a confluent cell monolayer. Contractile inter-cellular interactions lead to cell elongation, nematic ordering and active turbulence, characterised by motile topological defects. Extensile interactions result in frustration, and perpendicular cell orientations become more prevalent. Furthermore, we show that contractile behaviour can change to extensile behaviour if anisotropic fluctuations in cell shape are considered.


2021 ◽  
Author(s):  
Elizabeth Lawson-Keister ◽  
Lisa Manning

Collective chemotaxis, where single cells cannot climb a biochemical signaling gradient but clusters of cells can, has been observed in different biological contexts, including confluent tissues where there are no gaps or overlaps between cells. Although particle-based models have been developed that predict important features of collective chemotaxis, the mechanisms in those models depend on particle overlaps, and so it remains unclear if they can explain behavior in confluent systems. Here, we develop an open-source code that couples a 2D Voronoi simulation for confluent cell mechanics to a dynamic chemical signal that can diffuse, advect, and/or degrade, and use the code to study potential mechanisms for collective chemotaxis in cellular monolayers. We first study the impact of advection on collective chemotaxis, and delineate a regime where advective terms are important. Next, we investigate two possible chemotactic mechanisms, contact inhibition of locomotion and heterotypic interfacial tension, and demonstrate that both can drive collective chemotaxis in certain parameter regimes. We further demonstrate that the scaling behavior of cluster motion is well-captured by simple analytic theories.


Pharmaceutics ◽  
2021 ◽  
Vol 13 (10) ◽  
pp. 1563
Author(s):  
Cristiana L. Pires ◽  
Catarina Praça ◽  
Patrícia A. T. Martins ◽  
Ana L. M. Batista de Carvalho ◽  
Lino Ferreira ◽  
...  

Caco-2 monolayers are a common in vitro model used to evaluate human intestinal absorption. The reference protocol requires 21 days post-seeding to establish a stable and confluent cell monolayer, which is used in a single permeability assay during the period of monolayer stability (up to day 30). In this work, we characterize variations in the tightness of the cell monolayer over the stable time interval and evaluate the conditions required for their re-use in permeability assays. The monolayer integrity was assessed through TEER measurements and permeability of the paracellular marker Lucifer Yellow (LY), complemented with nuclei and ZO-1 staining for morphological studies and the presence of tight junctions. Over 150 permeability assays were performed, which showed that manipulation of the cell monolayer in the permeability assay may contribute significantly to the flux of LY, leading to Papp values that are dependent on the sampling duration. The assay also leads to a small decrease in the cell monolayer TEER, which is fully recovered when cell monolayers are incubated with culture media for two full days. When this procedure is followed, the cell monolayers may be used for permeability assays on days 22, 25, and 28, triplicating the throughput of this important assay.


2021 ◽  
Vol 6 (57) ◽  
pp. 2818
Author(s):  
Jens Eriksson ◽  
Daniel Styrström ◽  
Mikael Sellin

2020 ◽  
Vol 17 (169) ◽  
pp. 20200312
Author(s):  
Guanming Zhang ◽  
Romain Mueller ◽  
Amin Doostmohammadi ◽  
Julia M. Yeomans

The collective behaviour of confluent cell sheets is strongly influenced both by polar forces, arising through cytoskeletal propulsion, and by active inter-cellular forces, which are mediated by interactions across cell-cell junctions. We use a phase-field model to explore the interplay between these two contributions and compare the dynamics of a cell sheet when the polarity of the cells aligns to (i) their main axis of elongation, (ii) their velocity and (iii) when the polarity direction executes a persistent random walk. In all three cases, we observe a sharp transition from a jammed state (where cell rearrangements are strongly suppressed) to a liquid state (where the cells can move freely relative to each other) when either the polar or the inter-cellular forces are increased. In addition, for case (ii) only, we observe an additional dynamical state, flocking (solid or liquid), where the majority of the cells move in the same direction. The flocking state is seen for strong polar forces, but is destroyed as the strength of the inter-cellular activity is increased.


2020 ◽  
Vol 11 (1) ◽  
Author(s):  
Silke Henkes ◽  
Kaja Kostanjevec ◽  
J. Martin Collinson ◽  
Rastko Sknepnek ◽  
Eric Bertin

Lab on a Chip ◽  
2020 ◽  
Vol 20 (20) ◽  
pp. 3792-3805 ◽  
Author(s):  
András Kincses ◽  
Ana R. Santa-Maria ◽  
Fruzsina R. Walter ◽  
László Dér ◽  
Nóra Horányi ◽  
...  

Chip device to monitor streaming potential of confluent cell layers reflecting cell surface charge important for the function of biological barriers.


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