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1. Motility of Enzyme-Powered Vesicles

   https://doi.org/10.1021/acs.nanolett.9b01830  

   Ghosh, Subhadip; Mohajerani, Farzad; Son, Seoyoung; Velegol, Darrell; Butler, Peter J.; Sen, Ayusman (August 2019, Nano Letters)
2. Chemotactic Motility-Induced Phase Separation

   https://doi.org/10.1103/PhysRevLett.131.118301  

   Zhao, Hongbo; Košmrlj, Andrej; Datta, Sujit S. (September 2023, Physical Review Letters)
3. Cell motility dependence on adhesive wetting

   https://doi.org/10.1039/C8SM01832D  

   Cao, Yuansheng; Karmakar, Richa; Ghabache, Elisabeth; Gutierrez, Edgar; Zhao, Yanxiang; Groisman, Alex; Levine, Herbert; Camley, Brian A.; Rappel, Wouter-Jan (February 2019, Soft Matter)

   Adhesive cell–substrate interactions are crucial for cell motility and are responsible for the necessary traction that propels cells. These interactions can also change the shape of the cell, analogous to liquid droplet wetting on adhesive substrates. To address how these shape changes affect cell migration and cell speed we model motility using deformable, 2D cross-sections of cells in which adhesion and frictional forces between cell and substrate can be varied separately. Our simulations show that increasing the adhesion results in increased spreading of cells and larger cell speeds. We propose an analytical model which shows that the cell speed is inversely proportional to an effective height of the cell and that increasing this height results in increased internal shear stress. The numerical and analytical results are confirmed in experiments on motile eukaryotic cells. 

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4. Surface Hydrophilicity Promotes Bacterial Twitching Motility

   https://doi.org/10.1101/2024.03.23.586342  

   O’Hara, Megan T; Shimozono, Tori M; Dye, Keane J; Harris, David; Yang, Zhaomin (March 2024, bioRxiv)

   Abstract Twitching motility is a form of bacterial surface translocation powered by the type IV pilus (T4P). It is frequently analyzed by interstitial colony expansion between agar and the polystyrene surfaces of Petri dishes. In such assays, the twitching motility of Acinetobacter nosocomialis was observed with MacConkey but not Luria-Bertani (LB) agar media. One difference between these two media is the presence of bile salts as a selective agent in MacConkey but not in LB. Here, we demonstrate that the addition of bile salts to LB allowed A. nosocomialis to display twitching. Similarly, bile salts enhanced the twitching of Acinetobacter baumannii and Pseudomonas aeruginosa in LB. These observations suggest that there is a common mechanism whereby bile salts enhance bacterial twitching and promote interstitial colony expansion. Bile salts disrupt lipid membranes and apply envelope stress as detergents. Surprisingly, their stimulatory effect on twitching appears not to be related to a bacterial physiological response to stressors. Rather it is due to their ability to alter the physicochemical properties of a twitching surface. We observed that while other detergents promoted twitching like bile salts, stresses applied by antibiotics, including the outer membrane-targeting polymyxin B, did not enhanced twitching motility. More importantly, bacteria displayed increased twitching on hydrophilic surfaces such as those of glass and tissue culture-treated polystyrene plastics, and bile salts no longer stimulated twitching on these surfaces. Together, our results show that altering the hydrophilicity of a twitching surface significantly impacts T4P functionality. 

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5. The evolution of animal cell motility

   https://doi.org/10.1016/j.cub.2020.03.026  

   Fritz-Laylin, Lillian K. (May 2020, Current Biology)