In vivo optochemical control of cell contractility at single-cell resolution

Kong, D.; Lv, Z.; Häring, Matthias; Lin, B.; Wolf, Fred; Grosshans, J.

doi:10.15252/embr.201947755

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In vivo optochemical control of cell contractility at single-cell resolution

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Häring, Matthias
Research Group Theoretical Neurophysics, Max Planck Institute for Dynamics and Self-Organization, Max Planck Society;

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Wolf, Fred
Research Group Theoretical Neurophysics, Max Planck Institute for Dynamics and Self-Organization, Max Planck Society;

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Kong, D., Lv, Z., Häring, M., Lin, B., Wolf, F., & Grosshans, J. (2019). In vivo optochemical control of cell contractility at single-cell resolution. EMBO Reports, 20(12): e47755. doi:10.15252/embr.201947755.

Zitierlink: https://hdl.handle.net/21.11116/0000-0005-206E-C

Zusammenfassung

The spatial and temporal dynamics of cell contractility plays a key role in tissue morphogenesis, wound healing, and cancer invasion. Here, we report a simple optochemical method to induce cell contractions in vivo during Drosophila morphogenesis at single-cell resolution. We employed the photolabile Ca2+ chelator o-nitrophenyl EGTA to induce bursts of intracellular free Ca2+ by laser photolysis in the epithelial tissue. Ca2+ bursts appear within seconds and are restricted to individual target cells. Cell contraction reliably followed within a minute, causing an approximately 50% drop in the cross-sectional area. Increased Ca2+ levels are reversible, and the target cells further participated in tissue morphogenesis. Depending on Rho kinase (ROCK) activity but not RhoGEF2, cell contractions are paralleled with non-muscle myosin II accumulation in the apico-medial cortex, indicating that Ca2+ bursts trigger non-muscle myosin II activation. Our approach can be, in principle, adapted to many experimental systems and species, as no specific genetic elements are required.