1.
Mechanical worrying drives cell migration in crowded environments.
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Welf, ES
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Driscoll, MK
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Sapoznik, E
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Murali, VS
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Weems, A
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Garcia-Arcos, JM
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Roh-Johnson, MR
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Dean, KM
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Piel, M
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Fiolka, R
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Danuser, G
Abstract:
Migratory cells navigate through crowded 3D microenvironments in vivo. Amoeboid cells, such as immune cells and some cancer cells, are thought to do so by deforming their bodies to squeeze through tight spaces.1 Yet large populations of nearly spherical amoeboid cells migrate2–4 in microenvironments too dense5,6 to move through without extensive shape deformations. How they do so is unknown. We used high-resolution light-sheet microscopy to visualize metastatic melanoma cells in dense environments, finding that cells maintain a round morphology as they migrate and create a path through which to move via bleb-driven mechanical degradation and subsequent macropinocytosis of extracellular matrix components. Proteolytic degradation of the extracellular matrix via matrix metalloproteinases is not required. Membrane blebs are short-lived relative to the timescale of migration, and thus persistence in their polarization is critical for productive ablation of the extracellular matrix. Interactions between small but long-lived cortical adhesions and collagen at the cell front induce PI-3 Kinase signaling that drive bleb enlargement via branched actin polymerization. Large blebs in turn abrade collagen, creating a feedback between extracellular matrix structure, cell morphology, and cell polarization that results in both path generation and persistent cell movement.
2.
A versatile oblique plane microscope for large-scale and high-resolution imaging of subcellular dynamics.
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Sapoznik, E
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Chang, BJ
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Huh, J
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Ju, RJ
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Azarova, EV
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Pohlkamp, T
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Welf, ES
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Broadbent, D
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Carisey, AF
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Stehbens, SJ
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Lee, KM
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Marín, A
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Hanker, AB
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Schmidt, JC
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Arteaga, CL
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Yang, B
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Kobayashi, Y
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Tata, PR
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Kruithoff, R
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Doubrovinski, K
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Shepherd, DP
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Millett-Sikking, A
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York, AG
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Dean, KM
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Fiolka, RP
Abstract:
We present an oblique plane microscope (OPM) that uses a bespoke glass-tipped tertiary objective to improve the resolution, field of view, and usability over previous variants. Owing to its high numerical aperture optics, this microscope achieves lateral and axial resolutions that are comparable to the square illumination mode of lattice light-sheet microscopy, but in a user friendly and versatile format. Given this performance, we demonstrate high-resolution imaging of clathrin-mediated endocytosis, vimentin, the endoplasmic reticulum, membrane dynamics, and Natural Killer-mediated cytotoxicity. Furthermore, we image biological phenomena that would be otherwise challenging or impossible to perform in a traditional light-sheet microscope geometry, including cell migration through confined spaces within a microfluidic device, subcellular photoactivation of Rac1, diffusion of cytoplasmic rheological tracers at a volumetric rate of 14 Hz, and large field of view imaging of neurons, developing embryos, and centimeter-scale tissue sections.
