Ent imaging kit LIVE/DEADH Viability/ Cytotoxicity to determine cell viability (Invitrogen, USA). The staining was performed in accordance with the manufacturer’s instructions. The cells were stained just before the image acquisition when microplates have already been folded. All processes were performed at room temperature.text). (B) Culturing the cells onto substrates coated with and without MPC polymer. (TIF)S were seeded on cover-slips, starved and transfected with siRNA as Figure S2 Schematic illustration of the fabrication steps of self-folding using the microplates with a flexible joint. (i)?iv) The microplates with the flexible joint were produced with parylene and SU-8 by using standard photolithography. (v)?vi) MPC polymer was coated to prevent cells from adhering the areas without the microplates. (vii) Cells were cultured onto the microplates, and (viii) the plates were self-folded by CTF spontaneously (Figures 4D and 6 in main text). (TIF) Figure S3 Self-folding mechanism. The CTFs were in equilibrium between a set of two microplates before detaching the plates from the glass substrate. We then pushed the plates using a glass tip, triggering detachment of the plates from the substrate. The cells pulled the upper faces of the detached plates by the CTFs, dragging the plates towards one another until their edges contact. Although the edges were pushing each other, the CTFs acted only on the upper surfaces of the plates, generating a rotational movement along the contacted upper edge. Consequently, the plates lifted out from the glass substrate and self-folded (Movie S1). (TIF) Figure S4 Images of cylindrical tubes with (A) bovine carotid artery endothelial cells and (B) HUVECs as vessel-like structures. Scale bars, 50 mm. (TIF) Figure S5 Cross-section images of cells inside the microstructures after culturing the cells for 7 days. The images of the cells inside the (A) cube and (B) dodecahedron at top (t), middle (m), and bottom 1531364 (b) taken by a confocal scanning laser microscopy. Live and dead cells are shown in green and red colors, respectively. Scale bars, 50 mm. (TIF) Table S1 Concentrations of gelatin for folding microplates with and without a flexible joint. (TIF)Imaging equipmentThe morphology of the cultured cells on the microplates was observed using an inverted optical microscope with phase contrast (IX71, Olympus, Japan). The images (Figures 4B, D) were captured using a CCD camera (DP72, Olympus, Japan) with an image software (AioVision, Olympus, Japan). S not observed, even though ATP depletion occurred more rapidly as Time-lapse images of the self-folding process by CTF with phase contrast were captured with CCD cameras (QICAM, Roper, US) (Figures 5A?C) or (AxioCam HRc, Carl Zeiss, Germany) (Figures 6A, B). To observe the fluorescence images of actin filaments and nucleases, we used an inverted optical fluorescence microscope with CCD camera and imaging software (BZ-9000, Keyence, Japan). The zstack images of the cell origami (Figure 5E) were taken by a confocal laser scanning microscope (Fluoview FV1000, Olympus, Japan).Supporting InformationMovie S1 Time-lapse images of self-folding microstructures with cells across a pair of the microplates by CTF. (MOV) Movie S2 Time-lapse images of continuously folding anddeploying plates with a flexible joint driven by the cardiomyocytes cultured on the plates. (MOV)Movie S3 Time-lapse images of self-folding 3D cell-laden structure by CTF: cube. (MOV) Movie S4 Time-lapse images of self-folding 3D cell-laden structure by CTF: dodecahedron. (MOV) Movie S5 Time-lapse images of self-folding 3D cell-laden struct.Ent imaging kit LIVE/DEADH Viability/ Cytotoxicity to determine cell viability (Invitrogen, USA). The staining was performed in accordance with the manufacturer’s instructions. The cells were stained just before the image acquisition when microplates have already been folded. All processes were performed at room temperature.text). (B) Culturing the cells onto substrates coated with and without MPC polymer. (TIF)Figure S2 Schematic illustration of the fabrication steps of self-folding using the microplates with a flexible joint. (i)?iv) The microplates with the flexible joint were produced with parylene and SU-8 by using standard photolithography. (v)?vi) MPC polymer was coated to prevent cells from adhering the areas without the microplates. (vii) Cells were cultured onto the microplates, and (viii) the plates were self-folded by CTF spontaneously (Figures 4D and 6 in main text). (TIF) Figure S3 Self-folding mechanism. The CTFs were in equilibrium between a set of two microplates before detaching the plates from the glass substrate. We then pushed the plates using a glass tip, triggering detachment of the plates from the substrate. The cells pulled the upper faces of the detached plates by the CTFs, dragging the plates towards one another until their edges contact. Although the edges were pushing each other, the CTFs acted only on the upper surfaces of the plates, generating a rotational movement along the contacted upper edge. Consequently, the plates lifted out from the glass substrate and self-folded (Movie S1). (TIF) Figure S4 Images of cylindrical tubes with (A) bovine carotid artery endothelial cells and (B) HUVECs as vessel-like structures. Scale bars, 50 mm. (TIF) Figure S5 Cross-section images of cells inside the microstructures after culturing the cells for 7 days. The images of the cells inside the (A) cube and (B) dodecahedron at top (t), middle (m), and bottom 1531364 (b) taken by a confocal scanning laser microscopy. Live and dead cells are shown in green and red colors, respectively. Scale bars, 50 mm. (TIF) Table S1 Concentrations of gelatin for folding microplates with and without a flexible joint. (TIF)Imaging equipmentThe morphology of the cultured cells on the microplates was observed using an inverted optical microscope with phase contrast (IX71, Olympus, Japan). The images (Figures 4B, D) were captured using a CCD camera (DP72, Olympus, Japan) with an image software (AioVision, Olympus, Japan). Time-lapse images of the self-folding process by CTF with phase contrast were captured with CCD cameras (QICAM, Roper, US) (Figures 5A?C) or (AxioCam HRc, Carl Zeiss, Germany) (Figures 6A, B). To observe the fluorescence images of actin filaments and nucleases, we used an inverted optical fluorescence microscope with CCD camera and imaging software (BZ-9000, Keyence, Japan). The zstack images of the cell origami (Figure 5E) were taken by a confocal laser scanning microscope (Fluoview FV1000, Olympus, Japan).Supporting InformationMovie S1 Time-lapse images of self-folding microstructures with cells across a pair of the microplates by CTF. (MOV) Movie S2 Time-lapse images of continuously folding anddeploying plates with a flexible joint driven by the cardiomyocytes cultured on the plates. (MOV)Movie S3 Time-lapse images of self-folding 3D cell-laden structure by CTF: cube. (MOV) Movie S4 Time-lapse images of self-folding 3D cell-laden structure by CTF: dodecahedron. (MOV) Movie S5 Time-lapse images of self-folding 3D cell-laden struct.
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