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Corning Life Sciences 12-mm polyester transwell cell culture insert corning costar snapwell
( A to C ) Low-magnification photographic images depicting scaffold mounting into the <t>transwell</t> insert. (A) Transwell insert with PGS scaffold below. The outer edge of the scaffold was glued to the transwell insert with soft PDMS. The area of the transwell insert removed to mount scaffolds was 19.6 mm 2 (internal diameter, 5 mm). (B) Transwell insert holder with a PGS ice cube tray scaffold mounted into a transwell insert. (C) Six-transwell scaffold cell culture system. ( D to F ) Laminin-coated ice cube tray scaffolds are readily filled with hPSC-derived CRX +/tdTomato -expressing PRs. (D) 3D rendering of a scaffold (176 μm by 185 μm by 22 μm) confirms successful capture of multiple PRs (labeled in red) in individual capture wells. Cell nuclei are labeled with 4′,6-diamidino-2-phenylindole (DAPI) (blue). (E) Cells were seeded onto scaffolds at varying densities to determine the minimum number required to achieve the maximum carrying capacity of CRX +/tdTomato -PRs per well. Median (bold dashes) and quartiles (fine dashes) are shown within individual violin plots. (F) Scaffolds seeded with CRX +/tdTomato -PRs (RFP + , red) contain both ARR3-expressing cone PRs (green) and NR2E3-expressing rod PRs (pink). A 3D lateral view of the scaffold demonstrates relatively even distribution of ARR3 + cones and NR2E3 + rods. 3D rendering is 644 μm by 644 μm by 20 μm. Photo Credit: In-Kyu Lee, Department of Electrical and Computer Engineering, University of Wisconsin–Madison.
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Corning Life Sciences transwell cell culture inserts corning costar 0.4um
( A to C ) Low-magnification photographic images depicting scaffold mounting into the <t>transwell</t> insert. (A) Transwell insert with PGS scaffold below. The outer edge of the scaffold was glued to the transwell insert with soft PDMS. The area of the transwell insert removed to mount scaffolds was 19.6 mm 2 (internal diameter, 5 mm). (B) Transwell insert holder with a PGS ice cube tray scaffold mounted into a transwell insert. (C) Six-transwell scaffold cell culture system. ( D to F ) Laminin-coated ice cube tray scaffolds are readily filled with hPSC-derived CRX +/tdTomato -expressing PRs. (D) 3D rendering of a scaffold (176 μm by 185 μm by 22 μm) confirms successful capture of multiple PRs (labeled in red) in individual capture wells. Cell nuclei are labeled with 4′,6-diamidino-2-phenylindole (DAPI) (blue). (E) Cells were seeded onto scaffolds at varying densities to determine the minimum number required to achieve the maximum carrying capacity of CRX +/tdTomato -PRs per well. Median (bold dashes) and quartiles (fine dashes) are shown within individual violin plots. (F) Scaffolds seeded with CRX +/tdTomato -PRs (RFP + , red) contain both ARR3-expressing cone PRs (green) and NR2E3-expressing rod PRs (pink). A 3D lateral view of the scaffold demonstrates relatively even distribution of ARR3 + cones and NR2E3 + rods. 3D rendering is 644 μm by 644 μm by 20 μm. Photo Credit: In-Kyu Lee, Department of Electrical and Computer Engineering, University of Wisconsin–Madison.
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Corning Life Sciences transwell cell culture inserts with an 8-μm pore costar 3422
( A to C ) Low-magnification photographic images depicting scaffold mounting into the <t>transwell</t> insert. (A) Transwell insert with PGS scaffold below. The outer edge of the scaffold was glued to the transwell insert with soft PDMS. The area of the transwell insert removed to mount scaffolds was 19.6 mm 2 (internal diameter, 5 mm). (B) Transwell insert holder with a PGS ice cube tray scaffold mounted into a transwell insert. (C) Six-transwell scaffold cell culture system. ( D to F ) Laminin-coated ice cube tray scaffolds are readily filled with hPSC-derived CRX +/tdTomato -expressing PRs. (D) 3D rendering of a scaffold (176 μm by 185 μm by 22 μm) confirms successful capture of multiple PRs (labeled in red) in individual capture wells. Cell nuclei are labeled with 4′,6-diamidino-2-phenylindole (DAPI) (blue). (E) Cells were seeded onto scaffolds at varying densities to determine the minimum number required to achieve the maximum carrying capacity of CRX +/tdTomato -PRs per well. Median (bold dashes) and quartiles (fine dashes) are shown within individual violin plots. (F) Scaffolds seeded with CRX +/tdTomato -PRs (RFP + , red) contain both ARR3-expressing cone PRs (green) and NR2E3-expressing rod PRs (pink). A 3D lateral view of the scaffold demonstrates relatively even distribution of ARR3 + cones and NR2E3 + rods. 3D rendering is 644 μm by 644 μm by 20 μm. Photo Credit: In-Kyu Lee, Department of Electrical and Computer Engineering, University of Wisconsin–Madison.
Transwell Cell Culture Inserts With An 8 μm Pore Costar 3422, supplied by Corning Life Sciences, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Corning Life Sciences costar® transwell® 6.5 millimeter diameter tissue culture inserts
( A to C ) Low-magnification photographic images depicting scaffold mounting into the <t>transwell</t> insert. (A) Transwell insert with PGS scaffold below. The outer edge of the scaffold was glued to the transwell insert with soft PDMS. The area of the transwell insert removed to mount scaffolds was 19.6 mm 2 (internal diameter, 5 mm). (B) Transwell insert holder with a PGS ice cube tray scaffold mounted into a transwell insert. (C) Six-transwell scaffold cell culture system. ( D to F ) Laminin-coated ice cube tray scaffolds are readily filled with hPSC-derived CRX +/tdTomato -expressing PRs. (D) 3D rendering of a scaffold (176 μm by 185 μm by 22 μm) confirms successful capture of multiple PRs (labeled in red) in individual capture wells. Cell nuclei are labeled with 4′,6-diamidino-2-phenylindole (DAPI) (blue). (E) Cells were seeded onto scaffolds at varying densities to determine the minimum number required to achieve the maximum carrying capacity of CRX +/tdTomato -PRs per well. Median (bold dashes) and quartiles (fine dashes) are shown within individual violin plots. (F) Scaffolds seeded with CRX +/tdTomato -PRs (RFP + , red) contain both ARR3-expressing cone PRs (green) and NR2E3-expressing rod PRs (pink). A 3D lateral view of the scaffold demonstrates relatively even distribution of ARR3 + cones and NR2E3 + rods. 3D rendering is 644 μm by 644 μm by 20 μm. Photo Credit: In-Kyu Lee, Department of Electrical and Computer Engineering, University of Wisconsin–Madison.
Costar® Transwell® 6.5 Millimeter Diameter Tissue Culture Inserts, supplied by Corning Life Sciences, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Corning Life Sciences transwell tissue culture inserts costar, corning, ny; 6.5mm diameter, pore size
( A to C ) Low-magnification photographic images depicting scaffold mounting into the <t>transwell</t> insert. (A) Transwell insert with PGS scaffold below. The outer edge of the scaffold was glued to the transwell insert with soft PDMS. The area of the transwell insert removed to mount scaffolds was 19.6 mm 2 (internal diameter, 5 mm). (B) Transwell insert holder with a PGS ice cube tray scaffold mounted into a transwell insert. (C) Six-transwell scaffold cell culture system. ( D to F ) Laminin-coated ice cube tray scaffolds are readily filled with hPSC-derived CRX +/tdTomato -expressing PRs. (D) 3D rendering of a scaffold (176 μm by 185 μm by 22 μm) confirms successful capture of multiple PRs (labeled in red) in individual capture wells. Cell nuclei are labeled with 4′,6-diamidino-2-phenylindole (DAPI) (blue). (E) Cells were seeded onto scaffolds at varying densities to determine the minimum number required to achieve the maximum carrying capacity of CRX +/tdTomato -PRs per well. Median (bold dashes) and quartiles (fine dashes) are shown within individual violin plots. (F) Scaffolds seeded with CRX +/tdTomato -PRs (RFP + , red) contain both ARR3-expressing cone PRs (green) and NR2E3-expressing rod PRs (pink). A 3D lateral view of the scaffold demonstrates relatively even distribution of ARR3 + cones and NR2E3 + rods. 3D rendering is 644 μm by 644 μm by 20 μm. Photo Credit: In-Kyu Lee, Department of Electrical and Computer Engineering, University of Wisconsin–Madison.
Transwell Tissue Culture Inserts Costar, Corning, Ny; 6.5mm Diameter, Pore Size, supplied by Corning Life Sciences, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Image Search Results


( A to C ) Low-magnification photographic images depicting scaffold mounting into the transwell insert. (A) Transwell insert with PGS scaffold below. The outer edge of the scaffold was glued to the transwell insert with soft PDMS. The area of the transwell insert removed to mount scaffolds was 19.6 mm 2 (internal diameter, 5 mm). (B) Transwell insert holder with a PGS ice cube tray scaffold mounted into a transwell insert. (C) Six-transwell scaffold cell culture system. ( D to F ) Laminin-coated ice cube tray scaffolds are readily filled with hPSC-derived CRX +/tdTomato -expressing PRs. (D) 3D rendering of a scaffold (176 μm by 185 μm by 22 μm) confirms successful capture of multiple PRs (labeled in red) in individual capture wells. Cell nuclei are labeled with 4′,6-diamidino-2-phenylindole (DAPI) (blue). (E) Cells were seeded onto scaffolds at varying densities to determine the minimum number required to achieve the maximum carrying capacity of CRX +/tdTomato -PRs per well. Median (bold dashes) and quartiles (fine dashes) are shown within individual violin plots. (F) Scaffolds seeded with CRX +/tdTomato -PRs (RFP + , red) contain both ARR3-expressing cone PRs (green) and NR2E3-expressing rod PRs (pink). A 3D lateral view of the scaffold demonstrates relatively even distribution of ARR3 + cones and NR2E3 + rods. 3D rendering is 644 μm by 644 μm by 20 μm. Photo Credit: In-Kyu Lee, Department of Electrical and Computer Engineering, University of Wisconsin–Madison.

Journal: Science Advances

Article Title: Ultrathin micromolded 3D scaffolds for high-density photoreceptor layer reconstruction

doi: 10.1126/sciadv.abf0344

Figure Lengend Snippet: ( A to C ) Low-magnification photographic images depicting scaffold mounting into the transwell insert. (A) Transwell insert with PGS scaffold below. The outer edge of the scaffold was glued to the transwell insert with soft PDMS. The area of the transwell insert removed to mount scaffolds was 19.6 mm 2 (internal diameter, 5 mm). (B) Transwell insert holder with a PGS ice cube tray scaffold mounted into a transwell insert. (C) Six-transwell scaffold cell culture system. ( D to F ) Laminin-coated ice cube tray scaffolds are readily filled with hPSC-derived CRX +/tdTomato -expressing PRs. (D) 3D rendering of a scaffold (176 μm by 185 μm by 22 μm) confirms successful capture of multiple PRs (labeled in red) in individual capture wells. Cell nuclei are labeled with 4′,6-diamidino-2-phenylindole (DAPI) (blue). (E) Cells were seeded onto scaffolds at varying densities to determine the minimum number required to achieve the maximum carrying capacity of CRX +/tdTomato -PRs per well. Median (bold dashes) and quartiles (fine dashes) are shown within individual violin plots. (F) Scaffolds seeded with CRX +/tdTomato -PRs (RFP + , red) contain both ARR3-expressing cone PRs (green) and NR2E3-expressing rod PRs (pink). A 3D lateral view of the scaffold demonstrates relatively even distribution of ARR3 + cones and NR2E3 + rods. 3D rendering is 644 μm by 644 μm by 20 μm. Photo Credit: In-Kyu Lee, Department of Electrical and Computer Engineering, University of Wisconsin–Madison.

Article Snippet: To facilitate cell seeding, we incorporated scaffolds into a commercially available 12-mm polyester transwell cell culture insert (Corning Costar Snapwell, Sigma-Aldrich) before sterilization ( ).

Techniques: Cell Culture, Derivative Assay, Expressing, Labeling