human cadaveric primary islets  (Prodo Labs)

Journal: bioRxiv

Article Title: Stress-free Bioprinting of Human Primary and iPSC-derived Islets with Retained Functionality

doi: 10.1101/2024.10.14.617656

Figure Lengend Snippet: A) Schematic view of printing primary cadaveric human islets embedded in a 3% w/v alg/ 6% w/v MC bioink at 500 IEQ: 1 mL bioink. The printed primary islet construct is then cultured for 3-7 days to monitor for functionality and viability. Created using Biorender.com. B) Live Dead staining of printed primary islets 3 days post-printing. All scale bars convey 250 μm. Live cells are shown in green, dead cells are shown in red. C) Percentage of individual printed primary islet represented by viable cells, as indicated by green signal in Live/Dead staining (N=8). D) Location of dead cells present in individual printed primary islet as indicated by red signal in Live Dead staining. r/R of 0.0 indicates that the dead cell is present in the center of the islet, and an r/R of 1.0 indicates that the dead cell is present at the edge of the islet. E) Primary islets were printed and maintained in culture for 7 days. Islets are fluorescently stained for nuclei (DAPI), islet marker c-peptide (shown in green), and islet marker glucagon (shown in red). Scale bar representing 50 μm (*: p < 0.05). F) Glucose stimulated insulin secretion of printed primary islets after 7 days in culture G) Stimulation index from GSIS of second high glucose period normalized to second low glucose period (n=3).

Article Snippet: [ – ] Human cadaveric primary islets (Prodo Labs) were printed in the alginate/methylcellulose ink and maintained in culture for 3 to 7 days ( ).

Techniques: Construct, Cell Culture, Staining, Marker