Journal: Stem Cell Research & Therapy
Article Title: Good manufacturing practice production of human corneal limbus-derived stromal stem cells and in vitro quality screening for therapeutic inhibition of corneal scarring
doi: 10.1186/s13287-023-03626-8
Figure Lengend Snippet: Comparative assessment of cryopreservation media for cultured CSSCs. A Cell attachment efficiency—thawed cells after one month of frozen storage in different cryopreservation media was seeded on hFn-coated culture surface. After 24 h, the attachment rates of cells stored in CryoStor DMSO 5% and Cryopres DMSO 5% were similar to the research-grade DMSO [Res] (5%). Cell frozen in DMSO-free Stem-CellBanker, CryoStor DMSO 10%, and Cryopres DMSO 10% had poor cell attachment. B Cell index profiles of thawed CSSCs by xCELLigence. Cells in CryoStor DMSO 5% exhibited better growth kinetics. C Apoptosis assay by Annexin V-PI staining showed the percentages of live cells after frozen storage in 5% DMSO [Res] , CryoStor DMSO, 5% and Cryopres DMSO 5% were similar
Article Snippet: After allowing to attach for 24 h, the cells were differentiated to keratocytes by incubating with DMEM containing GlutaMAX I, 1 g/L D-glucose and sodium pyruvate (Thermo Fisher), ascorbate-2-phosphate (1 mM; Sigma), bFGF (10 ng/ml, Gibco), and transforming growth factor β3 (TGFβ3, 0.1 ng/ml; Gibco) [ ], and replenished with fresh medium every 2 to 3 days.
Techniques: Cell Culture, Cell Attachment Assay, Apoptosis Assay, Staining