Thieme D, Reuland L, Lindl T, Kruse FE, Fuchsluger TA (2017)
Publication Language: English
Publication Type: Journal article, Original article
Publication year: 2017
URI: https://onlinelibrary.wiley.com/doi/full/10.1002/term.2574
DOI: 10.1002/term.2574
The expansion of donor‐derived corneal endothelial cells (ECs) is a promising approach for regenerative therapies in corneal diseases. To achieve the best Good Manufacturing Practice standard the entire cultivation process should be devoid of nonhuman components. However, so far, there is no suitable xeno‐free protocol for clinical applications. We therefore introduce a processed variant of a platelet lysate for the use in corneal cell and tissue culture based on a Good Manufacturing Practice‐grade thrombocyte concentrate. This processed human platelet lysate (phPL), free of any animal components and of anticoagulants such as heparin with a physiological ionic composition, was used to cultivate corneal ECs in vitro and ex vivo in comparison to standard cultivation with fetal calf serum (FCS). Human donor corneas were cut in quarters while 2 quarters of each cornea were incubated with the respective medium supplement. Three fields of view per quarter were taken into account for the analysis. Evaluation of phPL as a medium supplement in cell culture of immortalized EC showed a superior viability compared with FCS control with reduced cell proliferation. Furthermore, the viability during the expansion of primary cells is significantly (3‐fold ±0.5) increased with phPL compared with FCS standard medium. Quartering donor corneas was traumatic for the endothelium and therefore resulted in increased EC loss. Interestingly, however, cultivation of the quartered pieces for 2 weeks in 0.1‐mg/ml pHPL in Biochrome I showed a 21 (±10) % EC loss compared with 67 (±12) % EC loss when cultivated in 2% FCS in Biochrome I. The cell culture protocol with pHPL as FCS replacement seems to be superior to the standard FCS protocols with respect to EC survival. It offers a xeno‐free and physiological environment for corneal endothelial cells. This alternative cultivation protocol could facilitate the use of EC for human corneal cell therapy.
APA:
Thieme, D., Reuland, L., Lindl, T., Kruse, F.E., & Fuchsluger, T.A. (2017). Optimized human platelet lysate as novel basis for a serum‐, xeno‐, and additive‐free corneal endothelial cell and tissue culture. Journal of Tissue Engineering and Regenerative Medicine. https://doi.org/10.1002/term.2574
MLA:
Thieme, Daniel, et al. "Optimized human platelet lysate as novel basis for a serum‐, xeno‐, and additive‐free corneal endothelial cell and tissue culture." Journal of Tissue Engineering and Regenerative Medicine (2017).
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