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The enzymatic de-epithelialization technique determines denuded amniotic membrane integrity and viability of harvested epithelial cells
P. Trosan, I. Smeringaiova, K. Brejchova, J. Bednar, O. Benada, O. Kofronova, K. Jirsova,
Language English Country United States
Document type Journal Article, Research Support, Non-U.S. Gov't
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- MeSH
- Amnion cytology metabolism pathology MeSH
- DNA analysis isolation & purification MeSH
- Edetic Acid chemistry MeSH
- Epithelial Cells cytology metabolism pathology MeSH
- Collagen Type IV metabolism MeSH
- Cells, Cultured MeSH
- Laminin metabolism MeSH
- Humans MeSH
- Microscopy, Electron, Scanning MeSH
- Nanog Homeobox Protein metabolism MeSH
- Cell Proliferation MeSH
- Re-Epithelialization MeSH
- SOXB1 Transcription Factors metabolism MeSH
- Trypsin metabolism MeSH
- Cell Survival MeSH
- Check Tag
- Humans MeSH
- Publication type
- Journal Article MeSH
- Research Support, Non-U.S. Gov't MeSH
The human amniotic membrane (HAM) is widely used for its wound healing effect in clinical practice, as a feeder for the cell cultivation, or a source of cells to be used in cell therapy. The aim of this study was to find effective and safe enzymatic HAM de-epithelialization method leading to harvesting of both denuded undamaged HAM and viable human amniotic epithelial cells (hAECs). The efficiency of de-epithelialization using TrypLE Express, trypsin/ ethylenediaminetetraacetic (EDTA), and thermolysin was monitored by hematoxylin and eosin staining and by the measurement of DNA concentration. The cell viability was determined by trypan blue staining. Scanning electron microscopy and immunodetection of collagen type IV and laminin α5 chain were used to check the basement membrane integrity. De-epithelialized hAECs were cultured and their stemness properties and proliferation potential was assessed after each passage. The HAM was successfully de-epithelialized using all three types of reagents, but morphological changes in basement membrane and stroma were observed after the thermolysin application. About 60% of cells remained viable using trypsin/EDTA, approximately 6% using TrypLE Express, and all cells were lethally damaged after thermolysin application. The hAECs isolated using trypsin/EDTA were successfully cultured up to the 5th passage with increasing proliferation potential and decreased stem cell markers expression (NANOG, SOX2) in prolonged cell culture. Trypsin/EDTA technique was the most efficient for obtaining both undamaged denuded HAM and viable hAECs for consequent culture.
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