- 作者:Janike Dickhuth ; DDSa ; &lowast ; ; Steffen Koerdt ; MD ; DDSa ; b ; &lowast ; ; Steffen.koerdt@web.de" class="auth_mail" title="E-mail the corresponding author ; Ulrike Kriegebaum ; PhDa ; &lowast ; ; Christian Linz ; MD ; DDSa ; Urs D. Mü ; ller-Richter ; MD ; DDS ; PhDa ; Oliver Ristow ; MD ; DDSc ; Alexander C. Kü ; bler ; MD ; DDS ; PhDa ; Tobias Reuther ; MD ; DDS ; PhDa
- 刊名:Oral Surgery, Oral Medicine, Oral Pathology and Oral Radiology
- 出版年:2015
- 出版时间:October 2015
- 年:2015
- 卷:120
- 期:4
- 页码:429-435
- 全文大小:1332 K
Material and Methods
Human oral keratinocytes were obtained from oral mucosal specimens and cultivated. According to their affinity to 尾1-integrin, epidermal stem cell populations were isolated by using collagen type IV and laminin-coated dishes. Cell proliferation and cell viability were measured by using the CASY cell counter, WST-1 assays, and real-time cell analysis (xCELLigence).
Results
Measurements on cell proliferation (CASY cell counter) and cell viability (WST-1 assay) showed the characteristic proliferation stages of in vitro–cultivated cells. No statistically significant differences could be monitored (P > .05). Real-time cell analysis, as a more direct and precise technique, revealed a steeper growth curve of adherent cells and therefore generally higher proliferation kinetics compared with cells derived from the supernate.
Conclusion
Data from real-time cell analysis showed an increased proliferation of adherent cells compared with those derived from the supernate. These results demonstrate the increase of the proliferation capacity by cultivation of keratinocytes derived by adhesion to extracellular matrix proteins.