4.1 Article

Development of a Cell Sheet Transportation Technique for Regenerative Medicine

Journal

TISSUE ENGINEERING PART C-METHODS
Volume 20, Issue 5, Pages 373-382

Publisher

MARY ANN LIEBERT, INC
DOI: 10.1089/ten.tec.2013.0266

Keywords

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Funding

  1. Advanced Medical Care Development Zone (Super Zone) program from the Cabinet Office
  2. Ministry of Economy, Trade and Industry
  3. Ministry of Health, Labor and Welfare
  4. Ministry of Education in Japan
  5. Health and Labor Sciences Research Grant from the Ministry of Health, Labor, and Welfare [H16-Jitsuyouka-Shitei-001]

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Purpose: A transportation technique for cell sheets is necessary to standardize regenerative medicine. The aim of this article is to develop and evaluate a new transportation technique for cell sheets. Material and Methods: We developed a transportation container with three basic functions: the maintenance of interior temperature, air pressure, and sterility. The interior temperature and air pressure were monitored by a recorder. Human oral mucosal epithelial cells obtained from two healthy volunteers were cultured on temperature-responsive culture dishes. The epithelial cell sheets were transported via an airplane between the Osaka University and Tohoku University using the developed cell transportation container. Histological and immunohistochemical analyses and flow cytometric analyses for cell viability and cell purity were performed for the cell sheets before and 12h after transportation to assess the influence of transportation on the cell sheets. Sterility tests and screening for endotoxin and mycoplasma in the cell sheets were performed before and after transportation. Results: During transportation via an airplane, the temperature inside the container was maintained above 32 degrees C, and the changes in air pressure remained within 10hPa. The cell sheets were well stratified and successfully harvested before and after transportation. The expression patterns of keratin 3/76, p63, and MUC16 were equivalent before and after transportation. However, the expression of ZO-1 in the cell sheet after transportation was slightly weaker than that before transportation. The cell viability was 72.0% before transportation and 77.3% after transportation. The epithelial purity was 94.6% before transportation and 87.9% after transportation. Sterility tests and screening for endotoxin and mycoplasma were negative for all cell sheets. Conclusion: The newly developed transportation technique for air travel is essential technology for regenerative medicine and promotes the standardization and spread of regenerative therapies.

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