Transcriptional profile of in vitro expanded human epidermal progenitor cells for the treatment of non-healing wounds

Paulina Langa; Anna Wardowska; Jacek Zieliński; Justyna Podolak-Popinigis; Piotr Sass; Paweł Sosnowski; Karolina Kondej; Alicja Renkielska; Paweł Sachadyn; Piotr Trzonkowski; Michał Pikuła

doi:10.1016/j.jdermsci.2017.12.003

Transcriptional profile of in vitro expanded human epidermal progenitor cells for the treatment of non-healing wounds

J Dermatol Sci. 2018 Mar;89(3):272-281. doi: 10.1016/j.jdermsci.2017.12.003. Epub 2017 Dec 13.

Affiliations

¹ Department of Clinical Immunology and Transplantology, Medical University of Gdansk, Poland.
² Department of Surgical Oncology, Medical University of Gdansk, Poland.
³ Department of Molecular Biotechnology & Microbiology, Gdansk University of Technology, Gdansk, Poland.
⁴ Department of Plastic Surgery, Medical University of Gdansk, Poland.
⁵ Department of Clinical Immunology and Transplantology, Medical University of Gdansk, Poland. Electronic address: pikula@gumed.edu.pl.

PMID: 29287803
DOI: 10.1016/j.jdermsci.2017.12.003

Abstract

Background: Epidermal progenitor cells (EPCs) have been under extensive investigation due to their increasing potential of application in medicine and biotechnology. Cultured human EPCs are used in the treatment of chronic wounds and have recently became a target for gene therapy and toxicological studies. One of the challenges in EPCs culture is to provide a high number of undifferentiated, progenitor cells displaying high viability and significant biological activity.

Objectives: The goal of this study was to characterize the in vitro cultured progenitor cells and to assess whether the cells with the progenitor phenotype are able to enhance wound healing. Additionally, we aimed to establish the complete procedure of the culture, analysis and clinical application of epidermal progenitor cells.

Methods: In this study we present a method of cell isolation and culture followed by a technique of transplantation of the cultured cells onto the wound bed. The applied isolation technique involves two enzymatic steps (dispase, trypsin) and it is characterized by a high yield of cells. The obtained cells were cultured in vitro up to the second passage in serum-free and xeno-free keratinocytes-dedicated medium. Key stem cell markers were determined with means of flow cytometry and quantitative real-time PCR.

Results: The in vitro expanded cells displayed high proliferative activity without features of neither apoptosis nor necrosis. The flow cytometry and transcriptomic analyses showed enhanced expression of stem cell markers (i.e. proteins: ΔNp63, CD29, CD49f and BNC1, CDKN1A transcripts) in the expanded cells. In the presented compassionate use study, cultured autologous cells from an oncological patient were suspended in fibrin sealant and transplanted directly to a non-healing wound, resulting in wound closure within 2 months.

Conclusion: The cells cultured in serum-free media display epidermal stem cells features and a potential to stimulate wound healing. This promising procedure of isolation, culture and application warrants further clinical trials in the treatment of chronic wounds.

Keywords: Cell therapy; Flow cytometry; Keratinocytes; Stem cells; Wound healing; qPCR.

MeSH terms

Cells, Cultured
Epidermal Cells*
Fibrin Tissue Adhesive
Humans
Stem Cell Transplantation*
Stem Cells / metabolism*
Transcription, Genetic*
Wound Healing*

Substances

Fibrin Tissue Adhesive