Decellularization of the human urethra for tissue engineering applications

Marcela Kuniakova; Martin Klein; Paulina Galfiova; Maria Csobonyeiova; Claudia Feitscherova; Stefan Polak; Zuzana Varchulova Novakova; Katarina Topoliova; Branislav Trebaticky; Ivan Varga; Lubos Danisovic; Stanislav Ziaran

doi:10.1177/15353702231162092

Decellularization of the human urethra for tissue engineering applications

Exp Biol Med (Maywood). 2023 Jun;248(12):1034-1042. doi: 10.1177/15353702231162092. Epub 2023 Apr 18.

Authors

Marcela Kuniakova^{1

2}, Martin Klein^{2

3}, Paulina Galfiova³, Maria Csobonyeiova^{2

3}, Claudia Feitscherova^{2

3}, Stefan Polak³, Zuzana Varchulova Novakova^{1

2}, Katarina Topoliova⁴, Branislav Trebaticky^{2

4}, Ivan Varga^{2

3}, Lubos Danisovic^{1

2}, Stanislav Ziaran^{2

4}

Affiliations

¹ Institute of Medical Biology, Genetics and Clinical Genetics, Faculty of Medicine, Comenius University Bratislava 811 08, Slovakia.
² National Institute of Rheumatic Diseases, Piestany 921 12, Slovakia.
³ Institute of Histology and Embryology, Faculty of Medicine, Comenius University Bratislava, Bratislava 811 08, Slovakia.
⁴ Department of Urology, Faculty of Medicine, Comenius University Bratislava, Bratislava 833 05, Slovakia.

Abstract

Recently, several scaffolds have been introduced for urethral tissue engineering. However, acellular human urethral scaffold harvested from deceased donors may provide significant advantages compared to synthetic, composite, or other biological scaffolds. This study aims to develop the protocol for decellularization of the human urethra that preserves substantial extracellular matrix (ECM) components, which are essential for subsequent recellularization mimicking the natural environment of the native ECM. A total of 12 human urethras were harvested from deceased donors. An equal part of every harvested urethra was used as a control sample for analyses. The protocol design was based on the enzyme-detergent-enzyme method. Trypsin and Triton X-100 were used to remove cells, followed by DNase treatment to remove DNA residues. Subsequently, the specimens were continually rinsed in deionized water for seven days. The efficiency of decellularization was determined by histochemistry, immunohistochemical staining, scanning electron microscopy (SEM), and DNA quantification. Histological analysis confirmed cell removal and preservation of urethral structure after decellularization. The preservation of collagen IV and fibronectin was confirmed by histologic examination and immunohistochemical staining. SEM confirmed the maintenance of the ultrastructural architecture of ECM and fibers. DNA content in decellularized urethra was significantly lower compared to the native sample (P < 0.001), and so the criteria for decellularized tissue were met. Cytotoxicity analysis data showed that the matrix-conditioned medium did not contain soluble toxins and had no significant inhibitory effect on cell proliferation, providing evidence that the decellularized samples are not toxic. This study demonstrates the feasibility of the enzyme-detergent-enzyme-based decellularization protocol for removing cellular components and maintaining urethral ECM and its ultrastructure. Moreover, obtained results provide solid ground for recellularization and urethral tissue engineering, which will follow.

Keywords: Urethra; decellularization; scaffold; tissue engineering.

MeSH terms

DNA
Detergents / pharmacology
Extracellular Matrix / chemistry
Humans
Tissue Engineering* / methods
Tissue Scaffolds
Urethra*

Substances

Detergents
DNA