Creation of Tissue-Engineered Urethras for Large Urethral Defect Repair in a Rabbit Experimental Model

被引:11
作者
Amesty, Maria Virginia [1 ]
Chamorro, Clara Ibel [2 ]
Lopez-Pereira, Pedro [1 ]
Martinez-Urrutia, Maria Jose [1 ]
Sanz, Beatriz [3 ]
Rivas, Susana [1 ]
Lobato, Roberto [1 ]
Fossum, Magdalena [2 ,4 ,5 ]
机构
[1] Hosp Univ La Paz, Dept Pediat Urol, Madrid, Spain
[2] Karolinska Inst, Dept Womens & Childrens Hlth, Bioclinicum J10 20, Stockholm, Sweden
[3] Hosp Univ La Paz, Dept Cell Culture, IdiPAZ Inst Invest, Madrid, Spain
[4] Copenhagen Univ Hosp, Dept Surg Gastroenterol, Div Pediat Surg, Rigshosp, Copenhagen, Denmark
[5] Univ Copenhagen, Dept Hlth Sci, Copenhagen, Denmark
关键词
tissue-engineering; regenerative medicine; tissue-engineered urethra; bladder washing; SIS matrix; hypospadias; hypospadias rabbit model; urethroplasty; INTESTINAL SUBMUCOSA GRAFT; HUMAN UROTHELIAL CELLS; LONG-TERM; FOLLOW-UP; RECONSTRUCTION; HYPOSPADIAS; URETHROPLASTY; REPLACEMENT; SCAFFOLDS; FIBERS;
D O I
10.3389/fped.2021.691131
中图分类号
R72 [儿科学];
学科分类号
100202 ;
摘要
Introduction: Tissue engineering is a potential source of urethral substitutes to treat severe urethral defects. Our aim was to create tissue-engineered urethras by harvesting autologous cells obtained by bladder washes and then using these cells to create a neourethra in a chronic large urethral defect in a rabbit model. Methods: A large urethral defect was first created in male New Zealand rabbits by resecting an elliptic defect (70 mm(2)) in the ventral penile urethra and then letting it settle down as a chronic defect for 5-6 weeks. Urothelial cells were harvested noninvasively by washing the bladder with saline and isolating urothelial cells. Neourethras were created by seeding urothelial cells on a commercially available decellularized intestinal submucosa matrix (Biodesign (R) Cook-Biotech (R)). Twenty-two rabbits were divided into three groups. Group-A (n = 2) is a control group (urethral defect unrepaired). Group-B (n = 10) and group-C (n = 10) underwent on-lay urethroplasty, with unseeded matrix (group-B) and urothelial cell-seeded matrix (group-C). Macroscopic appearance, radiology, and histology were assessed. Results: The chronic large urethral defect model was successfully created. Stratified urothelial cultures attached to the matrix were obtained. All group-A rabbits kept the urethral defect size unchanged (70 +/- 2.5 mm(2)). All group-B rabbits presented urethroplasty dehiscence, with a median defect of 61 mm(2) (range 34-70). In group-C, five presented complete correction and five almost total correction with fistula, with a median defect of 0.3 mm(2) (range 0-12.5), demonstrating a significant better result (p = 7.85 x 10(-5)). Urethrography showed more fistulas in group-B (10/10, versus 5/10 in group-C) (p = 0.04). No strictures were found in any of the groups. Group-B histology identified the absence of ventral urethra in unrepaired areas, with squamous cell metaplasia in the edges toward the defect. In group-C repaired areas, ventral multilayer urothelium was identified with cells staining for urothelial cell marker cytokeratin-7. Conclusions: The importance of this study is that we used a chronic large urethral defect animal model and clearly found that cell-seeded transplants were superior to nonseeded. In addition, bladder washing was a feasible method for harvesting viable autologous cells in a noninvasive way. There is a place for considering tissue-engineered transplants in the surgical armamentarium for treating complex urethral defects and hypospadias cases.
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页数:9
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