Constructing a Tissue-Engineered Ureter Using a Decellularized Matrix with Cultured Uroepithelial Cells and Bone Marrow-Derived Mononuclear Cells

去细胞化 移植 新生血管 组织工程 脚手架 细胞外基质 祖细胞 骨髓 基质(化学分析) 化学 输尿管 肉芽组织 血管生成 川地31 生物医学工程 病理 解剖 干细胞 细胞生物学 医学 生物 外科 癌症研究 伤口愈合 生物化学 色谱法
作者
Hiroshi Matsunuma,Hideaki Kagami,Yuji Narita,Kenichiro Hata,Yoshonari Ono,Shinichi Ohshima,Minoru Ueda
出处
期刊:Tissue Engineering [Mary Ann Liebert, Inc.]
卷期号:12 (3): 509-518 被引量:45
标识
DOI:10.1089/ten.2006.12.509
摘要

This study investigated the efficacy of the ureteral decellularized matrix (UDM) as a scaffold material for a tissue-engineered ureter, and the effect of bone marrow-derived mononuclear cells (BM-MNC) on the neovascularization of the scaffold. Canine ureters were treated with deoxycholic acid to remove all cells. Uroepithelial cells (UEC) were obtained from canine bladders, cultured, and then seeded onto the inner surface of the UDM before transplantation into the subcutaneous space of nude mice or the omentum of nude rats. The cultured UECs began showing vacuolar degeneration 3 days after transplantation and gradually disappeared thereafter. To facilitate neovascularization in the implant, BM-MNCs were seeded around the UDM before transplantation. This facilitated the survival of the UECs, which formed three to five cellular layers after 14 days. The mean microvessel density was significantly increased in tissues seeded with BM-MNCs. However, cell-tracking experiments revealed that the increased number of capillaries in the experimental group was not due to the direct differentiation of transplanted endothelial progenitor cells. Our results demonstrate that the UDM is a useful scaffold for a tissue-engineered ureter, especially when seeded with BM-MNCs to enhance angiogenesis.
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