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利用自体骨髓间充质干细胞的非人类灵长类动物膀胱再生模型。

A nonhuman primate model for urinary bladder regeneration using autologous sources of bone marrow-derived mesenchymal stem cells.

机构信息

Division of Pediatric Urology; Children's Memorial Hospital of Chicago, Chicago, Illinois, USA.

出版信息

Stem Cells. 2011 Feb;29(2):241-50. doi: 10.1002/stem.568.

DOI:10.1002/stem.568
PMID:21732482
Abstract

Animal models that have been used to examine the regenerative capacity of cell-seeded scaffolds in a urinary bladder augmentation model have ultimately translated poorly in the clinical setting. This may be due to a number of factors including cell types used for regeneration and anatomical/physiological differences between lower primate species and their human counterparts. We postulated that mesenchymal stem cells (MSCs) could provide a cell source for partial bladder regeneration in a newly described nonhuman primate bladder (baboon) augmentation model. Cell-sorted CD105(+) /CD73(+) /CD34(-) /CD45(-) baboon MSCs transduced with green fluorescent protein (GFP) were seeded onto small intestinal submucosa (SIS) scaffolds. Baboons underwent an approximate 40%-50% cystectomy followed by augmentation cystoplasty with the aforementioned scaffolds or controls and finally enveloped with omentum. Bladders from sham, unseeded SIS, and MSC/SIS scaffolds were subjected to trichrome, H&E, and immunofluorescent staining 10 weeks postaugmentation. Immunofluorescence staining for muscle markers combined with an anti-GFP antibody revealed that >90% of the cells were GFP(+) /muscle marker(+) and >70% were GFP(+) /Ki-67(+) demonstrating grafted cells were present and actively proliferating within the grafted region. Trichrome staining of MSC/SIS-augmented bladders exhibited typical bladder architecture and quantitative morphometry analyses revealed an approximate 32% and 52% muscle to collagen ratio in unseeded versus seeded animals, respectively. H&E staining revealed a lack of infiltration of inflammatory cells in grafted animals and in corresponding kidneys and ureters. Simple cystometry indicated recovery between 28% and 40% of native bladder capacity. Data demonstrate MSC/SIS composites support regeneration of bladder tissue and validate this new bladder augmentation model.

摘要

用于检查细胞接种支架在膀胱增大模型中的再生能力的动物模型在临床环境中最终效果不佳。这可能是由于多种因素造成的,包括用于再生的细胞类型以及灵长类动物和人类之间的解剖/生理差异。我们假设间充质干细胞(MSCs)可以为新描述的非人类灵长类动物(狒狒)膀胱增大模型中的部分膀胱再生提供细胞来源。分选的 CD105(+) / CD73(+) / CD34(-) / CD45(-) 狒狒 MSC 被转导为绿色荧光蛋白(GFP),然后接种到小肠黏膜下层(SIS)支架上。狒狒接受了大约 40%-50%的膀胱部分切除术,然后用上述支架或对照物进行膀胱增大成形术,最后用网膜包裹。在增强后 10 周,对 Sham、未接种 SIS 和 MSC/SIS 支架的膀胱进行三色、H&E 和免疫荧光染色。肌肉标志物的免疫荧光染色与抗 GFP 抗体结合,显示>90%的细胞为 GFP(+) /肌肉标志物(+),>70%的细胞为 GFP(+) / Ki-67(+),表明移植物细胞存在并在移植物区域内活跃增殖。MSC/SIS 增强的膀胱的三色染色显示出典型的膀胱结构,定量形态计量分析显示,未接种和接种动物的肌肉与胶原比分别约为 32%和 52%。H&E 染色显示移植物动物和相应肾脏和输尿管中缺乏炎症细胞浸润。简单膀胱测压表明,正常膀胱容量恢复了 28%-40%。数据表明 MSC/SIS 复合材料支持膀胱组织的再生,并验证了这种新的膀胱增大模型。

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