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Characterization of a Murine Model of Bioequivalent Bladder Wound Healing and Repair Following Subtotal Cystectomy

机译:膀胱全切术后生物等效膀胱伤口愈合和修复的小鼠模型的表征

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摘要

Previous work demonstrated restoration of a bioequivalent bladder within 8 weeks of removing the majority of the bladder (subtotal cystectomy or STC) in rats. The goal of the present study was to extend our investigations of bladder repair to the murine model, to harness the power of mouse genetics to delineate the cellular and molecular mechanisms responsible for the observed robust bladder regrowth. Female C57 black mice underwent STC, and at 4, 8, and 12 weeks post-STC, bladder repair and function were assessed via cystometry, ex vivo pharmacologic organ bath studies, and T2-weighted magnetic resonance imaging (MRI). Histology was also performed to measure bladder wall thickness. We observed a time-dependent increase in bladder capacity (BC) following STC, such that 8 and 12 weeks post-STC, BC and micturition volumes were indistinguishable from those of age-matched non-STC controls and significantly higher than observed at 4 weeks. MRI studies confirmed that bladder volume was indistinguishable within 3 months (11 weeks) post-STC. Additionally, bladders emptied completely at all time points studied (i.e., no increases in residual volume), consistent with functional bladder repair. At 8 and 12 weeks post-STC, there were no significant differences in bladder wall thickness or in the different components (urothelium, lamina propria, or smooth muscle layers) of the bladder wall compared with age-matched control animals. The maximal contractile response to pharmacological activation and electrical field stimulation increased over time in isolated tissue strips from repaired bladders but remained lower at all time points compared with controls. We have established and validated a murine model for the study of de novo organ repair that will allow for further mechanistic studies of this phenomenon after, for example, genetic manipulation.
机译:先前的研究表明,在去除大鼠大部分膀胱(膀胱全切术或STC)后的八周内,该生物等效性膀胱得以恢复。本研究的目的是将我们对膀胱修复的研究扩展到小鼠模型,以利用小鼠遗传学的力量来描绘造成观察到的强劲膀胱再生的细胞和分子机制。雌性C57黑鼠接受STC,在STC后第4、8和12周,通过膀胱测压,离体药理器官浸浴研究和T2加权磁共振成像(MRI)评估膀胱修复和功能。还进行组织学测量膀胱壁厚度。我们观察到STC后膀胱容量(BC)随时间的增加,因此STC后8周和12周,BC和排尿量与年龄相匹配的非STC对照者没有区别,并且显着高于4周时观察到的。 MRI研究证实,在STC后3个月(11周)内,膀胱容量是无法区分的。另外,在研究的所有时间点,膀胱完全排空(即,残余体积没有增加),这与功能性膀胱修复一致。与年龄匹配的对照动物相比,STC后第8周和第12周,膀胱壁厚度或膀胱壁的不同成分(尿路上皮,固有层或平滑肌层)无明显差异。在从修复的膀胱中分离出的组织条中,对药理激活和电场刺激的最大收缩反应随时间增加,但在所有时间点均保持低于对照组。我们已经建立并验证了用于新生器官修复研究的小鼠模型,该模型将允许在例如基因操作后对该现象进行进一步的机理研究。

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