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人尿道上皮在体内和体外的培养与特性分析

Culture and characterisation of human urothelium in vivo and in vitro.

作者信息

Petzoldt J L, Leigh I M, Duffy P G, Masters J R

机构信息

Institute of Urology and Nephrology, Research Laboratories, London, UK.

出版信息

Urol Res. 1994;22(2):67-74. doi: 10.1007/BF00310994.

Abstract

The aim of this study was to culture human urothelium and generate enough cells for subsequent reconstructive surgery. Using a modification of the Rheinwald-Green method for the routine culture of keratinocytes from patients with burns, we successfully cultured 91% of 57 biopsies from the renal pelvis, ureter, bladder and urethra of paediatric patients. The cells could be split one to three up to 9 times at 7-10 day intervals, giving a surface area of 1000 cm2 after a 2 month culture period. Primary cultures could not be initiated in defined medium MCDB153, although cells initiated using the Rheinwald-Green method could subsequently be propagated in this medium. Cytokeratin patterns in vitro were similar to those in vivo in the expression of keratins 7, 18 and 19 (characteristic of simple epithelia) and keratin 13 (characteristic of non-cornified stratified epithelia). Cultured urothelium also expressed keratin 14 (characteristic of cornified stratified epithelium) in about 25% of cells and keratin 16 (characteristic of fast-growing cells). These findings indicate that urothelial cells can be propagated in vitro for autologous grafting, and the next step is to identify substrates suitable for urothelial cell growth and differentiation and surgical manipulation.

摘要

本研究的目的是培养人尿路上皮细胞,并产生足够数量的细胞用于后续的重建手术。我们采用改良的Rheinwald-Green方法来常规培养烧伤患者的角质形成细胞,成功培养了57份取自儿科患者肾盂、输尿管、膀胱和尿道的活检组织中的91%。这些细胞可以每隔7 - 10天以1:3的比例传代培养9次,在2个月的培养期后可获得1000 cm²的表面积。虽然在限定培养基MCDB153中无法起始原代培养,但使用Rheinwald-Green方法起始培养的细胞随后可以在该培养基中传代培养。体外细胞角蛋白表达模式与体内相似,表达角蛋白7、18和19(单层上皮的特征性角蛋白)以及角蛋白13(非角化复层上皮的特征性角蛋白)。培养的尿路上皮细胞中约25%的细胞还表达角蛋白14(角化复层上皮的特征性角蛋白)和角蛋白16(快速生长细胞的特征性角蛋白)。这些发现表明尿路上皮细胞可以在体外扩增用于自体移植,下一步是确定适合尿路上皮细胞生长、分化及手术操作的基质。

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