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首页> 外文期刊>In Vitro Cellular and Developmental Biology. Animal: Journal of the Tissues Culture Association >Expansion and long-term culture of differentiated normal rat urothelial cells in vitro.
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Expansion and long-term culture of differentiated normal rat urothelial cells in vitro.

机译:分化的正常大鼠尿道上皮细胞的体外扩增和长期培养。

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摘要

The objective of this study is to establish a reliable cell culture system for the long-term culture of rat urothelial cells (RUC), in which the cells multiply in vitro and form stratified polarized urothelium. Urothelial cells were harvested by the enzymatic digestion of the urothelium exposed by the eversion of resected rat bladders. Primary cultures were initiated in keratinocyte serum-free medium (KSFM) for selective proliferation of urothelial cells. Subsequently, the cells were propagated in a mixture of conditioned medium (CM) derived from Swiss 3T3 cell culture supernatant and KSFM (CM-KSFM). Mean population doubling time was 13.8 +/- 0.9 h. RUC were successfully maintained for 18 passages over a period of 4-5 mo. Detailed investigations of culture conditions showed that CM-KSFM yielded a differentiated multilayer structure. The stratified urothelial sheets measuring 4 x 6 cm2 could be formed and then detached using dispase. Cytokeratin pattern in both the cultured urothelial monolayer and engineered stratified layers was similar to those seen in vivo, as assessed with monoclonal antibody against cytokeratin 17. Ultrastructural morphology showed microvilli, basal cell layer, and desmosomes between adjacent cells in the stratified urothelium.
机译:这项研究的目的是建立一个可靠的细胞培养系统,用于大鼠尿路上皮细胞(RUC)的长期培养,其中细胞在体外增殖并形成分层的极化尿路上皮。通过酶切消化被切除的大鼠膀胱暴露的尿路上皮收集尿道上皮细胞。在角质形成细胞无血清培养基(KSFM)中启动原代培养,以选择性增殖尿路上皮细胞。随后,将细胞在衍生自Swiss 3T3细胞培养上清液和KSFM(CM-KSFM)的条件培养基(CM)的混合物中繁殖。平均群体倍增时间为13.8 +/- 0.9 h。 RUC在4-5 mo的时间内成功维持了18次传代。对培养条件的详细研究表明,CM-KSFM产生了分化的多层结构。可以形成尺寸为4 x 6 cm2的分层尿路上皮片,然后使用分散酶将其剥离。培养的尿路上皮单层和工程分层层中的细胞角蛋白模式与体内观察到的相似,这是针对细胞角蛋白17的单克隆抗体评估的。超微结构形态显示微绒毛,基底细胞层和分层尿路上皮中相邻细胞之间的桥粒。

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