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大鼠膀胱正常上皮细胞、内皮细胞和成纤维细胞的体外分离与鉴定

The isolation and characterization in vitro of normal epithelial cells, endothelial cells and fibroblasts from rat urinary bladder.

作者信息

Pauli B U, Anderson S N, Memoli V A, Kuettner K E

出版信息

Tissue Cell. 1980;12(3):419-36. doi: 10.1016/0040-8166(80)90033-6.

Abstract

Epithelial cells, microvascular endothelial cells, and fibroblasts have been isolated in culture from normal urinary bladders of Fischer rats. Normal epithelial cells were cultured most efficiently when transitional epithelial sheets were plated on to collagen-coated roller flasks. The epithelial sheets were obtained by two micro-dissection techniques. In the first method, the epithelium was peeled as a large coherent sheet from the submucosal connective tissue following subepithelial injection of a collagenase solution, and after incubation of the bladders in the same enzyme solution. Epithelial sheets with intact basal cell layers were essential for culture success. On collagenous matrices, epithelial differentiation was similar to that in vivo. The in vitro transitional epithelium was composed of three cell layers, namely superficial, intermediate, and basal cells. Basal cells were attached to newly synthesized basal lamina by means of hemidesmosomes. Superficial cells were sealed at their apical lateral membranes by a junctional complex, i.e. a terminal bar. Asymmetric luminal membrane plaques were not apparent. In the second method, the epithelium was separated from the underlying connective tissue after collagenase--trypsin digestion of everted urinary bladders. Although the digest consisted mainly of epithelial cells, these rarely survived the first passage when plated on conventional plastic growth surfaces. After the third culture week, epithelial cells usually died and slowly growing colonies of fibroblasts or large flattened epitheloid cells became apparent. Epitheloid cells were identified by their typical ultrastructure as endothelial cells, showing Weibel--Palade bodies and pinocytotic caveolae. These cells were reactive with antiserum against factor VIII. The free surface of monolayer cultures was non-thrombogenic when incubated in the presence of platelets. Fibroblasts were isolated from heavily contaminated epithelial cell cultures after differential trypsinization. These three cells types represent the normal control cells of an in vitro tumor model for the study of invasiveness. All three cell types are involved in the formation and functional maintenance of the epithelial--stromal junction. The study of cell--cell and cell--matrix interactions may provide important clues for the understanding of tumor invasiveness, a process that starts at the epithelial--stromal junction and proceeds with its destruction.

摘要

上皮细胞、微血管内皮细胞和成纤维细胞已从Fischer大鼠的正常膀胱中分离出来进行培养。当将移行上皮片接种到胶原包被的滚瓶上时,正常上皮细胞的培养效率最高。上皮片通过两种显微解剖技术获得。在第一种方法中,在皮下注射胶原酶溶液并将膀胱在相同酶溶液中孵育后,将上皮作为一个大的连贯片从黏膜下结缔组织中剥离。具有完整基底细胞层的上皮片对于培养成功至关重要。在胶原基质上,上皮分化与体内相似。体外移行上皮由三层细胞组成,即表层细胞、中间层细胞和基底细胞。基底细胞通过半桥粒附着于新合成的基底膜。表层细胞在其顶端侧膜处通过连接复合体即终末棒封闭。不对称的腔面膜斑不明显。在第二种方法中,在胶原酶 - 胰蛋白酶消化外翻膀胱后,将上皮与下面的结缔组织分离。虽然消化物主要由上皮细胞组成,但当接种到传统的塑料生长表面时,这些细胞在首次传代时很少存活。在培养的第三周后,上皮细胞通常死亡,成纤维细胞或大的扁平上皮样细胞的缓慢生长菌落变得明显。上皮样细胞通过其典型的超微结构被鉴定为内皮细胞,显示有Weibel - Palade小体和吞饮小窝。这些细胞与抗因子VIII抗血清反应。当在血小板存在下孵育时,单层培养物的自由表面是非血栓形成性的。成纤维细胞是在差异胰蛋白酶消化后从严重污染的上皮细胞培养物中分离出来的。这三种细胞类型代表了用于侵袭性研究的体外肿瘤模型的正常对照细胞。所有这三种细胞类型都参与上皮 - 基质连接的形成和功能维持。细胞 - 细胞和细胞 - 基质相互作用的研究可能为理解肿瘤侵袭性提供重要线索,肿瘤侵袭性是一个始于上皮 - 基质连接并随着其破坏而进行的过程。

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