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A comprehensive characterization of pancreatic ductal carcinoma cell lines: towards the establishment of an in vitro research platform.

机译:胰腺导管癌细胞系的全面表征:建立体外研究平台。

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There are a large number of stable pancreatic ductal carcinoma cell lines that are used by researchers worldwide. Detailed data about their differentiation status and growth features are, however, often lacking. We therefore attempted to classify commonly used pancreatic carcinoma cell lines according to defined cell biological criteria. Twelve pancreatic ductal adenocarcinoma cell lines were cultured as monolayers and spheroids and graded according to their ultrastructural features. The grading system was based on the integrity of membrane structures and on the presence of mucin granules, cell organelles, nuclear and cellular polymorphism, cell polarity, and lumen formation. On the basis of the resulting scores the cell lines were classified as well, moderately, or poorly differentiated. In addition, immunocytochemistry was performed for the markers cytokeratin 7, 8, 18, 19, carcinoembryonic antigen, MUC1 MUC2, MUC5, and MUC6. The population doubling time of monolayer cultures, determined by a tetrazolium salt based proliferation assay was correlated with the ultrastructural grade. The grading of the ultrastructural features of the monolayers, and particularly of the spheroids, revealed that Capan-1 and Capan-2 cells were well differentiated; Colo357, HPAF-2, Aspc-1, A818-4, BxPc3, and Panc89 cells were moderately differentiated and PancTu-I, Panc1, Pt45P1, and MiaPaCa-2 cells poorly differentiated. Membrane-bound MUC1 staining was a characteristic of well differentiated cell lines. The population doubling time of the monolayer cultures was related to the differentiation grade. No relationship was found between the p53, K-ras, DPC4/Smad4, or p16(INK4a) mutation status and the grade of differentiation. We conclude that the proposed ultrastructural grading system combined with the proliferative activity provides a basis for further comparative studies of pancreatic ductal adenocarcinoma cell lines.
机译:世界各地的研究人员都在使用大量稳定的胰腺导管癌细胞系。但是,通常缺少有关其分化状态和生长特征的详细数据。因此,我们试图根据定义的细胞生物学标准对常用的胰腺癌细胞系进行分类。将十二个胰腺导管腺癌细胞系培养为单层和球状,并根据其超微结构特征进行分级。该分级系统基于膜结构的完整性以及粘蛋白颗粒,细胞器,核和细胞多态性,细胞极性和管腔形成的存在。根据所得的分数,将细胞系分为好,中或低分化。此外,对标记细胞角蛋白7、8、18、19,癌胚抗原,MUC1,MUC2,MUC5和MUC6进行了免疫细胞化学分析。通过基于四唑盐的增殖测定法确定的单层培养的群体倍增时间与超微结构等级相关。单层,特别是球状体的超微结构特征的分级显示,Capan-1和Capan-2细胞分化良好。 Colo357,HPAF-2,Aspc-1,A818-4,BxPc3和Panc89细胞中等分化,而PancTu-1,Panc1,Pt45P1和MiaPaCa-2细胞分化差。膜结合MUC1染色是高分化细胞系的特征。单层培养的群体倍增时间与分化程度有关。在p53,K-ras,DPC4 / Smad4或p16(INK4a)突变状态与分化程度之间未发现任何关系。我们得出的结论是,拟议的超微结构分级系统结合了增殖活性,为胰腺导管腺癌细胞系的进一步比较研究提供了基础。

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