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Tracing DiO-labelled tumour cells in liver sections by confocal laser scanning microscopy.

机译:通过共聚焦激光扫描显微镜追踪肝脏切片中DiO标记的肿瘤细胞。

摘要

Investigating rare cellular events is facilitated by studying thick sections with confocal laser scanning microscopy (CLSM). Localization of cells in tissue sections can be done by immunolabelling or by fluorescent labelling of cells prior to intravenous administration. Immunolabelling is technically complicated because of the preservation of antigens during fixation and the problems associated with the penetration of the antibodies. In this study, an alternative and simple approach for the labelling of cells in vitro with the fluorescent probe DiO and its subsequent application in vivo will be outlined. The method was applied to trace DiO-labelled colon carcinoma cells (CC531s) in 100 microm thick liver sections. In vitro and in vivo experiments revealed that DiO-labelling of CC531s cells had no cytotoxic or antiproliferative effect and the cells preserved their susceptibility towards hepatic NK cells or Kupffer cells. In addition, DiO remained stable for at least 72 h in the living cell. DiO-labelled CC531s cells could be traced all over the tissue depth and anti-metastatic events such as phagocytosis of tumour cells by Kupffer cells could be easily observed. In situ staining with propidium iodide (nucleic acids) or rhodamine-phalloidin (filamentous actin) resulted in additional tissue information. The data presented improved the understanding of the possible effects of the vital fluorescent probe DiO on cell function and provided a limit of confidence for CLSM imaging of DiO-labelled cells in tissue sections.
机译:通过使用共聚焦激光扫描显微镜(CLSM)研究厚切片,有助于研究罕见的细胞事件。可以在静脉内施用之前通过免疫标记或通过荧光标记细胞来完成组织切片中细胞的定位。由于固定过程中抗原的保存以及与抗体渗透有关的问题,免疫扩口技术在技术上很复杂。在这项研究中,将概述使用荧光探针DiO体外标记细胞的另一种简单方法及其在体内的后续应用。该方法用于在100微米厚的肝脏切片中痕量DiO标记的结肠癌细胞(CC531s)。体外和体内实验表明,CC531s细胞的DiO标记没有细胞毒性或抗增殖作用,并且细胞保留了它们对肝NK细胞或库普弗细胞的敏感性。此外,DiO在活细胞中保持稳定至少72小时。可以在整个组织深度上追踪DiO标记的CC531s细胞,并且可以很容易地观察到抗转移事件,例如库普弗细胞吞噬肿瘤细胞。用碘化丙啶(核酸)或若丹明-鬼笔环肽(丝状肌动蛋白)原位染色可产生其他组织信息。呈现的数据增进了对重要荧光探针DiO对细胞功能可能影响的理解,并为组织切片中DiO标记细胞的CLSM成像提供了可信度限制。

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