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Tumor-stem cells interactions by fluorescence imaging

机译:肿瘤干细胞相互作用的荧光成像

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Recently, great deal of interest is investigation the function of the stem cells (SC) in tumors. In this study, we studied «recipient-tumor- fluorescent stem cells » system using the methods of in vivo imaging and laser scanning microscopy (LSM). We used adipose-derived adult stem (ADAS) cells of human lentiviral transfected with the gene of fluorescent protein Turbo FP635. ADAS cells were administrated into nude mice with transplanted tumor HeLa Kyoto (human cervical carcinoma) at different stages of tumor growth (0-8 days) intravenously or into tumor. In vivo imaging was performed on the experimental setup for epi - luminescence bioimaging (IAP RAS, Nizhny Novgorod). The results of the imaging showed localization of fluorophore tagged stem cells in the spleen on day 5-9 after injection. The sensitivity of the technique may be improved by spectral separation autofluorescence and fluorescence of stem celts. We compared the results of in vivo imaging and confocal laser scanning microscopy (LSM 510 META, Carl Zeiss, Germany). Internal organs of the animals and tumor tissue were investigated. It was shown that with i.v. injection of ADAS, bright fluorescent structures with spectral characteristics corresponding to TurboFP635 protein are locally accumulated in the marrow, lungs and tumors of animals. These findings indicate that ADAS cells integrate in the animal body with transplanted tumor and can be identified by fluorescence bioimaging techniques in vivo and ex vivo.
机译:近来,引起人们极大兴趣的是研究干细胞(SC)在肿瘤中的功能。在这项研究中,我们使用体内成像和激光扫描显微镜(LSM)的方法研究了“受体-肿瘤-荧光干细胞”系统。我们使用转染了荧光蛋白Turbo FP635基因的人慢病毒的脂肪来源成人干细胞(ADAS)。将ADAS细胞静脉内或在肿瘤生长的不同阶段(0-8天)施用于具有移植的肿瘤HeLa Kyoto(人宫颈癌)的裸鼠。在落射荧光生物成像的实验装置(IAP RAS,下诺夫哥罗德)上进行体内成像。成像结果显示荧光素标记的干细胞在注射后第5-9天在脾脏中定位。该技术的灵敏度可以通过光谱分离自发荧光和茎干的荧光来提高。我们比较了体内成像和共聚焦激光扫描显微镜(LSM 510 META,卡尔·蔡司,德国)的结果。研究了动物的内脏器官和肿瘤组织。事实证明,与注射ADAS后,具有与TurboFP635蛋白相对应的光谱特征的明亮的荧光结构局部聚集在动物的骨髓,肺和肿瘤中。这些发现表明ADAS细胞与移植的肿瘤整合在动物体内,并且可以通过体内和离体的荧光生物成像技术进行鉴定。

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