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首页> 外文期刊>Cancer Cell International >Identification of the xenograft and its ascendant sphere-forming cell line as belonging to EBV-induced lymphoma, and characterization of the status of sphere-forming cells
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Identification of the xenograft and its ascendant sphere-forming cell line as belonging to EBV-induced lymphoma, and characterization of the status of sphere-forming cells

机译:鉴定异种移植物及其上升的成球细胞系属于EBV诱导的淋巴瘤,并鉴定成球细胞的状态

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We have characterized the human cell line arised from the Epstein–Barr virus (EBV) positive multiple myeloma aspirate subjected to the long-term cultivation. This cell line has acquired the ability to form free-floating spheres and to produce a xenograft upon transplantation into NOD/SCID mice. Cells from both in vitro culture and developed xenografts were investigated with a number of analytical approaches, including pathomorphological analysis, FISH analysis, and analysis of the surface antigens and of the VDJ locus rearrangement. The obtained results, as well as the confirmed presence of EBV, testify that both biological systems are derived from B-cells, which, in turn, is a progeny of the EBV-transformed B-cellular clone that supplanted the primordial multiple myeloma cells. Next we assessed whether cells that (i) were constantly present in vitro in the investigated cell line, (ii) were among the sphere-forming cells, and (iii) were capable of internalizing a fluorescent TAMRA-labeled DNA probe (TAMRA+ cells) belonged to one of the three types of undifferentiated bone marrow cells of a multiple myeloma patient: CD34+ hematopoietic stem cells, CD90+ mesenchymal stem cells, and clonotypic multiple myeloma cell. TAMRA+ cells were shown to constitute the fourth independent subpopulation of undifferentiated bone marrow cells of the multiple myeloma patient. We have demonstrated the formation of ectopic contacts between TAMRA+ cells and cells of other types in culture, in particular with CD90+ mesenchymal stem cells, followed by the transfer of some TAMRA+ cell material into the contacted cell.
机译:我们已经对人类细胞系进行了长期培养,该细胞系来自爱泼斯坦-巴尔病毒(EBV)阳性多发性骨髓瘤抽吸物。该细胞系具有形成自由漂浮的球体的能力,并具有在移植到NOD / SCID小鼠中后产生异种移植物的能力。用多种分析方法研究了来自体外培养和已发展的异种移植物的细胞,包括病理形态学分析,FISH分析,表面抗原分析和VDJ基因座重排。获得的结果以及已证实的EBV的存在证明,这两个生物学系统均源自B细胞,而B细胞又是EBV转化的B细胞克隆的后代,该克隆取代了原发性多发性骨髓瘤细胞。接下来,我们评估了(i)在所研究的细胞系中体外持续存在的细胞,(ii)是否在形成球体的细胞中以及(iii)是否能够内化荧光TAMRA标记的DNA探针(TAMRA +细胞)属于多发性骨髓瘤患者的三种类型的未分化骨髓细胞之一:CD34 +造血干细胞,CD90 +间充质干细胞和克隆型多发性骨髓瘤细胞。 TAMRA +细胞显示出构成多发性骨髓瘤患者未分化骨髓细胞的第四个独立亚群。我们已经证明了TAMRA +细胞与培养物中其他类型的细胞之间异位接触的形成,特别是与CD90 +间充质干细胞之间的异位接触,然后将一些TAMRA +细胞物质转移到接触的细胞中。

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