首页> 外文期刊>In Vitro Cellular and Developmental Biology. Animal: Journal of the Tissues Culture Association >Microgravity assay of neuroblastoma: in vitro aggregation kinetics and organoid morphology correlate with MYCN expression
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Microgravity assay of neuroblastoma: in vitro aggregation kinetics and organoid morphology correlate with MYCN expression

机译:神经母细胞瘤的微重力测定:体外聚集动力学和类器官形态与MYCN表达相关

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Neuroblastoma, the most common and deadly solid pediatric tumor, features genetic and biologic heterogeneity that defies simple risk assessments, drives diverse clinical behavior, and demands more extensive characterization. This research served to investigate the utility of a microgravity assay-rotary bioreactor culture-to evaluate and characterize the cell-specific, in vitro behavior of neuroblastoma cell lines: aggregation kinetics of single cells and the morphology of the formed structures, called organoids. Specifically, we examined the effect of amplification of the oncogene MYCN, a genetic factor that is strongly associated with poor clinical outcome. Three human neuroblastoma cell lines with varied MYCN expression (CHP-212 (unamplified), SK-N-AS (unamplified), IMR-32 (amplified)) were cultured in the microgravity rotary bioreactor. Simple aggregation kinetics were determined by periodically performing counts of non-aggregated single cells in the media. Organoids were harvested, stained with hematoxylin and eosin, and evaluated microscopically in terms of size and shape. The MYCN-amplified cell line (IMR32) aggregated much more rapidly than the unamplified cell lines, as indicated by a significantly lower area under its aggregation curve (single non-aggregated cells vs. time): IMR32 = 4.3, CHP-212 =12.4, SK-N-AS = 9.8 (adhesion index x10(5)). Further, the organoid morphology of the MYCN-amplified cell line was noticeably different compared to the unamplified lines. The CHP-212 and SK-N-AS cells formed spherical structures with average cross-sectional area 0.213 and 0.138 mm(2), respectively, and featured an outer viable zone of cells (average length of 0.175, 0.129 mm, respectively; the "diffusion distance"), surrounding an inner necrotic core. In contrast, the MYCN-amplified cell line formed a large single mass of cells but had a similar diffusion distance (0.175 mm). This microgravity assay provides a rapid, reproducible assessment of in vitro behavior of neuroblastoma, and the measured parameters, aggregation kinetics and organoid size and shape correlated with malignant potential in terms of MYCN amplification. This assay allows for the examination of cell-specific biologic and genetic factors that should provide valuable insight into the clinical behavior of neuroblastoma.
机译:神经母细胞瘤是最常见和致命的小儿实体瘤,具有遗传和生物学异质性,无视简单的风险评估,驱动多种临床行为并需要更广泛的表征。这项研究有助于调查微重力测定法-旋转生物反应器培养的效用,以评估和表征神经母细胞瘤细胞系的细胞特异性体外行为:单个细胞的聚集动力学和形成的结构(称为类器官)的形态。具体来说,我们检查了癌基因MYCN的扩增效果,该基因是与不良临床结局密切相关的遗传因素。在微重力旋转生物反应器中培养了三种具有不同MYCN表达的人神经母细胞瘤细胞系(CHP-212(未扩增),SK-N-AS(未扩增),IMR-32(已扩增))。通过定期对培养基中未聚集的单细胞进行计数来确定简单的聚集动力学。收集类器官,用苏木精和曙红染色,并在大小和形状方面进行显微镜评估。 MYCN扩增的细胞系(IMR32)的聚集速度比未扩增的细胞系快得多,这是由其聚集曲线下的面积明显减小(单个非聚集的细胞与时间的关系)所表示的:IMR32 = 4.3,CHP-212 = 12.4 ,SK-N-AS = 9.8(粘合指数×10(5))。此外,MYCN扩增的细胞系的类器官形态与未扩增的系明显不同。 CHP-212和SK-N-AS电池分别形成平均横截面积为0.213和0.138 mm(2)的球形结构,并具有电池的外部可行区(平均长度分别为0.175、0.129 mm; “扩散距离”),围绕内部坏死核。相反,MYCN扩增的细胞系形成大量单个细胞,但具有相似的扩散距离(0.175 mm)。这种微重力测定提供了对神经母细胞瘤体外行为的快速,可再现的评估,并且根据MYCN扩增,所测得的参数,聚集动力学以及类器官的大小和形状与恶性潜能相关。该测定法可以检查特定于细胞的生物学和遗传因素,这些因素应为神经母细胞瘤的临床行为提供有价值的见解。

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