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STR 基因座异常在 Jurkat 细胞系亚克隆中的积累作为肿瘤克隆进化的模型。

Accumulation of STR-Loci Aberrations in Subclones of Jurkat Cell Line as a Model of Tumor Clonal Evolution.

机构信息

National Research Center for Hematology, 125167 Moscow, Russia.

School of Medicine, Lomonosov Moscow State University, 119991 Moscow, Russia.

出版信息

Genes (Basel). 2023 Feb 24;14(3):571. doi: 10.3390/genes14030571.

Abstract

Many genetic markers are known to distinguish tumor cells from normal. Genetic lesions found at disease onset often belong to a predominant tumor clone, and further observation makes it possible to assess the fate of this clone during therapy. However, minor clones escape monitoring and become unidentified, leading to relapses. Here we report the results of in vitro study of clonal evolution in cultured tumor cell line (Jurkat) compared to the cell line of non-tumor origin (WIL2-S). Cell lines were cultured and cloned by limiting dilutions. Subclones were tested by short tandem repeats (STR) profiling. Spontaneous STR aberrations in cells of non-tumor origin occur in less than 1 of 100 cultured cells. While in the cells of tumor origin, new aberrations appear in 1 or even more of 3 cultured cells. At the same time, a significant relationship was found between the accumulation of aberrations in the pool of subclones and the rate of cell growth. One can speculate that this approach could be applied for the analysis of primary patient tumor cell culture to obtain information concerning the evolutionary potential of the tumor cells that may be useful for the selection of a therapy approach.

摘要

许多遗传标记可用于区分肿瘤细胞和正常细胞。疾病起始时发现的遗传病变通常属于主要的肿瘤克隆,进一步的观察使我们能够评估该克隆在治疗过程中的命运。然而,小克隆逃避监测并变得无法识别,导致复发。在这里,我们报告了体外培养肿瘤细胞系(Jurkat)与非肿瘤起源细胞系(WIL2-S)克隆进化比较的研究结果。细胞系通过有限稀释进行培养和克隆。通过短串联重复(STR)分析对亚克隆进行测试。非肿瘤起源细胞中的自发 STR 异常少于每 100 个培养细胞中的 1 个。而在肿瘤起源的细胞中,新的异常出现在 1 个甚至 3 个培养细胞中的 1 个。同时,还发现亚克隆池中的异常积累与细胞生长速度之间存在显著关系。可以推测,这种方法可应用于原发性患者肿瘤细胞培养的分析,以获得有关肿瘤细胞进化潜力的信息,这可能对治疗方法的选择有用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/936c/10048572/2d0c4e110683/genes-14-00571-g001.jpg

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