Fluorescence In Situ Hybridization (FISH) for the Characterization and Monitoring of Primary Cultures from Human Tumors

Ruth Román-Lladó, C. Aguado, N. Jordana-Ariza, Jaume Roca-Arias, S. Rodríguez, E. Aldeguer, Mónica Garzón-Ibáñez, B. García-Peláez, M. Vives-Usano, A. Giménez-Capitán, A. Aguilar, A. Martínez-Bueno, M. G. Cao, F. García-Casabal, S. Viteri, C. Mayo de las Casas, R. Rosell, M. Molina-Vila
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Abstract

Genetic and drug sensitivity assays on primary cultures are not only of basic but also of translational interest and could eventually aid oncologists in the selection of treatments. However, cancer cells need to be identified and differentiated from the non-tumor cells always present in primary cultures. Also, successive passages can change the proportions of these two subpopulations. In this study, we propose fluorescence in situ hybridization (FISH) analysis on cell smears to determine the presence of tumor cells in primary cultures obtained from patients carrying translocations or copy number gains. FISH proved to be an easy, fast, economic, and reliable method of characterizing cell populations, which could be used repeatedly at different passages to monitor variations and to confirm the maintenance of translocations and copy number gains throughout the culture process.
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荧光原位杂交(FISH)用于人类肿瘤原代培养物的表征和监测
原代培养的遗传和药物敏感性分析不仅具有基础意义,而且具有转化意义,最终可以帮助肿瘤学家选择治疗方法。然而,癌细胞需要从非肿瘤细胞中识别和区分,而非肿瘤细胞总是存在于原代培养中。同时,连续传代可以改变这两个亚种群的比例。在这项研究中,我们提出对细胞涂片进行荧光原位杂交(FISH)分析,以确定从携带易位或拷贝数增加的患者获得的原代培养物中是否存在肿瘤细胞。FISH被证明是一种简单、快速、经济和可靠的表征细胞群体的方法,可以在不同的传代中重复使用,以监测变异,并确认在整个培养过程中易位和拷贝数增益的维持。
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