基于体外药物敏感性成像的原发性急性淋巴细胞白血病细胞平台。

Lauren Rowland, Brandon Smart, Anthony Brown, Gino M Dettorre, Yoshihiro Gocho, Jeremy Hunt, Wenjian Yang, Satoshi Yoshimura, Noemi Reyes, Guoqing Du, August John, Dylan Maxwell, Wendy Stock, Steven Kornblau, Mary V Relling, Hiroto Inaba, Ching-Hon Pui, Jean-Pierre Bourquin, Seth E Karol, Charles G Mullighan, William E Evans, Jun J Yang, Kristine R Crews
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引用次数: 0

摘要

急性淋巴细胞白血病(ALL)细胞对化疗的耐药性,无论是在诊断时出现还是在治疗过程中获得,都是治疗失败的主要原因。原发性ALL细胞可用于新诊断或复发时的药物敏感性试验,但目前测定体外药物敏感性的方法存在主要局限性。在这里,我们描述了一种功能精准医学方法,使用荧光成像平台来测试原代ALL细胞的药物敏感性谱。白血病细胞与间充质间质细胞共培养,用40种抗白血病药物进行测试,以确定耐药性和敏感性的个体模式(“药效型”)。这种基于成像的药物分型分析方法通过自动化数据分析来产生高通量数据,从而解决了先前体外药物敏感性方法的局限性,同时需要更少的细胞,并显着减少了进行分析所需的劳动密集型时间。药物敏感性数据与基因组图谱的整合为基因组学指导下的合理精准医疗提供了依据。主要特征分析原发性急性淋巴细胞白血病(ALL)在骨髓抽吸或外周血诊断时获得的母细胞。实验采用间充质间质细胞体外共培养,需4天完成。这种基于荧光成像的方案增强了以前的体外药物敏感性分析,并通过需要更少的原代细胞而提高效率,同时将测试的药物数量增加到40种。样品制备和处理大约需要2-3小时,成像时间为1.5小时。图形的概述。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Ex vivo Drug Sensitivity Imaging-based Platform for Primary Acute Lymphoblastic Leukemia Cells.

Ex vivo Drug Sensitivity Imaging-based Platform for Primary Acute Lymphoblastic Leukemia Cells.

Ex vivo Drug Sensitivity Imaging-based Platform for Primary Acute Lymphoblastic Leukemia Cells.

Ex vivo Drug Sensitivity Imaging-based Platform for Primary Acute Lymphoblastic Leukemia Cells.

Resistance of acute lymphoblastic leukemia (ALL) cells to chemotherapy, whether present at diagnosis or acquired during treatment, is a major cause of treatment failure. Primary ALL cells are accessible for drug sensitivity testing at the time of new diagnosis or at relapse, but there are major limitations with current methods for determining drug sensitivity ex vivo. Here, we describe a functional precision medicine method using a fluorescence imaging platform to test drug sensitivity profiles of primary ALL cells. Leukemia cells are co-cultured with mesenchymal stromal cells and tested with a panel of 40 anti-leukemia drugs to determine individual patterns of drug resistance and sensitivity ("pharmacotype"). This imaging-based pharmacotyping assay addresses the limitations of prior ex vivo drug sensitivity methods by automating data analysis to produce high-throughput data while requiring fewer cells and significantly decreasing the labor-intensive time required to conduct the assay. The integration of drug sensitivity data with genomic profiling provides a basis for rational genomics-guided precision medicine. Key features Analysis of primary acute lymphoblastic leukemia (ALL) blasts obtained at diagnosis from bone marrow aspirate or peripheral blood. Experiments are performed ex vivo with mesenchymal stromal cell co-culture and require four days to complete. This fluorescence imaging-based protocol enhances previous ex vivo drug sensitivity assays and improves efficiency by requiring fewer primary cells while increasing the number of drugs tested to 40. It takes approximately 2-3 h for sample preparation and processing and a 1.5-hour imaging time. Graphical overview.

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