首页> 美国卫生研究院文献>Toxicology Reports >Cell culture conditions affect the ability of high content imaging assay to detect drug-induced changes in cellular parameters in human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs)
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Cell culture conditions affect the ability of high content imaging assay to detect drug-induced changes in cellular parameters in human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs)

机译:细胞培养条件影响高含量成像分析检测人类诱导的多能干细胞来源的心肌细胞(hiPSC-CMs)中药物诱导的细胞参数变化的能力

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摘要

Human induced pluripotent stem cell-derived cardiomyocytes (hiPSC-CMs) are widely used for drug safety and efficacy testing with various techniques, including high content imaging (HCI). Upon drug treatment, a significant number of hiPSC-CMs grown in regular 96-well plates coated with fibronectin detached from the bottom of the plate, complicating data acquisition. Several cell culture configurations were tested to improve cell adherence, and the effects of these configurations on total cell number, separation of feature values between the negative (DMSO 0.1%) and positive (antimycin, staurosporine) controls, scale of feature value differences, and data variability were statistically calculated. hiPSC-CMs were plated on fibronectin- (in “blanket” configuration) or MaxGel- (in “sandwich” configuration) coated plates and covered with a layer of either HydroMatrix or MaxGel 2, 7, or 11d after plating. After a total of 14d in culture, cells were treated with compounds, labeled with four fluorescent dyes (Hoechst, TMRM, NucView, and RedDot), and imaged with GE INCell2000. Based on the statistical parameters calculated, the MaxGel 25% 7d “sandwich” was superior to all other tested conditions when the cells were treated with 0.3 μM antimycin for 2 h and test compounds 10 μM crizotinib and 30 μM amiodarone for 48 h. For staurosporine treatment, the best culturing condition varied between MaxGel “sandwich” systems, depending on which parameters were under consideration. Thus, cell culturing conditions can significantly affect the ability of high content imaging to detect changes in cellular features during compound treatment and should be thoroughly evaluated before committing to compound testing.
机译:人类诱导的多能干细胞衍生的心肌细胞(hiPSC-CMs)已通过多种技术(包括高含量成像(HCI))广泛用于药物安全性和功效测试。经过药物处理,大量的hiPSC-CMs在覆盖有纤连蛋白的常规96孔板中从板底部脱离,使数据采集变得复杂。测试了几种细胞培养配置以改善细胞粘附性,以及这些配置对总细胞数,阴性(DMSO 0.1%)和阳性(抗霉素,星形孢菌素)对照之间的特征值分离,特征值差异的范围以及统计上计算数据变异性。将hiPSC-CMs镀在纤连蛋白-(“毯”构型)或MaxGel-(“三明治”构型)包被的板上,并在镀膜后用HydroMatrix或MaxGel 2、7或11d覆盖一层。培养总共14天后,将细胞用化合物处理,用四种荧光染料(Hoechst,TMRM,NucView和RedDot)标记,并用GE INCell2000成像。根据计算的统计参数,当将细胞分别用0.3μmM抗霉素处理2h和10μmcrizotinib和30μm胺碘酮处理48h时,MaxGel 25%7d“三明治”优于所有其他测试条件。对于星形孢菌素治疗,MaxGel“三明治”系统的最佳培养条件有所不同,具体取决于所考虑的参数。因此,细胞培养条件会显着影响高内涵成像检测化合物处理过程中细胞特征变化的能力,在进行化合物测试之前应进行彻底评估。

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