细胞死亡的高频超声检测:体外不同形式细胞死亡的光谱分化

Maurice Pasternak, A. Sadeghi-Naini, Shawn Ranieri, A. Giles, M. Oelze, Michael C. Kolios, G. Czarnota
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引用次数: 11

摘要

研究了高频定量超声技术表征体外不同形式的细胞死亡。悬浮生长的急性髓系白血病细胞经处理后可引起细胞凋亡、肿瘤、有丝分裂停止和热致死亡。用20和40 MHz超声扫描样本,并根据细胞结构进行组织学评估。20 MHz超声数据的频域分析显示,48小时顺铂诱导的细胞凋亡、48小时肿瘤坏死、36小时秋水仙碱诱导的有丝分裂停止和热处理后,中频拟合变化分别为6.0±0.7 dBr、6.2±1.8 dBr、4.0±1.0 dBr和- 4.6±1.7 dBr。40兆赫超声波的趋势相似。从40兆赫超声数据中获得的光谱斜率变化反映了细胞和细胞核大小的变化。染色质固缩或溶解趋势表明核物质的密度可能是超声后向散射观察到的变化的原因。流式细胞术分析证实了细胞死亡模式,并支持超声数据的中带拟合趋势。从充满流体的球体形状因子模型获得的散射体大小和浓度估计进一步与光谱分析和组织学相对应。结果表明,定量超声光谱分析可用于探讨体外肿瘤的抗癌反应和区分不同的细胞死亡模式。
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High-frequency ultrasound detection of cell death: Spectral differentiation of different forms of cell death in vitro
High frequency quantitative ultrasound techniques were investigated to characterize different forms of cell death in vitro. Suspension-grown acute myeloid leukemia cells were treated to cause apoptosis, oncosis, mitotic arrest, and heat-induced death. Samples were scanned with 20 and 40 MHz ultrasound and assessed histologically in terms of cellular structure. Frequency-domain analysis of 20 MHz ultrasound data demonstrated midband fit changes of 6.0 ± 0.7 dBr, 6.2 ± 1.8 dBr, 4.0 ± 1.0 dBr and −4.6 ± 1.7 dBr after 48-hour cisplatinum-induced apoptosis, 48-hour oncotic decay, 36-hour colchicine-induced mitotic arrest, and heat treatment compared to control, respectively. Trends from 40 MHz ultrasound were similar. Spectral slope changes obtained from 40 MHz ultrasound data were reflective of alterations in cell and nucleus size. Chromatin pyknosis or lysis trends suggested that the density of nuclear material may be responsible for observed changes in ultrasound backscatter. Flow cytometry analysis confirmed the modes of cell death and supported midband fit trends in ultrasound data. Scatterer-size and concentration estimates obtained from a fluid-filled sphere form factor model further corresponded with spectral analysis and histology. Results indicate quantitative ultrasound spectral analysis may be used for probing anti-cancer response and distinguishing various modes of cell death in vitro.
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