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利用共焦拉曼光谱技术在图案化单细胞生物传感器上检测药物诱导的细胞变化。

Detection of drug-induced cellular changes using confocal Raman spectroscopy on patterned single-cell biosensors.

机构信息

Department of Materials Science & Engineering, University of Washington, 302L Roberts Hall, Seattle, WA 98195-2120, USA.

出版信息

Analyst. 2009 Jul;134(7):1440-6. doi: 10.1039/b900420c. Epub 2009 Apr 30.

Abstract

We report on a cell-based biosensor application that utilizes patterned single-cell arrays combined with confocal Raman spectroscopy to observe the time-dependent drug response of individual cells in real time. The patterned single-cell platform enables individual cells to be easily located and continuously addressable for Raman spectroscopy characterization of biochemical compositional changes in a non-destructive, quantitative manner so that discrete cellular behavior and cell-to-cell variations are preserved. In this study, human medulloblastoma (DAOY) cells were exposed to the common chemotherapeutic agent etoposide, and Raman spectra from patterned cells were recorded over 48 hours. It was found that 87.5% of the cells monitored exhibited a sharp decrease in DNA and protein associated peaks 48 hours after drug exposure, corresponding to cell death. The remaining 12.5% of the cells showed little to no reduction in key Raman biomarkers, indicating their drug resistance. Furthermore, the patterned cell population showed a very similar response to etoposide as confluent cell cultures, as confirmed by flow cytometry. Finally, patterned cells were assessed with TUNEL assay for apoptosis due to DNA fragmentation after etoposide exposure. The results agree well with those from the Raman spectroscopy analysis. This combined biosensor-Raman platform provides a quick, simple way to assess cell responses to chemical and biological agents with high throughput and can be potentially used for a wide variety of biomedical applications such as pharmaceutical drug discovery, toxin tests, and biothreat detection.

摘要

我们报告了一种基于细胞的生物传感器应用,该应用利用图案化单细胞阵列结合共焦拉曼光谱,实时观察单个细胞的时间依赖性药物反应。图案化单细胞平台使单个细胞能够轻松定位,并可连续进行拉曼光谱特征分析,以非破坏性、定量的方式观察生物化学成分的变化,从而保留离散的细胞行为和细胞间的变化。在这项研究中,人类髓母细胞瘤(DAOY)细胞暴露于常见的化疗药物依托泊苷中,并在 48 小时内记录图案化细胞的拉曼光谱。结果发现,87.5%的监测细胞在药物暴露 48 小时后,与 DNA 和蛋白质相关的峰急剧下降,这与细胞死亡相对应。其余 12.5%的细胞显示出很少或没有关键拉曼生物标志物的减少,表明它们具有耐药性。此外,图案化细胞群体对依托泊苷的反应与汇合细胞培养物非常相似,这通过流式细胞术得到了证实。最后,用 TUNEL assay 评估了依托泊苷暴露后由于 DNA 片段化引起的凋亡。结果与拉曼光谱分析的结果吻合较好。这种组合的生物传感器-拉曼平台提供了一种快速、简单的方法来评估细胞对化学和生物制剂的反应,具有高通量,可潜在用于各种生物医学应用,如药物发现、毒素测试和生物威胁检测。

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