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Dielectrophoresis-based cellular microarray chip for anticancer drug screening in perfusion microenvironments

机译:基于介电电泳的细胞微阵列芯片在灌注微环境中的抗癌药物筛选

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摘要

We present a dielectrophoresis (DEP)-based cellular microarray chip for cell-based anticancer drug screening in perfusion microenvironments. Human breast cancer cells, MCF7, were seeded into the chip and patterned via DEP forces onto the planar inter digitated ring electrode (PIRE) arrays. Roughly, only one third of the cell amount was required for the chip compared to that for a 96-well plate control. Drug concentrations (cisplatin or docetaxel) were stably generated by functional integration of a concentration gradient generator (CGG) and an anti-crosstalk valve (ACV) to treat cells for 24 hours. Cell viability was quantified using a dual staining method. Results of cell patterning show substantial uniformity of patterned cells (92 ± 5 cells per PIRE). Furthermore, after 24 hour drug perfusion, no statistical significance in dose-responses between the chip and the 96-well plate controls was found. The IC_(50) value from the chip also concurred with the values from the literature. Moreover, the perfusion culture exhibited reproducibility of drug responses of cells on different PIREs in the same chamber. The chip would enable applications where cells are of limited supply, and supplement microfluidic perfusion cultures for clinical practices.
机译:我们提出了一种基于介电泳(DEP)的细胞微阵列芯片,用于在灌注微环境中进行基于细胞的抗癌药物筛选。将人乳腺癌细胞MCF7接种到芯片中,并通过DEP力将其图案化到平面叉指环电极(PIRE)阵列上。大致而言,与96孔板对照相比,芯片仅需要细胞数量的三分之一。通过浓度梯度发生器(CGG)和抗串扰阀(ACV)的功能整合,可以稳定地产生药物浓度(顺铂或多西他赛),以处理细胞24小时。使用双重染色方法定量细胞活力。细胞图案化的结果显示出图案化细胞的均匀性(每个PIRE为92±5个细胞)。此外,在药物灌注24小时后,在芯片与96孔板对照之间的剂量反应中未发现统计学意义。芯片的IC_(50)值也与文献中的值一致。此外,灌注培养在同一腔室中展示了不同PIREs上细胞的药物反应的可重复性。该芯片将使细胞供应有限的应用成为可能,并为临床实践补充微流灌注培养。

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