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Assessment of multidrug resistance on cell coculture patterns using scanning electrochemical microscopy

机译:使用扫描电化学显微镜评估细胞共培养模式的多药耐药性

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摘要

The emergence of resistance to multiple unrelated chemotherapeutic drugs impedes the treatment of several cancers. Although the involvement of ATP-binding cassette transporters has long been known, there is no in situ method capable of tracking this transporter-related resistance at the single-cell level without interfering with the cell’s environment or metabolism. Here, we demonstrate that scanning electrochemical microscopy (SECM) can quantitatively and noninvasively track multidrug resistance-related protein 1–dependent multidrug resistance in patterned adenocarcinoma cervical cancer cells. Nonresistant human cancer cells and their multidrug resistant variants are arranged in a side-by-side format using a stencil-based patterning scheme, allowing for precise positioning of target cells underneath the SECM sensor. SECM measurements of the patterned cells, performed with ferrocenemethanol and [Ru(NH3)6]3+ serving as electrochemical indicators, are used to establish a kinetic “map” of constant-height SECM scans, free of topography contributions. The concept underlying the work described herein may help evaluate the effectiveness of treatment administration strategies targeting reduced drug efflux.
机译:对多种无关化学疗法药物的耐药性的出现阻碍了几种癌症的治疗。尽管ATP结合盒转运蛋白的参与早已为人所知,但没有一种原位方法能够在不干扰细胞环境或新陈代谢的情况下在单细胞水平上追踪这种与转运蛋白相关的抗性。在这里,我们证明了扫描电化学显微镜(SECM)可以定量和无创地追踪模式化腺癌宫颈癌细胞中与多药耐药性相关的蛋白1依赖性多药耐药性。使用基于模板的图案化方案,将非耐药性人类癌细胞及其多药耐药性变体并排排列,从而可以将目标细胞精确定位在SECM传感器下方。用二茂铁甲醇和[Ru(NH3)6] 3 + 作为电化学指示剂进行的图案化细胞的SECM测量,用于建立恒定高度SECM扫描的动力学“图”,而无需地形贡献。本文所述工作的基础概念可能有助于评估针对药物流出减少的治疗管理策略的有效性。

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