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对场效应晶体管单个细胞结合事件的时间依赖性观察。

Time-dependent observation of individual cellular binding events to field-effect transistors.

作者信息

Schäfer S, Eick S, Hofmann B, Dufaux T, Stockmann R, Wrobel G, Offenhäusser A, Ingebrandt S

机构信息

Institute of Bio- and Nanosystems (IBN-2) and Center of Nanoelectronic Systems for Information Technology, Forschungszentrum Jülich GmbH, 52425 Jülich, Germany.

出版信息

Biosens Bioelectron. 2009 Jan 1;24(5):1201-8. doi: 10.1016/j.bios.2008.07.003. Epub 2008 Jul 12.

DOI:10.1016/j.bios.2008.07.003
PMID:18692383
Abstract

Electrolyte-gate field-effect transistors (EG-FETs) gained continuously more importance in the field of bioelectronics. The reasons for this are the intrinsic properties of these FETs. Binding of analysts or changes in the electrolyte composition are leading to variations of the drain-source current. Furthermore, due to the signal amplification upon voltage-to-current conversion even small extracellular signals can be detected. Here we report about impedance spectroscopy with an FET array to characterize passive components of a cell attached to the transistor gate. We developed a 16-channel readout system, which provides a simultaneous, lock-in based readout. A test signal of known amplitude and phase was applied via the reference electrode. We monitored the electronic transfer function of the FETs with the attached cell. The resulting frequency spectrum was used to investigate the surface adhesion of individual HEK293 cells. We applied different chemical treatments with either the serinpeptidase trypsin or the ionophor amphotericin B (AmpB). Binding studies can be realized by a time-dependent readout of the lock-in amplifier at a constant frequency. We observed cell detachment upon trypsin activity as well as membrane decomposition induced by AmpB. The results were interpreted in terms of an equivalent electrical circuit model of the complete system. The presented method could in future be applied to monitor more relevant biomedical manipulations of individual cells. Due to the utilization of the silicon technology, our method could be easily up-scaled to many output channels for high throughput pharmacological screening.

摘要

电解质栅场效应晶体管(EG - FET)在生物电子学领域的重要性持续增加。原因在于这些FET的固有特性。分析物的结合或电解质成分的变化会导致漏源电流的变化。此外,由于电压 - 电流转换时的信号放大,即使是微小的细胞外信号也能被检测到。在此,我们报告一种使用FET阵列进行阻抗谱分析的方法,以表征附着在晶体管栅极上的细胞的无源元件。我们开发了一个16通道读出系统,该系统提供基于锁相放大器的同步读出。通过参比电极施加已知幅度和相位的测试信号。我们监测了带有附着细胞的FET的电子传递函数。所得频谱用于研究单个HEK293细胞的表面粘附情况。我们用丝氨酸蛋白酶胰蛋白酶或离子载体两性霉素B(AmpB)进行了不同的化学处理。结合研究可以通过在恒定频率下对锁相放大器进行随时间的读出实现。我们观察到胰蛋白酶活性导致细胞 detachment以及AmpB诱导的膜分解。结果根据整个系统的等效电路模型进行了解释。所提出的方法未来可应用于监测单个细胞更相关的生物医学操作。由于采用了硅技术,我们的方法可以很容易地扩展到许多输出通道,用于高通量药理学筛选。 (注:原文中“cell detachment”未明确中文释义,暂保留英文)

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