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In/Ex-sItu Detection of HBV DNA Using Dynamic Microcantilever

机译:使用动态微电子HBV DNA的/ ex原位检测

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The microcantilevers have emerged as a versatile biosensor, and showed excellent performance such as high sensitivity, high selectivity, and label-free detection. They have been successfully used for the detection of nucleic acids, disease marker proteins, cells, and pathogens including small molecules. So far, our group has successfully demonstrated the marker protein detection using the actuating layer (PZT)-embedded microcantilevers for the last decade. Here, we introduce in/ex-situ monitoring of the DNA binding events using performance improved actuating layer-embedded microcantilever sensors. To obtain the stable and reliable resonant frequency shifts, the microcantilevers were passivated with parylene-C film for in-situ detection and perfluorosilane (PF-Si) film for ex-situ detection. To achieve the recognition layer, the probe DNA (37-mer including T10 spacers) specific to HBV DNA was immobilized on the gold-coated microcantilever, and followed by backfilling of ethylene glycol spacer (HSC11-EG3-OH) to increase the DNA binding efficiency. After the surface treatment, the detection of HBV DNA (27-mer) was performed through two manners, in-situ and ex-situ. Target DNA in the range of 1 to 20 ìM and 10 nM to 5 ìM were applied for the in-situ and ex-situ detection respectively, and the resonant frequency shifts according to the concentration was examined quantitatively. From the results, we explained the relationship between the DNA hybridization and the nanomechanical response. In addition, we presented a hypothesis on the different tendency of in-situ and ex-situ results.
机译:微型膜已经出现为通用的生物传感器,并且表现出优异的性能,例如高灵敏度,高选择性和无标记检测。它们已成功用于检测核酸,疾病标志物,细胞和病原体,包括小分子。到目前为止,我们的小组已经成功地证明了过去十年的致动层(PZT)-embedded的微电势来证明标记蛋白检测。在这里,我们使用性能改进的致动层嵌入式微电机传感器介绍了对DNA结合事件的/前原位监测。为了获得稳定且可靠的谐振频率换档,将微膜与聚对二甲苯-C膜钝化的用于原位检测和全氟硅烷(PF-Si)膜,用于前原位检测。为了实现识别层,将特异于HBV DNA的探针DNA(包括T10间隔物)固定在金涂覆的微膜上,然后通过回填乙二醇间隔物(HSC11-EG3-OH)来增加DNA结合效率。表面处理后,通过两个方式,原位和前原位检测HBV DNA(27-ME1)的检测。施用1至20μm和10nm至5ìm的靶DNA分别用于原位和前原位检测,并且定量地检查根据浓度的谐振频率偏移。从结果中,我们解释了DNA杂交与纳米机械反应之间的关系。此外,我们提出了一个假设的原位趋势和前地结果。

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