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基于微点的微流控 ELISA:使用集成薄膜氢化非晶硅光电二极管的化学发光和比色检测。

Microspot-based ELISA in microfluidics: chemiluminescence and colorimetry detection using integrated thin-film hydrogenated amorphous silicon photodiodes.

机构信息

INESC Microsistemas e Nanotecnologias and IN-Institute of Nanoscience and Nanotechnology, Lisbon, Portugal.

出版信息

Lab Chip. 2011 Dec 7;11(23):4063-71. doi: 10.1039/c1lc20362b. Epub 2011 Oct 20.

DOI:10.1039/c1lc20362b
PMID:22012414
Abstract

Microfluidic technology has the potential to decrease the time of analysis and the quantity of sample and reactants required in immunoassays, together with the potential of achieving high sensitivity, multiplexing, and portability. A lab-on-a-chip system was developed and optimized using optical and fluorescence microscopy. Primary antibodies are adsorbed onto the walls of a PDMS-based microchannel via microspotting. This probe antibody is then recognised using secondary FITC or HRP labelled antibodies responsible for providing fluorescence or chemiluminescent and colorimetric signals, respectively. The system incorporated a micron-sized thin-film hydrogenated amorphous silicon photodiode microfabricated on a glass substrate. The primary antibody spots in the PDMS-based microfluidic were precisely aligned with the photodiodes for the direct detection of the antibody-antigen molecular recognition reactions using chemiluminescence and colorimetry. The immunoassay takes ~30 min from assay to the integrated detection. The conditions for probe antibody microspotting and for the flow-through ELISA analysis in the microfluidic format with integrated detection were defined using antibody solutions with concentrations in the nM-μM range. Sequential colorimetric or chemiluminescence detection of specific antibody-antigen molecular recognition was quantitatively detected using the photodiode. Primary antibody surface densities down to 0.182 pmol cm(-2) were detected. Multiplex detection using different microspotted primary antibodies was demonstrated.

摘要

微流控技术具有缩短分析时间、减少所需样品和反应物数量的潜力,同时还具有实现高灵敏度、多重检测和便携性的潜力。本研究开发并优化了一种基于光学和荧光显微镜的芯片实验室系统。通过微点样将抗体固定在 PDMS 基微通道的壁上。然后,使用二级 FITC 或 HRP 标记的抗体识别探针抗体,这些抗体分别负责提供荧光、化学发光和比色信号。该系统集成了一个在玻璃衬底上制造的微米级氢化非晶硅薄膜光电二极管。PDMS 基微流控中的一级抗体斑点与光电二极管精确对准,用于直接检测化学发光和比色法的抗体-抗原分子识别反应。免疫分析从检测到集成检测大约需要 30 分钟。使用浓度在 nM-μM 范围内的抗体溶液,定义了用于探针抗体微点样和用于微流控格式中流动式 ELISA 分析的条件。使用光电二极管对特定抗体-抗原分子识别的顺序比色或化学发光检测进行定量检测。检测到的初级抗体表面密度低至 0.182 pmol cm(-2)。使用不同微点样的初级抗体进行了多重检测。

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