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表面生物钝化一次性聚二甲基硅氧烷/玻璃芯片在含内标的异质竞争性人血清免疫球蛋白G免疫分析中的应用。

Application of surface biopassivated disposable poly(dimethylsiloxane)/glass chips to a heterogeneous competitive human serum immunoglobulin G immunoassay with incorporated internal standard.

作者信息

Linder Vincent, Verpoorte Elisabeth, de Rooij Nico F, Sigrist Hans, Thormann Wolfgang

机构信息

Centre Suisse d'Electronique et de Microtechnique (CSEM), Neuchâtel, Switzerland.

出版信息

Electrophoresis. 2002 Mar;23(5):740-9. doi: 10.1002/1522-2683(200203)23:5<740::AID-ELPS740>3.0.CO;2-7.

DOI:10.1002/1522-2683(200203)23:5<740::AID-ELPS740>3.0.CO;2-7
PMID:11891707
Abstract

A microfluidic platform for a heterogeneous competitive immunoassay of human immunoglobulin G (IgG) employing Cy5-human IgG as tracer and Cy3-mouse IgG as internal standard was developed. The device consisted of microchannels made of poly(dimethylsiloxane) and glass which were patterned with antibodies against human IgG and mouse IgG. Electrokinetic sample transport was employed in order to exploit the small difference between the net mobilities of analyte and tracer, thereby achieving favorable conditions for the performance of the competitive immunoreaction. The overall quality of the disposable chip and performance of the immunoassay were controlled by monitoring the fluorescence of bound tracer and bound internal standard. Analyses with an insufficient internal standard response were discarded, and immunoassay data evaluation was based on the ratio of tracer and internal standard fluorescence. Using synthetic samples in the range from 0 to 80 microg/mL IgG and alkaline running conditions, a concentration-dependent response with reproducible Cy5/Cy3 signal ratios (average relative standard deviation of 6.8%) was obtained. Chips stored with solution in the channels at 4 degrees C over a two-month period were found to perform like freshly prepared chips, whereas chips stored dry at -20 degrees C and rehydrated prior to use could not be employed. The analysis of patient sera showed that the immunoassay platform behaved differently in the presence of serum-based samples. Using the same conditions as for the synthetic samples, no concentration dependence was noted. With a large excess of tracer, however, an IgG concentration dependence was observed, permitting distinction of samples of patients with normal IgG serum levels (8-16 mg/mL) from those with elevated IgG concentrations (>16 mg/mL).

摘要

开发了一种用于人免疫球蛋白G(IgG)异质竞争免疫分析的微流控平台,该平台采用Cy5标记的人IgG作为示踪剂,Cy3标记的小鼠IgG作为内标。该装置由聚二甲基硅氧烷和玻璃制成的微通道组成,这些微通道上印有抗人IgG和抗小鼠IgG的抗体。采用电动样品传输方式,以利用分析物和示踪剂净迁移率之间的微小差异,从而为竞争免疫反应的进行创造有利条件。通过监测结合示踪剂和结合内标的荧光来控制一次性芯片的整体质量和免疫分析的性能。舍弃内标响应不足的分析结果,免疫分析数据评估基于示踪剂和内标荧光的比值。在0至80μg/mL IgG范围内使用合成样品并采用碱性运行条件,获得了浓度依赖性响应,Cy5/Cy3信号比值具有可重复性(平均相对标准偏差为6.8%)。发现将芯片在4℃下于通道中储存溶液两个月后,其性能与新制备的芯片相同,而在-20℃下干燥储存并在使用前重新水化的芯片则无法使用。对患者血清的分析表明,在基于血清的样品存在下,免疫分析平台的表现有所不同。在与合成样品相同的条件下,未观察到浓度依赖性。然而,在示踪剂大量过量的情况下,观察到了IgG浓度依赖性,从而能够区分IgG血清水平正常(8 - 16mg/mL)的患者样本和IgG浓度升高(>16mg/mL)的患者样本。

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