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基质对唾液睾酮竞争性酶免疫测定中抗原固定化形式的影响。

Matrix effects on an antigen immobilized format for competitive enzyme immunoassay of salivary testosterone.

作者信息

Mitchell John S, Lowe Tim E

机构信息

Health and Food Group, The New Zealand Institute For Plant & Food Research Limited, Private Bag 3123, Hamilton, New Zealand.

出版信息

J Immunol Methods. 2009 Sep 30;349(1-2):61-6. doi: 10.1016/j.jim.2009.07.012. Epub 2009 Aug 4.

DOI:10.1016/j.jim.2009.07.012
PMID:19660465
Abstract

Matrix interferences in salivary testosterone enzyme immunoassays are important in the development of direct ELISA. An alternative format for sensitive enzyme immunoassay of testosterone was developed using immobilization of the antigen as part of a protein conjugate using oligoethylene glycol linker to project the antigen, with color development via enzyme labeled secondary antibody. This technique gave the required sensitivity for detection of testosterone from male saliva with a limit of detection (LOD) of 8.9 pg/mL (31 pmol/L). Application of the immunoassay directly in human saliva gave suppression of binding signals for the samples, indicating clear matrix interference with antibody binding. A wide variety of treatments were used in an attempt to overcome this effect, including use of both synthetic saliva and stripped human saliva for standard preparation, use of bovine serum albumin (BSA) to reduce non-specific binding of contaminants, pH adjustment of samples and/or standards and use of different antibodies. None of these techniques proved effective, causing either substantial suppression or enhancement of signal, and dilution was not possible because of the very low physiological concentrations. Complete removal of the saliva medium by chemical extraction was the only technique studied that could overcome this problem. These issues have not been explored previously for direct ELISA of salivary testosterone using alternative assay formats and have implications for the design of small molecule plate-based immunoassays in this medium.

摘要

唾液睾酮酶免疫测定中的基质干扰在直接酶联免疫吸附测定(ELISA)的发展中很重要。开发了一种用于睾酮灵敏酶免疫测定的替代形式,该方法利用低聚乙二醇连接子将抗原作为蛋白质偶联物的一部分进行固定,以使抗原突出,并通过酶标记的二抗进行显色。该技术对男性唾液中睾酮的检测具有所需的灵敏度,检测限(LOD)为8.9 pg/mL(31 pmol/L)。将免疫测定直接应用于人类唾液时,样品的结合信号受到抑制,表明存在明显的基质干扰抗体结合。为克服这种影响,尝试了多种处理方法,包括使用合成唾液和脱蛋白人唾液制备标准品、使用牛血清白蛋白(BSA)减少污染物的非特异性结合、调节样品和/或标准品的pH值以及使用不同的抗体。这些技术均未证明有效,要么导致信号大幅抑制,要么导致信号增强,而且由于生理浓度极低,无法进行稀释。通过化学萃取完全去除唾液介质是所研究的唯一能够克服此问题的技术。以前尚未使用替代测定形式对唾液睾酮的直接ELISA进行过此类研究,这些问题对该介质中小分子板基免疫测定的设计具有重要意义。

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