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甲状腺抗体检测的分析方面

Analytical aspects of thyroid antibodies estimation.

作者信息

Sinclair David

机构信息

Department of Clinical Biochemistry, Queen Alexandra Hospital, Portsmouth, UK.

出版信息

Autoimmunity. 2008 Feb;41(1):46-54. doi: 10.1080/08916930701619466.

DOI:10.1080/08916930701619466
PMID:18176864
Abstract

The search for antibodies that will reliably diagnose, predict and monitor the autoimmune thyroid diseases is a quest that is beset with difficulties. This review will describe the various antigens involved in autoimmune thyroid disease, the development of a humoral response to these antigens and some of the technical difficulties involved in trying to detect and then measure their concentrations. Multiple antigen configurations of thyroglobulin (TG) are produced when it is iodinated resulting in functionally active but immunologically distinct molecules. Thyroid peroxidase (TPO), originally described as thyroid microsomal antigen, is present on the apical surface of thyroid follicular cells and is the antigen most closely involved in cell-mediated cytotoxicity. Multiple B cell reactive epitopes exist each giving rise to different antibodies. The third antigen is the TSH receptor (TSHR) which is a two subunit glycoprotein. The extracellular A subunit is recognised by thyroid stimulating antibodies whilst those antibodies recognising the B subunit, located much nearer the cell surface, appear to function as blocking antibodies. The aetiology and mechanics of the autoimmune cellular and antibody responses involves a combination of HLA linkage, genetics and environmental factors to determine the initial and subsequent stages of the development of autoimmune thyroid disease. Starting off with immunofluorescence or passive tanned red cell agglutination assays, we now favour more sensitive TPO antibody quantitative immunoassays which are standardised using MRC 66/387. The apparent incidence of these antibodies is influenced by the techniques used to detect them and the significance of those positive antibody concentrations detected using assays that report very high incidence rates in the "normal" population remains to be proven using longitudinal studies. Older immunofluorescence and passive tanned red cell agglutination methods have been improved upon to give the current, competitive and non-competitive immunoassays that are much more sensitive and specific for anti-TG antibodies. However, because a wide-range of methods are still being used in clinical laboratories, the sensitivity and specificity of available methods will vary depending on the method used. There are still assays that are calibrated with purified or crude preparations of TG antibody by pooling patient sera or blood donor material. These various secondary standards are often, but not always, calibrated against the primary standard (MRC 65/93). All requests for TG estimation in thyroid carcinoma patients should have TG antibody estimated at the same time because of the possibility of interference in the tumour marker assay by the antibody. Two methods are widely used for the estimation of TSHR antibodies. The first involves bioassays based on cultured cells to measure the stimulating class of antibodies and the second involves receptor assays based on (125)I-labeled TSH. The most widely used assay uses detergent-solubilized porcine TSHR with TSHR antibodies to inhibit the TSHR-(125)I-TSH interaction, and polyethylene glycol to separate receptor-bound and free labelled-TSH by precipitation. TSHR antibody heterogeneity can coexist within an individual patient and change over time is one reason why it has been difficult to develop diagnostically accurate TSHR antibody tests.

摘要

寻找能够可靠诊断、预测和监测自身免疫性甲状腺疾病的抗体是一项充满困难的探索。本综述将描述自身免疫性甲状腺疾病中涉及的各种抗原、针对这些抗原的体液免疫反应的发展以及在试图检测并测量其浓度时所涉及的一些技术难题。甲状腺球蛋白(TG)碘化时会产生多种抗原构型,从而形成功能活跃但免疫特性不同的分子。甲状腺过氧化物酶(TPO)最初被描述为甲状腺微粒体抗原,存在于甲状腺滤泡细胞的顶端表面,是最密切参与细胞介导的细胞毒性的抗原。存在多个B细胞反应性表位,每个表位都会产生不同的抗体。第三种抗原是促甲状腺激素受体(TSHR),它是一种双亚基糖蛋白。细胞外A亚基可被促甲状腺激素刺激抗体识别,而那些识别位于更靠近细胞表面的B亚基的抗体似乎起阻断抗体的作用。自身免疫性细胞和抗体反应的病因及机制涉及HLA连锁、遗传和环境因素的综合作用,以确定自身免疫性甲状腺疾病发展的初始和后续阶段。从免疫荧光或被动鞣酸红细胞凝集试验开始,我们现在更倾向于使用更敏感的TPO抗体定量免疫测定法,这些方法使用MRC 66/387进行标准化。这些抗体的表观发病率受检测技术的影响,而使用在“正常”人群中报告非常高发病率的检测方法检测到的那些阳性抗体浓度的意义,仍有待通过纵向研究来证实。较旧的免疫荧光和被动鞣酸红细胞凝集方法已得到改进,形成了目前具有竞争力的非竞争性免疫测定法,这些方法对抗TG抗体更敏感、更特异。然而,由于临床实验室仍在使用多种方法,现有方法的敏感性和特异性将因所使用的方法而异。仍有一些检测方法是通过汇集患者血清或献血者材料,用纯化或粗制的TG抗体制剂进行校准的。这些各种二级标准通常(但并非总是)相对于一级标准(MRC 65/93)进行校准。由于抗体可能干扰甲状腺癌患者肿瘤标志物检测,因此所有甲状腺癌患者的TG估计请求都应同时估计TG抗体。两种方法广泛用于估计TSHR抗体。第一种方法涉及基于培养细胞的生物测定法,以测量刺激性抗体类别,第二种方法涉及基于(125)I标记促甲状腺激素的受体测定法。最广泛使用的检测方法是使用去污剂溶解的猪TSHR与TSHR抗体来抑制TSHR-(125)I-促甲状腺激素相互作用,并使用聚乙二醇通过沉淀分离受体结合的和游离的标记促甲状腺激素。TSHR抗体异质性可在个体患者中共存并随时间变化,这是难以开发诊断准确的TSHR抗体检测方法的一个原因。

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