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抗促甲状腺激素受体抗体活性的放射受体测定:使用未提取血清和免疫球蛋白组分的测定方法比较及活性表达的标准化

Radioreceptor assay of anti-TSH receptor antibody activity: comparison of assays using unextracted serum and immunoglobulin fractions, and standardization of expression of activities.

作者信息

Tamaki H, Amino N, Watanabe Y, Aozasa M, Hayashi H, Tachi J, Miyai K

出版信息

J Clin Lab Immunol. 1986 May;20(1):1-6.

PMID:3016274
Abstract

A radioreceptor assay for TSH receptor antibodies developed by Shewring and Smith is described in which unextracted serum is used. The assay is simple and reproducible. TSH-binding inhibitor immunoglobulin (TBII) activity determined using unextracted serum correlated well with that determined using the immunoglobulin fraction purified with polyethylene glycol. The assay detected TSH receptor antibodies in 81 of 85 patients (95%) with untreated Graves' disease, no patients with Graves' disease in remission, and 7 of 57 patients (12%) with Hashimoto's disease. TSH-binding inhibitor activity of a human TSH preparation (Kabi Diagnostica) was not detectable at 100 mU/L, but detectable at 1,000 mU/L. Consistent with this, TBII activity was not detectable in hypothyroid patients with goitrous Hashimoto's disease, whose serum TSH concentrations were 11-520 mU/L. Of 57 patients with Hashimoto's disease positive TBII activity was detected in only 7 of 15 patients (46%) with primary atrophic hypothyroidism. Five of these had very high TBII activities (greater than 90% inhibition of labelled TSH binding), and no linear dose-response relationship was observed in dilution experiments. For exact determination of TBII activity in specimens with high activities, serum samples were diluted with normal pooled serum and activities were expressed in U/ml by comparison with values for standard serum, prepared from bovine TSH diluted with normal pooled serum. In this way, samples with TBII activities of 1-50 U/ml (20-90% inhibition of binding of labelled TSH) showed linear dose-response relations in dilution experiments, and the dilution curves of all samples examined were parallel to the standard curve. This standardization procedure was used in determining the half life of TBII.

摘要

本文描述了由谢林和史密斯开发的一种用于检测促甲状腺激素(TSH)受体抗体的放射受体分析法,该方法使用未提取的血清。该分析方法简单且可重复。使用未提取血清测定的TSH结合抑制免疫球蛋白(TBII)活性与使用聚乙二醇纯化的免疫球蛋白部分测定的活性相关性良好。该分析方法在85例未经治疗的格雷夫斯病患者中的81例(95%)检测到TSH受体抗体,在缓解期的格雷夫斯病患者中未检测到,在57例桥本氏病患者中的7例(12%)检测到。人TSH制剂(卡比诊断公司)在100 mU/L时未检测到TSH结合抑制活性,但在1000 mU/L时可检测到。与此一致的是,在甲状腺肿性桥本氏病的甲状腺功能减退患者中未检测到TBII活性,其血清TSH浓度为11 - 520 mU/L。在57例桥本氏病患者中,仅在15例原发性萎缩性甲状腺功能减退患者中的7例(46%)检测到阳性TBII活性。其中5例具有非常高的TBII活性(对标记TSH结合的抑制率大于90%),并且在稀释实验中未观察到线性剂量反应关系。为了准确测定高活性标本中的TBII活性,血清样本用正常混合血清稀释,并通过与用正常混合血清稀释的牛TSH制备的标准血清的值比较,以U/ml表示活性。通过这种方式,TBII活性为1 - 50 U/ml(对标记TSH结合的抑制率为20 - 90%)的样本在稀释实验中显示出线性剂量反应关系,并且所有检测样本的稀释曲线与标准曲线平行。该标准化程序用于测定TBII的半衰期。

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