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用间接 ELISA 法测量静脉注射用免疫球蛋白中的抗 Abeta1-42 抗体:非特异性结合问题。

Measurement of anti-Abeta1-42 antibodies in intravenous immunoglobulin with indirect ELISA: the problem of nonspecific binding.

机构信息

Department of Neurology Research, William Beaumont Hospital Research Institute, 3811 West Thirteen Mile Road, Suite 507, Royal Oak, MI 48073, USA.

出版信息

J Neurosci Methods. 2010 Mar 30;187(2):263-9. doi: 10.1016/j.jneumeth.2010.01.018. Epub 2010 Jan 25.

Abstract

Improvement in cognitive scores in patients with Alzheimer's disease (AD) has been reported in two trials in which intravenous immunoglobulin (IvIg) preparations were administered. IvIg's benefits in AD patients have been suggested to be due to antibodies to amyloid-beta (Abeta). Our previous study using indirect enzyme-linked immunosorbent assay (ELISA) indicated that much of IvIg's apparent binding to Abeta1-42 is nonspecific; it is detectable even when IvIg is incubated on "specificity controls" (bovine serum albumin [BSA] and Abeta reverse sequence Abeta42-1) rather than Abeta1-42. The objective of this study was to evaluate procedures that might reduce this nonspecific binding. The IvIg preparation used was Gamunex (Talecris Biotherapeutics). Multiple blocking agents were evaluated, but even the most effective blocker only reduced nonspecific binding by 48%. Dissociating Gamunex's antibody-antigen complexes had no effect on specific binding when Abeta42-1 was used as the specificity control, although it increased this binding when BSA was the specificity control. Decreasing Gamunex's dilution from 1:1,500 to 1:500 resulted in a slight (7.4%) but significant (p=0.027) increase in specific binding. Using a sandwich ELISA to measure Gamunex's anti-Abeta antibodies resulted in even less specific binding to Abeta1-42 than with the indirect ELISA. Despite Gamunex's low percentage of specific binding to Abeta1-42, it inhibited Abeta oligomer formation. We conclude that, when anti-Abeta antibodies in IvIg are measured by indirect ELISA, extensive nonspecific binding occurs despite procedures taken to prevent it. This must be subtracted from total binding to accurately measure specific anti-Abeta antibody concentrations.

摘要

在两项静脉注射免疫球蛋白(IVIg)制剂治疗阿尔茨海默病(AD)患者的试验中,报道了认知评分的改善。AD 患者中 IvIg 的益处被认为是由于针对淀粉样蛋白-β(Abeta)的抗体。我们之前使用间接酶联免疫吸附试验(ELISA)的研究表明,IvIg 对 Abeta1-42 的大部分明显结合是非特异性的;即使 IvIg 在“特异性对照物”(牛血清白蛋白[BSA]和 Abeta 反向序列 Abeta42-1)而不是 Abeta1-42 上孵育,也可以检测到它。本研究的目的是评估可能减少这种非特异性结合的程序。使用的 IvIg 制剂是 Gamunex(Talecris Biotherapeutics)。评估了多种阻断剂,但即使是最有效的阻断剂也只能将非特异性结合减少 48%。当 Abeta42-1 用作特异性对照物时,解离 Gamunex 的抗体-抗原复合物对特异性结合没有影响,尽管当 BSA 用作特异性对照物时,它增加了这种结合。将 Gamunex 的稀释度从 1:1500 降低至 1:500 导致特异性结合略有增加(7.4%),但具有统计学意义(p=0.027)。使用夹心 ELISA 测量 Gamunex 的抗 Abeta 抗体导致与间接 ELISA 相比,对 Abeta1-42 的特异性结合更少。尽管 Gamunex 对 Abeta1-42 的特异性结合百分比较低,但它抑制了 Abeta 寡聚物的形成。我们得出结论,当通过间接 ELISA 测量 IvIg 中的抗 Abeta 抗体时,尽管采取了防止非特异性结合的措施,但仍会发生广泛的非特异性结合。必须从总结合中减去该值,以准确测量特异性抗 Abeta 抗体浓度。

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