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抗电负性 LDL 自身抗体和免疫复合物免疫测定法的建立。

Development of immunoassays for anti-electronegative LDL autoantibodies and immune complexes.

机构信息

Faculty of Pharmaceutical Sciences, University of Sao Paulo, São Paulo, SP, Brazil.

出版信息

Clin Chim Acta. 2012 Jan 18;413(1-2):291-7. doi: 10.1016/j.cca.2011.10.004. Epub 2011 Oct 18.

DOI:10.1016/j.cca.2011.10.004
PMID:22037508
Abstract

BACKGROUND

Electronegative low-density lipoprotein (LDL-) promotes atherosclerosis through inflammatory and immunologic mechanisms that lead to the production of anti-LDL(-) autoantibodies and to the subsequent formation of immune complexes (IC) and macrophage foam cells. We described the development and validation of an ELISA for the quantification of free anti-LDL(-) autoantibodies and an ELISA for the quantification of IC consisting of LDL(-)-bound IgG in human plasma.

METHODS

LDL(-) purified from human plasma, and anti-LDL(-) monoclonal antibody Fab fragments were adsorbed onto ELISA plates to capture anti-LDL(-) autoantibodies and IC-LDL(-), respectively. The performance characteristics of both ELISAs, including the limits of detection and quantification, accuracy and inter- and intra-assay precision were evaluated. Linearity, interference and stability tests were also performed.

RESULTS

The calibration range of the anti-LDL(-) assay was 0.004-0.125 mU/l and plasma demonstrated a dilutional linearity when diluted 1:100, 1:200, 1:400 and 1:800. The calibration range of the IC-LDL(-) assay was 0.06-4 U/l, and plasma demonstrated a dilutional linearity when diluted 1:12.5, 1:25, 1:50 and 1:100. Both ELISAs showed intra- and inter-assay precision and recovery within the required limits for immunoassays.

CONCLUSION

These ELISAs can be used in clinical studies and for the biochemical investigation of atherosclerosis. In addition, they will enable the comprehensive evaluation of the importance of bound or free autoantibodies against LDL(-) in this disease.

摘要

背景

通过导致抗 LDL(-) 自身抗体产生的炎症和免疫机制,电负性低密度脂蛋白(LDL-)促进动脉粥样硬化的形成,并随后形成免疫复合物(IC)和巨噬细胞泡沫细胞。我们描述了一种用于定量检测人血浆中游离抗 LDL(-) 自身抗体的 ELISA 以及一种用于定量检测 LDL(-) 结合 IgG 形成的 IC-LDL(-) 的 ELISA 的开发和验证。

方法

从人血浆中纯化 LDL(-),并将抗 LDL(-) 单克隆抗体 Fab 片段吸附到 ELISA 板上,分别捕获抗 LDL(-) 自身抗体和 IC-LDL(-)。评估了两种 ELISA 的性能特征,包括检测限和定量限、准确性以及批内和批间精密度。还进行了线性、干扰和稳定性测试。

结果

抗 LDL(-) 测定的校准范围为 0.004-0.125 mU/l,当以 1:100、1:200、1:400 和 1:800 稀释时,血浆显示出稀释线性。IC-LDL(-) 测定的校准范围为 0.06-4 U/l,当以 1:12.5、1:25、1:50 和 1:100 稀释时,血浆显示出稀释线性。两种 ELISA 均显示出批内和批间精密度以及回收率在免疫测定要求的范围内。

结论

这些 ELISA 可用于临床研究和动脉粥样硬化的生化研究。此外,它们将能够全面评估在这种疾病中结合或游离抗 LDL(-) 自身抗体的重要性。

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