Preparation and Characterization of C-Reactive Protein Dual-Particle Latex-Enhanced Immunoturbidimetric Reagents.

IF 7.7 Q1 ENGINEERING, BIOMEDICAL BME frontiers Pub Date : 2024-12-23 eCollection Date: 2024-01-01 DOI:10.34133/bmef.0085
Yanyan Liu, Meijiao Li, Hao Zhang, Le Gao, Jitao Liu, Xuetong Zhu, Chenzhong Li, Shan Liu, Yue Hou, Jiancheng Xu
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Abstract

Objective and Impact Statement: This study aims to couple C-reactive protein (CRP) antibodies onto latex spheres of 2 different sizes to enhance the accuracy and sensitivity of CRP detection. Furthermore, it seeks to establish a robust methodological framework crucial for advancing the development of latex-enhanced immunoturbidimetric detection reagents. Introduction: CRP, an acute-phase protein, rapidly elevates in response to infections or tissue damage. Double-particle latex-enhanced immunoturbidimetry offers important advantages for accurately measuring CRP levels. Methods: CRP antibodies were coupled with 2 sizes of polystyrene latex spheres. Coupling rates were evaluated to determine optimal conditions. Particle sizes suitable for CRP detection, as well as coupling and mixing ratios, were optimized using automated biochemical analysis. Transmission electron microscopy and nanoparticle size analysis were employed to characterize the morphology and size changes of CRP antibodies and coupled latex spheres before and after immune reaction. Results: Optimization identified 168- and 80-nm latex sphere sizes, with CRP antibody coupling rates of 92% and 91%, respectively. The optimal ratios were 10:1.5 for large latex spheres to polyclonal antibodies and 5:1.5 for small latex spheres to monoclonal antibodies. A 1:8 mixing ratio of large to small latex spheres was effective. Transmission electron microscopy confirmed uniform sizes postcoupling, maintaining dispersion with no morphological changes. CRP reacted with the double-particle latex reagent, forming immune complexes that exhibited agglutination. Mixed latex spheres showed varied agglutination states with CRP concentration, altering solution absorbance. Conclusion: This study validates the efficacy of the dual-particle-size CRP antibody latex reagent, highlighting its potential for future immunoturbidimetric analysis applications.

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c -反应蛋白双颗粒乳胶增强免疫比浊试剂的制备与表征。
目的及影响声明:本研究旨在将c -反应蛋白(CRP)抗体偶联到两种不同大小的乳胶球上,以提高CRP检测的准确性和灵敏度。此外,它寻求建立一个强大的方法框架,对推进乳胶增强免疫比浊检测试剂的发展至关重要。CRP是一种急性期蛋白,在感染或组织损伤时迅速升高。双颗粒乳胶增强免疫比浊法为准确测量CRP水平提供了重要的优势。方法:CRP抗体与2种尺寸的聚苯乙烯乳胶球偶联。评估耦合率以确定最佳条件。采用自动化生化分析优化了适合CRP检测的粒径、耦合和混合比例。采用透射电镜和纳米颗粒大小分析表征免疫反应前后CRP抗体和偶联乳胶球的形态和大小变化。结果:优化后鉴定出粒径为168 nm和80 nm的乳胶球,CRP抗体偶联率分别为92%和91%。大乳胶球与多克隆抗体的最佳比例为10:1.5,小乳胶球与单克隆抗体的最佳比例为5:1.5。大小乳胶球的混合比例为1:8。透射电镜证实尺寸均匀后耦合,保持分散性,无形态改变。CRP与双颗粒乳胶试剂反应,形成具有凝集作用的免疫复合物。混合乳胶球随着CRP浓度的变化呈现出不同的凝集状态,从而改变溶液的吸光度。结论:本研究验证了双粒径CRP抗体乳胶试剂的有效性,强调了其在未来免疫比浊分析中的应用潜力。
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N-hydroxysuccinimide (NHS)
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1-Ethyl-(3-dimethylaminopropyl) carbodiimide hydrochloride (EDC·HCl)
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1-Ethyl-(3-dimethylaminopropyl) carbodiimide hydrochloride (EDC·HCl)
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N-hydroxysuccinimide (NHS)
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1-Ethyl-(3-dimethylaminopropyl) carbodiimide hydrochloride (EDC·HCl)
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7.10
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审稿时长
16 weeks
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