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基于可切换镧系元素发光的心肌肌钙蛋白 I 的快速均相免疫分析

Rapid homogeneous immunoassay for cardiac troponin I using switchable lanthanide luminescence.

机构信息

Department of Biochemistry/Biotechnology, Tykistökatu 6A, 6th Floor, FI-20520 Turku, Finland.

出版信息

Biosens Bioelectron. 2014 Dec 15;62:201-7. doi: 10.1016/j.bios.2014.06.042. Epub 2014 Jun 25.

Abstract

Homogeneous assays are advantageous because of their simplicity and rapid kinetics but typically their performance is severely compromised compared to heterogeneous assay formats. Here, we report a homogeneous immunoassay utilizing switchable lanthanide luminescence for detection and site-specifically labeled recombinant antibody fragments as binders to improve the assay performance. Switchable lanthanide luminescence enabled elimination of assay background due to division of the luminescent lanthanide chelate into two non-luminescent label moieties. Simultaneous biomolecular recognition of model analyte cardiac troponin I by two antibody fragments brought the label moieties together and resulted in self-assembly of luminescent mixed chelate complex. The assay was very rapid as maximal signal-to-background ratios were achieved already after 6 min of incubation. Additionally, the limit of detection was 0.38 ng/mL (16 pM), which was comparable to the limit of detection for the heterogeneous reference assay based on the same binders (0.26 ng/mL or 11 pM). This is the first study to apply switchable lanthanide luminescence in immunoassays and demonstrates the versatile potential of the technology for rapid and sensitive homogeneous assays.

摘要

均相测定法具有简单、快速动力学的优点,但与异质测定格式相比,其性能通常严重受损。在这里,我们报告了一种利用可切换镧系元素发光进行检测的均相免疫测定法,并使用特异性标记的重组抗体片段作为结合物来提高测定性能。可切换的镧系元素发光使由于将发光镧系元素螯合物分成两个非发光标记部分而消除了测定背景。两个抗体片段同时对模型分析物心肌肌钙蛋白 I 的生物分子识别使标记部分聚集在一起,并导致发光混合螯合物复合物的自组装。由于孵育 6 分钟后即可达到最大信号与背景比值,因此测定非常迅速。此外,检测限为 0.38ng/mL(16pM),与基于相同结合物的异质参考测定法(0.26ng/mL 或 11pM)的检测限相当。这是首次将可切换镧系元素发光应用于免疫测定法的研究,并证明了该技术在快速灵敏的均相测定法中的多功能潜力。

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