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多重单分子免疫分析。

Multiplexed single molecule immunoassays.

机构信息

Quanterix Corporation, 113 Hartwell Avenue, Lexington, MA 02421, USA.

出版信息

Lab Chip. 2013 Aug 7;13(15):2902-11. doi: 10.1039/c3lc50416f.

DOI:10.1039/c3lc50416f
PMID:23719780
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10540087/
Abstract

We have developed a method that enables the multiplexed detection of proteins based on counting single molecules. Paramagnetic beads were labeled with fluorescent dyes to create optically distinct subpopulations of beads, and antibodies to specific proteins were then immobilized to individual subpopulations. Mixtures of subpopulations of beads were then incubated with a sample, and specific proteins were captured on their specific beads; these proteins were then labeled with enzymes via immunocomplex formation. The beads were suspended in enzyme substrate, loaded into arrays of femtoliter wells--or Single Molecule Arrays (Simoa)--that were integrated into a microfluidic device (the Simoa disc). The wells were then sealed with oil, and imaged fluorescently to determine: a) the location and subpopulation identity of individual beads in the femtoliter wells, and b) the presence or absence of a single enzyme associated with each bead. The images were analyzed to determine the average enzyme per bead (AEB) for each bead subpopulation that provide a quantitative parameter for determining the concentration of each protein. We used this approach to simultaneously detect TNF-α, IL-6, IL-1α, and IL-1β in human plasma with single molecule resolution at subfemtomolar concentrations, i.e., 200- to 1000-fold more sensitive than current multiplexed immunoassays. The simultaneous, specific, and sensitive measurement of several proteins using multiplexed digital ELISA could enable more reliable diagnoses of disease.

摘要

我们开发了一种基于单分子计数的多重蛋白检测方法。将顺磁珠用荧光染料标记,以创建具有明显光学区别的珠亚群,然后将针对特定蛋白的抗体固定到各个亚群上。随后,将珠亚群混合物与样品孵育,使特定蛋白与其特定珠群结合;这些蛋白随后通过免疫复合物形成被标记上酶。将珠悬浮在酶底物中,加载到集成到微流控装置(Simoa 盘)中的纳升级井(或单分子阵列(Simoa))阵列中。然后用油密封井,并进行荧光成像,以确定:a)纳升级井中单个珠的位置和亚群身份,以及 b)与每个珠相关联的单个酶的存在或不存在。对图像进行分析以确定每个珠亚群的平均酶量(AEB),为确定每种蛋白的浓度提供定量参数。我们使用这种方法以亚 femtomolar 浓度(即比当前多重免疫分析灵敏 200 到 1000 倍),以单分子分辨率同时检测人血浆中的 TNF-α、IL-6、IL-1α 和 IL-1β。使用多重数字 ELISA 进行的同时、特异和灵敏的多种蛋白测量可以实现更可靠的疾病诊断。

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