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通过DNA定向固定实现有利的抗体微阵列制备:迈向细胞外囊泡在诊断中应用的一步。

Advantageous antibody microarray fabrication through DNA-directed immobilization: A step toward use of extracellular vesicles in diagnostics.

作者信息

Brambilla Dario, Sola Laura, Chiari Marcella

机构信息

Institute of Chemical Science and Technology, National Research Council of Italy (CNR-SCITEC), Milan, Italy.

Institute of Chemical Science and Technology, National Research Council of Italy (CNR-SCITEC), Milan, Italy.

出版信息

Talanta. 2021 Jan 15;222:121542. doi: 10.1016/j.talanta.2020.121542. Epub 2020 Aug 15.

DOI:10.1016/j.talanta.2020.121542
PMID:33167250
Abstract

Microarrays were introduced to run multiple assays on a single platform. Since then, researchers developed DNA and protein microarrays to study both transcription and expression of genes. Protein microarray technology represents a powerful tool to get an insight into living systems. However, despite their enormous potential, the fabrication of protein arrays is affected by technological hurdles that limit their application. One of the significant challenges is the immobilization of proteins on solid surfaces. To overcome this limitation, DNA-directed immobilization (DDI) of proteins, an approach that exploits DNA-protein conjugates to transform DNA microarrays into a protein array, has been developed. The adoption of DDI is limited, as this approach requires the synthesis of DNA-protein conjugates. Herein, we introduce an optimized general protocol for DNA-protein ligation, and demonstrate the use of conjugates to convert DNA arrays into antibody microarrays. Arrays obtained through DDI were used to capture and characterize extracellular vesicles (EVs), an emerging class of biomarkers. The proposed platform was tested against commercially available antibody microarrays, showing good performance combined with ease of fabrication.

摘要

微阵列被引入以在单个平台上进行多种检测。从那时起,研究人员开发了DNA和蛋白质微阵列来研究基因的转录和表达。蛋白质微阵列技术是深入了解生命系统的有力工具。然而,尽管它们具有巨大潜力,但蛋白质阵列的制造受到限制其应用的技术障碍的影响。一个重大挑战是蛋白质在固体表面的固定。为了克服这一限制,已经开发了蛋白质的DNA定向固定(DDI),一种利用DNA-蛋白质缀合物将DNA微阵列转化为蛋白质阵列的方法。DDI的采用受到限制,因为这种方法需要合成DNA-蛋白质缀合物。在此,我们介绍了一种优化的DNA-蛋白质连接通用方案,并展示了使用缀合物将DNA阵列转化为抗体微阵列。通过DDI获得的阵列用于捕获和表征细胞外囊泡(EV),这是一类新兴的生物标志物。所提出的平台与市售抗体微阵列进行了测试,显示出良好的性能且易于制造。

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