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通过表面增强拉曼光谱和相似性分析进行蛋白质定量与成像

Protein Quantification and Imaging by Surface-Enhanced Raman Spectroscopy and Similarity Analysis.

作者信息

Shin Hyunku, Oh Seunghyun, Kang Daehyeon, Choi Yeonho

机构信息

Department of Bio-convergence Engineering Korea University Seoul 02841 Republic of Korea.

School of Biomedical Engineering Korea University Seoul 02841 Republic of Korea.

出版信息

Adv Sci (Weinh). 2020 Apr 16;7(11):1903638. doi: 10.1002/advs.201903638. eCollection 2020 Jun.

Abstract

Protein quantification techniques such as immunoassays have been improved considerably, but they have several limitations, including time-consuming procedures, low sensitivity, and extrinsic detection. Because direct surface-enhanced Raman spectroscopy (SERS) can detect intrinsic signals of proteins, it can be used as an effective detection method. However, owing to the complexity and reliability of SERS signals, SERS is rarely adopted for quantification without a purified target protein. This study reports an efficient and effective direct SERS-based immunoassay (SERSIA) technique for protein quantification and imaging. SERSIA relies on the uniform coating of gold nanoparticles (GNPs) on a target-protein-immobilized substrate by simple centrifugation. As centrifugation induces close contact between the GNPs and target proteins, the intrinsic signals of the target protein can be detected. For quantification, the protein levels in a cell lysate are estimated using similarity analysis between antibody-only and protein-conjugated samples. This method reliably estimates the protein level at a sub-picomolar detection limit. Furthermore, this method enables quantitative imaging of immobilized protein at a micrometer range. Because this technique is fast, sensitive, and requires only one type of antibody, this approach can be a useful method to detect proteins in biological samples.

摘要

免疫测定等蛋白质定量技术已得到显著改进,但仍存在一些局限性,包括操作耗时、灵敏度低以及外部检测等问题。由于直接表面增强拉曼光谱(SERS)能够检测蛋白质的固有信号,因此可作为一种有效的检测方法。然而,由于SERS信号的复杂性和可靠性,在没有纯化目标蛋白的情况下,SERS很少用于定量分析。本研究报告了一种高效且有效的基于直接SERS的免疫测定(SERSIA)技术,用于蛋白质定量和成像。SERSIA通过简单的离心操作,依赖于在固定有目标蛋白的底物上均匀包覆金纳米颗粒(GNP)。由于离心作用促使GNP与目标蛋白紧密接触,从而能够检测到目标蛋白的固有信号。对于定量分析,通过仅含抗体的样品与蛋白质缀合样品之间的相似性分析来估算细胞裂解液中的蛋白质水平。该方法能够在亚皮摩尔检测限可靠地估算蛋白质水平。此外,该方法能够在微米范围内对固定化蛋白质进行定量成像。由于该技术快速、灵敏且仅需一种抗体,因此这种方法可成为检测生物样品中蛋白质的有用手段。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/06c4/7284192/e250d6ea28b0/ADVS-7-1903638-g001.jpg

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