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通过毛细管等电聚焦法对蛋白质及其异构体进行高灵敏度定量检测

Highly Sensitive and Quantitative Detection of Proteins and Their Isoforms by Capillary Isoelectric Focusing Method.

作者信息

Padhan Narendra

机构信息

Uppsala University, Dept. Immunology, Genetics and Pathology, Rudbeck Laboratory, 751 85, Uppsala, Sweden;

出版信息

J Vis Exp. 2018 Sep 19(139):56794. doi: 10.3791/56794.

DOI:10.3791/56794
PMID:30295655
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6235248/
Abstract

Immunoblotting has become a routine technique in many laboratories for protein characterization from biological samples. The following protocol provides an alternative strategy, capillary isoelectric focusing (cIEF), with many advantages compared to conventional immunoblotting. This is an antibody-based, automated, rapid, and quantitative method in which a complete western blotting procedure takes place inside an ultrathin capillary. This technique does not require a gel to transfer to a membrane, stripping of blots, or x-ray films, which are typically required for conventional immunoblotting. Here, proteins are separated according to their charge (isoelectric point; pI), using less than a microliter (400 nL) of total protein lysate. After electrophoresis, proteins are immobilized onto the capillary walls by ultraviolet light treatment, followed by primary and secondary (horseradish peroxidase (HRP) conjugated) antibody incubation, whose binding is detected through enhanced chemiluminescence (ECL), generating a light signal that can be captured and recorded by a charge-coupled device (CCD) camera. The digital image can be analyzed and quantified (peak area) using software. This high throughput procedure can handle 96 samples at a time; is highly sensitive, with protein detection in the picogram range; and produces highly reproducible results because of automation. All of these aspects are extremely valuable when the quantity of samples (e.g., tissue samples and biopsies) is a limiting factor. The technique has wider applications as well, including screening of drugs or antibodies, biomarker discovery, and diagnostic purposes.

摘要

免疫印迹已成为许多实验室用于从生物样品中鉴定蛋白质的常规技术。以下方案提供了一种替代策略——毛细管等电聚焦(cIEF),与传统免疫印迹相比具有许多优势。这是一种基于抗体的、自动化、快速且定量的方法,其中完整的蛋白质印迹程序在超薄毛细管内进行。该技术不需要将凝胶转移到膜上、剥离印迹或使用传统免疫印迹通常所需的X光片。在这里,使用不到一微升(400纳升)的总蛋白裂解物,根据蛋白质的电荷(等电点;pI)对其进行分离。电泳后,通过紫外线处理将蛋白质固定在毛细管壁上,然后进行一抗和二抗(辣根过氧化物酶(HRP)偶联)孵育,通过增强化学发光(ECL)检测其结合情况,产生一个可被电荷耦合器件(CCD)相机捕获和记录的光信号。可以使用软件对数字图像进行分析和定量(峰面积)。这种高通量程序一次可以处理96个样品;灵敏度高,可检测皮克级别的蛋白质;并且由于自动化而产生高度可重复的结果。当样品量(例如组织样品和活检样本)是限制因素时,所有这些方面都极具价值。该技术还有更广泛的应用,包括药物或抗体筛选、生物标志物发现以及诊断用途。