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蛋白质复合物的固相制备。

Solid-phase preparation of protein complexes.

机构信息

Xeptagen SpA, Via delle Industrie 9, Marghera-Venezia I-30175, Italy.

出版信息

J Mol Recognit. 2010 Nov-Dec;23(6):551-8. doi: 10.1002/jmr.1095.

DOI:10.1002/jmr.1095
PMID:21038355
Abstract

Protein-protein conjugation is usually achieved by solution phase methods requiring concentrated protein solution and post-synthetic purification steps. In this report we describe a novel continuous-flow solid-phase approach enabling the assembly of protein complexes minimizing the amount of material needed and allowing the repeated use of the same solid phase. The method exploits an immunoaffinity matrix as solid support; the matrix reversibly binds the first of the complex components while the other components are sequentially introduced, thus allowing the complex to grow while immobilized. The tethering technique employed relies on the use of the very mild synthetic conditions and fast association rates allowed by the avidin-biotin system. At the end of the assembly, the immobilized complexes can be removed from the solid support and recovered by lowering the pH of the medium. Under the conditions used for the sequential complexation and recovery, the solid phase was not damaged or irreversibly modified and could be reused without loss of binding capacity. The method was specifically designed to prepare protein complexes to be used in immunometric methods of analysis, where the immunoreactivity of each component needs to be preserved. The approach was successfully exploited for the preparation of two different immunoaffinity reagents with immunoreactivity mimicking native squamous cell carcinoma antigen-immunoglobulin M (SCCA-IgM) and alphafetoprotein-immunoglobulin M (AFP-IgM) immune complexes, which were characterized by dedicated sandwich enzyme-linked immunosorbent assay (ELISA) and immunoblot. Besides the specific application described in the paper, the method is sufficiently general to be used for the preparation of a broad range of protein assemblies.

摘要

蛋白质-蛋白质偶联通常通过溶液相方法实现,需要浓缩的蛋白质溶液和合成后的纯化步骤。在本报告中,我们描述了一种新颖的连续流固相方法,可最小化所需材料的量并允许重复使用相同的固相,从而实现蛋白质复合物的组装。该方法利用免疫亲和基质作为固相支持物;基质可逆地结合复合物的第一个成分,而其他成分则依次引入,从而允许复合物在固定化的同时生长。所采用的连接技术依赖于使用非常温和的合成条件和亲和素-生物素系统允许的快速缔合速率。在组装结束时,通过降低介质的 pH 值,可以将固定化的复合物从固相上洗脱下来并回收。在用于顺序络合和回收的条件下,固相没有损坏或不可逆修饰,可以重复使用而不会损失结合能力。该方法是专门为制备用于免疫分析的蛋白质复合物而设计的,其中每个成分的免疫反应性需要保留。该方法成功地用于制备两种不同的免疫亲和试剂,其免疫反应性模拟天然鳞状细胞癌抗原-免疫球蛋白 M(SCCA-IgM)和甲胎蛋白-免疫球蛋白 M(AFP-IgM)免疫复合物,通过专用的夹心酶联免疫吸附测定(ELISA)和免疫印迹进行了表征。除了本文中描述的特定应用外,该方法足够通用,可以用于制备广泛的蛋白质组装物。

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1
Solid-phase preparation of protein complexes.蛋白质复合物的固相制备。
J Mol Recognit. 2010 Nov-Dec;23(6):551-8. doi: 10.1002/jmr.1095.
2
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Monitoring SCCA-IgM complexes in serum predicts liver disease progression in patients with chronic hepatitis.监测血清中的鳞状细胞癌抗原免疫球蛋白M复合物可预测慢性肝炎患者的肝病进展。
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Interaction proteomics: characterization of protein complexes using tandem affinity purification-mass spectrometry.相互作用蛋白质组学:使用串联亲和纯化-质谱法对蛋白质复合物进行表征。
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Biotin IgM antibodies in human blood: a previously unknown factor eliciting false results in biotinylation-based immunoassays.
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