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可溶性细胞因子受体-免疫球蛋白融合蛋白的表达及配体结合分析

Expression and ligand binding assays of soluble cytokine receptor-immunoglobulin fusion proteins.

作者信息

Brown S J, Becherer K A, Blumeyer K, Kautzer C, Axelrod F, Le H, McConnell S J, Whalley A, Spinella D G

机构信息

Chugai Biopharmaceuticals, Inc., 6275 Nancy Ridge Drive, San Diego, California, 92121, USA.

出版信息

Protein Expr Purif. 1998 Oct;14(1):120-4. doi: 10.1006/prep.1998.0940.

Abstract

We have developed a cloning vector for the expression of type I cytokine receptor, NO, extracellular domain (ECD)-mouse IgG1 Fc fusion proteins. The vector has a versatile polylinker that allows in-frame cloning of the receptor ECD with the mouse IgG1 sequence to encode a receptor ECD-IgG1 fusion construct. The receptor-IgG1 fusion proteins are transiently expressed in useful amounts following transfection of the expression vector into COS7 cells and G418 selection. The mouse IgG1 portion of the fusion protein provides a universal handle for purification on an affinity matrix and detection by anti-mouse IgG antibodies in ELISA or Western blot formats. The expressed receptor ECD-IgG1 fusion proteins bind their cognate ligands. In order to demonstrate that the fusion proteins have similar ligand binding affinities as the native receptors, the affinity constants (Kd) for EPOR, TNFR, IL-4R, and IL-6R-IgG1 fusion proteins were measured by surface plasmon resonance and shown to be in good agreement with published values. The TNFR-IgG1 fusion protein was employed in a demonstration of a novel ELISA format for detecting cytokine receptor binding to cytokine.

摘要

我们开发了一种用于表达I型细胞因子受体、一氧化氮(NO)、细胞外结构域(ECD)-小鼠IgG1 Fc融合蛋白的克隆载体。该载体有一个通用的多克隆位点,允许将受体ECD与小鼠IgG1序列进行读码框内克隆,以编码受体ECD-IgG1融合构建体。将表达载体转染到COS7细胞并进行G418筛选后,受体-IgG1融合蛋白能以有用的量瞬时表达。融合蛋白的小鼠IgG1部分为在亲和基质上纯化以及通过ELISA或Western blot形式用抗小鼠IgG抗体进行检测提供了通用手段。表达的受体ECD-IgG1融合蛋白能结合其同源配体。为了证明融合蛋白与天然受体具有相似的配体结合亲和力,通过表面等离子体共振测量了EPOR、TNFR、IL-4R和IL-6R-IgG1融合蛋白的亲和常数(Kd),结果显示与已发表的值高度一致。TNFR-IgG1融合蛋白被用于一种新型ELISA形式的验证,该形式用于检测细胞因子受体与细胞因子的结合。

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