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一种与抑制剂高通量筛选兼容的人胰岛素样生长因子结合蛋白4闪烁邻近分析方法的开发。

Development of a scintillation proximity assay for human insulin-like growth factor-binding protein 4 compatible with inhibitor high-throughput screening.

作者信息

Khawaja X Z

机构信息

Neuroscience Discovery Research, Wyeth Research, Princeton, NJ 08543, USA.

出版信息

Anal Biochem. 2007 Jul 1;366(1):80-6. doi: 10.1016/j.ab.2007.03.011. Epub 2007 Mar 18.

DOI:10.1016/j.ab.2007.03.011
PMID:17482135
Abstract

The insulin-like growth factor-binding protein 4 (IGFBP-4), which exists in many different tissues and biological fluids, modulates insulin-like growth factor 1 (IGF-1) bioavailability in part by competitive sequestration and prevention of interaction with cell membrane IGF-1 receptors. Accordingly, small molecules that inhibit the ability of IGF-1 to associate with IGFBP-4 may have clinical utility as regulators of cellular proliferation, survival, and differentiation. Currently, a polyethylene glycol-based precipitation of [(125)I]IGF-1 bound to IGFBP-4 is used to quantify selective IGFBP-4 ligand interactions. We have developed a novel 96-well plate scintillation proximity assay (SPA) for measuring small molecule interactions at IGFBP-4 using a biotinylated form of IGFBP-4 coupled to streptavidin-coated polyvinyltoluene (PVT) SPA microbeads and using [(125)I]IGF-1 as the endogenous ligand. Dose-displacement curves with unlabeled IGF-1 exhibited a mean K(d) value of 0.46 nM. Parallel studies using the nonselective IGFBP inhibitor, NBI-31772, generated a K(i) value of 47 nM. Under optimized conditions, the IGFBP-4 SPA was stable for up to 24h at room temperature and was unaffected by dimethyl sulfoxide (DMSO,<0.5%). This homogeneous binding assay is simple, stable, sensitive, and amenable to automation. The good signal/noise ratio (10:1) and Z' factor (0.7-0.8) make it compatible with high-throughput screening platforms for the identification of IGFBP-4 inhibitors. The IGFBP-4 binding assay may be expanded to other IGFBP members, in biotinylated form, to provide a powerful tool amenable to drug screening and the design of therapeutics to treat a variety of IGF-responsive diseases.

摘要

胰岛素样生长因子结合蛋白4(IGFBP - 4)存在于许多不同组织和生物体液中,它部分通过竞争性隔离以及阻止胰岛素样生长因子1(IGF - 1)与细胞膜IGF - 1受体相互作用来调节IGF - 1的生物利用度。因此,抑制IGF - 1与IGFBP - 4结合能力的小分子可能作为细胞增殖、存活和分化的调节剂具有临床应用价值。目前,基于聚乙二醇沉淀法用于定量[(125)I]IGF - 1与IGFBP - 4的选择性配体相互作用。我们开发了一种新型的96孔板闪烁邻近分析法(SPA),用于测量小分子与IGFBP - 4的相互作用,该方法使用生物素化形式的IGFBP - 4偶联到链霉亲和素包被的聚对甲苯乙烯(PVT)SPA微珠上,并使用[(125)I]IGF - 1作为内源性配体。未标记IGF - 1的剂量置换曲线显示平均解离常数(K(d))值为0.46 nM。使用非选择性IGFBP抑制剂NBI - 31772进行的平行研究得出抑制常数(K(i))值为47 nM。在优化条件下,IGFBP - 4 SPA在室温下长达24小时稳定,且不受二甲基亚砜(DMSO,<0.5%)影响。这种均相结合分析方法简单、稳定、灵敏且适合自动化操作。良好的信噪比(10:1)和Z'因子(0.7 - 0.8)使其适用于高通量筛选平台以鉴定IGFBP - 4抑制剂。IGFBP - 4结合分析可扩展到其他生物素化形式的IGFBP成员,为药物筛选和治疗多种IGF反应性疾病的治疗药物设计提供有力工具。

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