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Novel Fluorescence Competition Assay for Retinoic Acid Binding Proteins

机译:用于视黄酸结合蛋白的新型荧光竞争测定

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Vitamin A derived retinoid compounds have multiple, powerful roles in the cellular growth and development cycle and, as a result, have attracted significant attention from both academic and pharmaceutical research in developing and characterizing synthetic retinoid analogues. Simplifying the hit development workflow for retinoid signaling will improve options available for tackling related pathologies, including tumor growth and neurodegeneration. Here, we present a novel assay that employs an intrinsically fluorescent synthetic retinoid, DC271, which allows direct measurement of the binding of nonlabeled compounds to relevant proteins. The method allows for straightforward initial measurement of binding using existing compound libraries and is followed by calculation of binding constants using a dilution series of plausible hits. The ease of use, high throughput format, and measurement of both qualitative and quantitative binding offer a new direction for retinoid-related pharmacological development.
机译:维生素A衍生的类视黄醇化合物具有多重,在细胞生长和发育循环中具有多种强大的作用,因此,在开发和表征合成类化醇类似物的学术和药物研究中引起了显着的关注。简化Retinoid Signaling的命中开发工作流程将改善可用于处理相关病理的选项,包括肿瘤生长和神经变性。这里,我们提出了一种使用内在荧光合成的类缬氨酸DC271的新型测定,其允许直接测量非标记化合物与相关蛋白质的结合。该方法允许使用现有化合物文库的结合的直接初始测量,然后使用稀释系列合理的命中计算结合常数。易用性,高通量格式和定性和定量结合的测量提供了与类视网膜相关药理学发育的新方向。

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