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Label-free target identification using in-gel fluorescence difference via thermal stability shift

机译:通过热稳定性转移利用凝胶内荧光差异来进行无标记目标识别

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摘要

Target engagement is a prerequisite for the therapeutic effects of bioactive small molecules, and unbiased identification of their target proteins can facilitate drug discovery and chemical biology research. Structural modifications of bioactive natural products for target identification exhibit potential limitations such as synthetic difficulties, limited supplies from natural sources, and loss of original efficacy. Herein, we developed a label-free method for proteome-wide target identification using in-gel fluorescence difference caused by thermal stability shift, namely TS-FITGE. Quantitative intra-gel image analysis of each protein spot revealed target proteins with shifted thermal stability upon drug engagement, and plotting of melting curves by inter-gel analysis confirmed the positive targets. We demonstrated the robustness and applicability of the TS-FITGE method by identifying target proteins, including membrane-anchored proteins, of complex bioactive compounds. Furthermore, we identified and functionally validated nucleophosmin as a novel target protein of hordenine, a natural product upregulator of in vitro translation.
机译:靶标参与是生物活性小分子治疗效果的先决条件,其靶蛋白的无偏鉴定可以促进药物发现和化学生物学研究。用于靶标鉴定的生物活性天然产物的结构修饰具有潜在的局限性,例如合成困难,天然来源的供应有限以及原始功效的丧失。本文中,我们开发了一种无标记方法,可利用由热稳定性变化引起的凝胶内荧光差异(TS-FITGE)来进行蛋白质组范围内的目标识别。每个蛋白质斑点的定量凝胶内图像分析揭示了目标蛋白质在药物参与后热稳定性发生了变化,并且通过凝胶间分析绘制的熔解曲线证实了阳性目标。通过鉴定复杂生物活性化合物的靶蛋白(包括膜锚定蛋白),我们证明了TS-FITGE方法的鲁棒性和适用性。此外,我们确定了核磷酸蛋白并对其进行了功能验证,它是一种新的靶蛋白hordenine,它是体外翻译的天然产物上调剂。

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