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A Luminescence-Based System for Identification of Genetically Encodable Inhibitors of Protein Aggregation

机译:基于发光的系统,用于鉴定蛋白质聚集的转基因可评估抑制剂

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Molecules that disrupt protein aggregation represent potential tool compounds for the investigation of numerous human disease states. However, the identification of small molecules capable of disrupting protein aggregation has proven challenging. Larger biomolecules such as antibodies and proteins are promising alternatives due to their increased size. Despite the promise of protein-based inhibitors, generalizable assays are needed to more readily identify proteins capable of inhibiting aggregation. Herein, we utilize our previously reported self-assembling NanoLuc luciferase fragments to engineer a platform in which both detection reagents are expressed from the same plasmid, enabling facile co-transformation with a genetically encodable inhibitor. This streamlined system is capable of detecting changes in the solubility of amylin, huntingtin, and amyloid-β (Aβ) proteins in response to mutations, small-molecule inhibitors, and expression of genetically encodable inhibitors. This improved platform provides a means to begin to identify protein-based inhibitors with improved efficacy.
机译:破坏蛋白质聚集的分子代表了用于调查众多人类疾病状态的潜在工具化合物。然而,鉴定了能够破坏蛋白质聚集的小分子已被证明是挑战性的。较大的生物分子如抗体和蛋白质是由于其尺寸增加而导致的替代品。尽管存在基于蛋白质的抑制剂,但需要更容易地识别能够抑制聚集的蛋白质来达到可推广的测定。在此,我们利用我们先前报道的自组装纳米荧光素酶片段来工程师,其中两个检测试剂从相同的质粒表达,使得能够与遗传可接受的抑制剂进行体内共转化。该流线型系统能够检测氨基素,亨廷顿和淀粉样蛋白-β(Aβ)蛋白响应突变,小分子抑制剂和转基因可评估抑制剂的表达的溶解度的变化。这种改进的平台提供了开始鉴定基于蛋白质的抑制剂的方法,具有改善的功效。

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