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Fluorescent labeling of specific protein targets in vitro and in vivo

机译:体外和体内特定蛋白质靶标的荧光标记

摘要

New methods are provided for the post-genomic era that will permit the analysis of the dynamic expression and localization of gene products in living cells. Herein we propose the development of such a method from a bioorganic approach involving organic synthesis and protein engineering. Specifically, novel compounds bearing two maleimide groups attached directly to fluorescent cores will be prepared, whose latent fluorescence is quenched until their maleimide groups undergo a specific thiol addition reaction. Complementary a-helical proteins are designed bearing two cysteine residues appropriately positioned to react with our novel fluorogens. Genetically fusing our helical probe peptides to test proteins of interest, we can selectively label the target sequence in living cells with our small synthetic fluorogenic molecules. The scope of this technique is described in the context of studying protein localization and protein-protein interactions in living cells.
机译:为后基因组时代提供了新方法,该方法将允许分析活细胞中基因产物的动态表达和定位。本文中,我们建议从涉及有机合成和蛋白质工程的生物有机方法开发这种方法。具体而言,将制备带有两个直接连接至荧光核心的马来酰亚胺基团的新型化合物,将其潜在的荧光猝灭直至其马来酰亚胺基团进行特定的硫醇加成反应。设计了互补的α-螺旋蛋白,带有两个半胱氨酸残基,这些残基的位置适当,可以与我们的新型氟反应。通过遗传融合我们的螺旋探针肽来测试目标蛋白,我们可以用我们的合成荧光小分子选择性标记活细胞中的靶序列。在研究活细胞中的蛋白质定位和蛋白质-蛋白质相互作用的背景下描述了该技术的范围。

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