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Exonuclease III protection assay with FRET probe for detecting DNA-binding proteins

机译:用FRET探针进行核酸外切酶III保护检测以检测DNA结合蛋白

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We describe a new method for the assay of sequence-specific DNA-binding proteins in this paper. In this method, the sensitive fluorescence resonance energy transfer (FRET) technology is combined with the common DNA footprinting assay in order to develop a simple, rapid and high-throughput approach for quantitatively detecting the sequence-specific DNA-binding proteins. We named this method as exonuclease III (ExoIII) protection assay with FRET probe. The FRET probe used in this assay was a duplex DNA which was designed to contain one FRET pair in the center and two flanking protein-binding sites. During protein detection, if a target protein exists, it will bind to the two protein-binding sites of the FRET probe and thus protect the FRET pair from ExoIII digestion, resulting in high FRET. However, if the target protein does not exist, the FRET pair on the naked FRET probe will be degraded by ExoIII, resulting in low FRET. Three kinds of recombinant transcription factors including NF-κB, SP1 and p50, and the target protein of NF-κB in HeLa cell nuclear extracts, were successfully detected by the assay. This assay can be extensively used in biomedical research targeted at DNA-binding proteins.
机译:我们在本文中描述了一种测定序列特异性DNA结合蛋白的新方法。在这种方法中,将敏感的荧光共振能量转移(FRET)技术与常见的DNA足迹测定法相结合,以开发出一种简单,快速,高通量的方法来定量检测序列特异性DNA结合蛋白。我们将该方法命名为FRET探针的核酸外切酶III(ExoIII)保护试验。用于该测定的FRET探针是双链DNA,其被设计为在中心包含一对FRET,在两个侧翼结合蛋白质的结合位点。在蛋白质检测过程中,如果存在目标蛋白质,它将与FRET探针的两个蛋白质结合位点结合,从而保护FRET对免于被ExoIII消化,从而导致高FRET。但是,如果目标蛋白不存在,则裸FRET探针上的FRET对将被ExoIII降解,导致FRET降低。通过检测成功地检测到了HeLa细胞核提取物中的三种重组转录因子,包括NF-κB,SP1和p50以及NF-κB的靶蛋白。该测定法可广泛用于针对DNA结合蛋白的生物医学研究。

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