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Sharp DNA bends as landmarks of protein-binding sites on straightened DNA

机译:锋利的DNA弯曲为拉直的DNA上蛋白质结合位点的标志

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We have developed a fluorescence-based method for mapping single or multiple protein-binding sites on straightened, large-size DNA molecules (>5 kbp). In the described method, protein-DNA complexes were straightened and immobilized on a flat surface using surface tension. A fraction of the immobilized complexes displayed a sharp DNA bend with two DNA segments extending from the apex. The presence of DNA-binding proteins at the apex was verified by atomic force microscopy. The position of protein binding relative to the ends of the DNA molecule was determined by measuring the length of two DNA segments using fluorescence microscopy. We demonstrate the potential of the fluorescence-based method to localize protein-binding sites on the DNA template and to evaluate relative binding affinity. The proposed protein-binding-site mapping technique is simple and easy to perform. Practical applications include screening for DNA-binding proteins and the localization of protein-binding sites on large segments of DNA. [References: 41]
机译:我们已经开发出了一种基于荧光的方法,用于绘制拉直的大尺寸DNA分子(> 5 kbp)上的单个或多个蛋白质结合位点。在所述方法中,使用表面张力将蛋白质-DNA复合物拉直并固定在平坦表面上。固定化的复合物的一部分显示出尖锐的DNA弯曲,带有两个从顶点延伸的DNA片段。通过原子力显微镜证实了在顶点处DNA结合蛋白的存在。相对于DNA分子末端的蛋白质结合位置是通过使用荧光显微镜测量两个DNA片段的长度来确定的。我们证明了基于荧光的方法在DNA模板上定位蛋白质结合位点并评估相对结合亲和力的潜力。提出的蛋白质结合位点作图技术简单易行。实际应用包括筛选DNA结合蛋白和蛋白质结合位点在大片段DNA上的定位。 [参考:41]

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