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~1H NMR studies of a 17-mer DNA duplex

机译:17-mer DNA双链体的〜1 H NMR研究

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摘要

Transcription factor 1 (TF1), encoded by the Bacillus subtilis bacteriophage SPO1, is a DNA-binding protein of the HU family. In preparation for a determination of the structure of the DNA-TF1 complex, we have studied the conformation of one core 17-mer duplex d(5'-CACTACTCTTTGTAGTG-3')-d(5'-CACTACAAAGAGTAGTG-3'). NOESY, DQF-COSY and TOCSY spectroscopy provide resonance assignments of non-exchangeable and exchangeable protons, internucleotide and interstrand proton-proton distances, and dihedral angle constraints. Restrained molecular dynamics calculations yield a family of NMR solution structures for which the RMSD is 0.7 A (all atoms). The helical twist is 34.9° for the central 15 bp. Bends toward the major groove are located between the second and fourth base pairs from each end. The G12·C23 base pair, which is bounded on each side by consecutive A·T pairs, causes a local disturbance to the DNA helix that makes the conformations of the two end segments unsymmetrical. The pyrimidine rings at T9, T10 and T11 experience more extensive rotational movement than the rest of the structure.
机译:枯草芽孢杆菌噬菌体SPO1编码的转录因子1(TF1)是HU家族的一种DNA结合蛋白。在准备确定DNA-TF1复合物的结构时,我们研究了一个核心的17-mer双链体d(5'-CACTACTCTTTGTAGTG-3')-d(5'-CACTACAAAGAGTAGTG-3')的构象。 NOESY,DQF-COSY和TOCSY光谱提供了不可交换和可交换质子的共振分配,核苷酸间和链间质子-质子距离以及二面角约束。约束分子动力学计算产生了一系列的NMR溶液结构,其RMSD为0.7 A(所有原子)。中心15 bp的螺旋扭曲为34.9°。朝向主要凹槽的弯曲从每个端部位于第二和第四基对之间。 G12·C23碱基对在每一侧均由连续的A·T对限制,对DNA螺旋造成局部干扰,使两个末端片段的构象不对称。 T9,T10和T11处的嘧啶环比该结构的其余部分经历更广泛的旋转运动。

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