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Experimental maps of DNA structure at nucleotide resolution distinguish intrinsic from protein-induced DNA deformations

机译:核苷酸分辨率下的DNA结构实验图可区分蛋白质诱导的DNA内在变形

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摘要

Recognition of DNA by proteins depends on DNA sequence and structure. Often unanswered is whether the structure of naked DNA persists in a protein–DNA complex, or whether protein binding changes DNA shape. While X-ray structures of protein–DNA complexes are numerous, the structure of naked cognate DNA is seldom available experimentally. We present here an experimental and computational analysis pipeline that uses hydroxyl radical cleavage to map, at single-nucleotide resolution, DNA minor groove width, a recognition feature widely exploited by proteins. For 11 protein–DNA complexes, we compared experimental maps of naked DNA minor groove width with minor groove width measured from X-ray co-crystal structures. Seven sites had similar minor groove widths as naked DNA and when bound to protein. For four sites, part of the DNA in the complex had the same structure as naked DNA, and part changed structure upon protein binding. We compared the experimental map with minor groove patterns of DNA predicted by two computational approaches, DNAshape and ORChID2, and found good but not perfect concordance with both. This experimental approach will be useful in mapping structures of DNA sequences for which high-resolution structural data are unavailable. This approach allows probing of protein family-dependent readout mechanisms.
机译:蛋白质对DNA的识别取决于DNA序列和结构。裸DNA的结构是否持久存在于蛋白质-DNA复合物中,还是蛋白质结合是否改变了DNA形状,这通常是无法回答的。尽管蛋白质-DNA复合物的X射线结构很多,但裸同源DNA的结构很少能通过实验获得。我们在这里介绍了一个实验和计算分析流程,该流程使用羟基自由基切割来以单核苷酸分辨率映射DNA小沟宽度,这种识别特征被蛋白质广泛利用。对于11种蛋白质-DNA复合物,我们比较了裸露的DNA小沟槽宽度和从X射线共晶体结构测量的小沟槽宽度的实验图。当结合到蛋白质上时,七个位点的凹槽宽度与裸露的DNA相似。对于四个位点,复合物中的部分DNA具有与裸露DNA相同的结构,而部分在蛋白质结合后会改变结构。我们将实验图与通过两种计算方法(DNAshape和ORChID2)预测的较小的DNA凹槽模式进行了比较,发现两者的一致性很好,但不是完美的一致性。这种实验方法将可用于绘制无法获得高分辨率结构数据的DNA序列的结构图。这种方法允许探测蛋白质家族依赖性的读出机制。

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