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Rationally designed helix-turn-helix proteins and their conformational changes upon DNA binding.

机译:合理设计的螺旋-转-螺旋蛋白质及其结合DNA后的构象变化。

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摘要

Circular dichroism and electrophoretic mobility shift studies were performed to confirm that dimerized N-terminal domains of bacterial repressors containing helix-turn-helix motifs are capable of high-affinity and specific DNA recognition as opposed to the monomeric N-terminal domains. Specific, high-affinity DNA binding proteins were designed and produced in which two copies of the N-terminal 1-62 domain of the bacteriophage 434 repressor are connected either in a dyad-symmetric fashion, with a synthetic linker attached to the C-termini, or as direct sequence repeats. Both molecules bound to their presumptive cognate nearly as tightly as does the natural (full-length and non-covalently dimerized) 434 repressor, showing that covalent dimerization can be used to greatly enhance the binding activity of individual protein segments. Circular dichroism spectroscopy showed a pronounced increase in the alpha-helix content when these new proteins interacted with their cognate DNA and a similar, although 30% lower, increase was also seen upon their interaction with non-cognate DNA. These results imply that a gradual conformational change may occur when helix-turn-helix motifs bind to DNA, and that a scanning mechanism is just as plausible for this motif class as that which is proposed for the more flexible basic-leucine zipper and basic-helix-loop-helix motifs.
机译:进行了圆二色性和电泳迁移率转移研究,以确认与螺旋N-末端-螺旋结构域相反,含有螺旋-转-螺旋基序的细菌阻遏物的二聚N-末端结构域能够具有高亲和力和特异性DNA识别。设计并生产了特异性,高亲和力的DNA结合蛋白,其中两个拷贝的噬菌体434阻遏物的N末端1-62结构域以对偶对称的方式连接,并在C末端连接了合成接头,或直接重复。两种分子与其推测的同源分子的结合几乎与天然(全长和非共价二聚体的)434阻遏物一样紧密,表明共价二聚体可用于大大增强单个蛋白质片段的结合活性。圆二色光谱显示,当这些新蛋白质与其同源DNA相互作用时,α-螺旋含量显着增加,尽管它们与非同源DNA相互作用也可见类似的增加,尽管降低了30%。这些结果表明,当螺旋-转-螺旋基序与DNA结合时,可能会发生逐渐的构象变化,并且对于这种基序类别,扫描机制与为更灵活的碱性-亮氨酸拉链和碱性-亮氨酸所提出的机制一样合理。螺旋-环-螺旋基序。

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