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Use of site-specifically tethered chemical nucleases to study macromolecular reactions

机译:使用位点特异性束缚的化学核酸酶研究大分子反应

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During a complex macromolecular reaction multiple changes in molecular conformation and interactions with ligands may occur. X-ray crystallography may provide only a limited set of snapshots of these changes. Solution methods can augment such structural information to provide a more complete picture of a macromolecular reaction. We analyzed the changes in protein conformation and protein:nucleic acid interactions which occur during transcription initiation by using a chemical nuclease tethered to cysteines introduced site-specifically into the RNA polymerase of bacteriophage T7 (T7 RNAP). Changes in cleavage patterns as the polymerase steps through transcription reveal a series of structural transitions which mediate transcription initiation. Cleavage by tethered chemical nucleases is seen to be a powerful method for revealing the conformational dynamics of macromolecular reactions, and has certain advantages over cross-linking or energy transfer approaches.
机译:在复杂的大分子反应过程中,可能会发生分子构象变化以及与配体的相互作用。 X射线晶体学可能仅提供这些变化的有限快照。解决方法可以增强此类结构信息,以提供有关大分子反应的更完整描述。我们分析了转录过程中发生的蛋白质构象和蛋白质:核酸相互作用的变化,方法是使用与位点特异性引入到噬菌体T7的RNA聚合酶(T7 RNAP)中的半胱氨酸相连的化学核酸酶。随着聚合酶逐步转录,切割模式的变化揭示了一系列介导转录起始的结构转变。被束缚的化学核酸酶切割被认为是揭示大分子反应的构象动力学的有力方法,并且比交联或能量转移方法具有某些优势。

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