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Locking the ATP-operated clamp of DNA gyrase: Probing the mechanism ofstrand passage

机译:锁定由ATP操作的DNA促旋酶夹:探究链通过的机制

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DNA gyrase catalyses DNA supercoiling by passing one segment of DNA (the T segment) through another (the G segment) in a reaction coupled to the binding and hydrolysis of ATP. The N-terminal domains of the gyrase B dimer constitute an ATP-operated clamp that is proposed to capture the T segment during the DNA supercoiling reaction. We have locked this clamp in the closed conformation using the non-hydrolysable ATP analogue ADPNP (5'-adenylyl beta,gamma -imidodiphosphate). The clamp-locked enzyme is able to bind and cleave DNA, albeit at a reduced level. Although the locked enzyme is not capable of carrying out DNA supercoiling, it can catalyse limited DNA relaxation, consistent with the ability to complete one strand passage event per enzyme molecule via entry of the T segment through the exit gate of the enzyme. The DNA-protein complex of the clamp-locked enzyme has a conformation that differs From the normal positively wrapped conformation of the gyrase-DNA complex. These experiments confirm the role of the ATP-operated clamp in the strand-passage reactions of gyrase and suggest a model for the interaction of DNA with gyrase in which a conformation with the T segment in equilibrium across the DNA gate can be achieved via T-segment entry through the ATP-operated clamp or through the exit gate.
机译:DNA促旋酶通过在与ATP的结合和水解偶联的反应中使一个DNA片段(T片段)通过另一个片段(G片段)来催化DNA超螺旋。促旋酶B二聚体的N-末端结构域构成了ATP操作的钳,该钳被提议在DNA超螺旋反应期间捕获T区段。我们已经使用不可水解的ATP类似物ADPNP(5'-腺苷基β,γ-亚氨基二磷酸酯)将该钳位锁定在闭合构象中。钳位锁定的酶能够结合和切割DNA,尽管含量降低了。尽管锁定的酶不能进行DNA超螺旋,但是它可以催化有限的DNA松弛,这与通过T区段通过酶的出口进入每个酶分子完成一个链传递事件的能力相一致。钳锁式酶的DNA-蛋白质复合物的构象与正常的旋回酶-DNA复合物的正包裹构象不同。这些实验证实了ATP操纵的夹具在回旋酶的链通道反应中的作用,并提出了DNA与回旋酶相互作用的模型,其中可通过T-来实现跨DNA门平衡的T段构象。通过ATP操作的夹具或通过出口进入段。

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