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首页> 外文期刊>Nucleic acids research >ATP-regulated interactions between P1 ParA, ParB and non-specific DNA that are stabilized by the plasmid partition site, parS
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ATP-regulated interactions between P1 ParA, ParB and non-specific DNA that are stabilized by the plasmid partition site, parS

机译:P1 ParA,ParB与非特异性DNA之间的ATP调节相互作用,该相互作用由质粒分配位点parS稳定

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Localization of the P1 plasmid requires two proteins, ParA and ParB, which act on the plasmid partition site, parS. ParB is a site-specific DNA-binding protein and ParA is a Walker-type ATPase with non-specific DNA-binding activity. In vivo ParA binds the bacterial nucleoid and forms dynamic patterns that are governed by the ParB–parS partition complex on the plasmid. How these interactions drive plasmid movement and localization is not well understood. Here we have identified a large protein–DNA complex in vitro that requires ParA, ParB and ATP, and have characterized its assembly by sucrose gradient sedimentation and light scattering assays. ATP binding and hydrolysis mediated the assembly and disassembly of this complex, while ADP antagonized complex formation. The complex was not dependent on, but was stabilized by, parS. The properties indicate that ParA and ParB are binding and bridging multiple DNA molecules to create a large meshwork of protein–DNA molecules that involves both specific and non-specific DNA. We propose that this complex represents a dynamic adaptor complex between the plasmid and nucleoid, and further, that this interaction drives the redistribution of partition proteins and the plasmid over the nucleoid during partition.
机译:P1质粒的定位需要两个蛋白ParA和ParB,它们作用于质粒分配位点parS。 ParB是一种位点特异性DNA结合蛋白,ParA是具有非特异性DNA结合活性的Walker型ATPase。在体内,ParA结合细菌核苷并形成动态模式,该模式由质粒上的ParB–parS分配复合体控制。这些相互作用如何驱动质粒的移动和定位尚不清楚。在这里,我们已经鉴定出需要ParA,ParB和ATP的大型蛋白质-DNA复合物,并通过蔗糖梯度沉降和光散射法对其组装进行了表征。 ATP结合和水解介导该复合物的组装和拆卸,而ADP拮抗复合物的形成。复合体不依赖于parS,而是由parS稳定。这些特性表明,ParA和ParB结合并桥接多个DNA分子,形成了一个包含特定DNA和非特定DNA的大型蛋白质-DNA分子网。我们提出,该复合物代表质粒和核苷之间的动态衔接子复合物,并且进一步,这种相互作用驱动分配蛋白和质粒在分配过程中在核苷上的重新分布。

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