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Biochemical characterisation of the clamp/clamp loader proteins from the euryarchaeon Archaeoglobus fulgidus

机译:中华古细菌的钳/钳装载蛋白的生化特性

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Replicative polymerases of eukaryotes, prokaryotes and archaea obtain processivity using ring-shaped DNA sliding clamps that are loaded onto DNA by clamp loaders [replication factor C (RFC) in eukaryotes]. In this study, we cloned the two genes for the subunits of the RFC homologue of the euryarchaeon Archaeoglobus fulgidus. The proteins were expressed and purified from Escherichia coli both individually and as a complex. The afRFC subunits form a heteropentameric complex consisting of one copy of the large subunit and four copies of the small subunits. To analyse the functionality of afRFC, we also expressed the A.fulgidus PCNA homologue and a type B polymerase (PoIB1) in E.coli. In primer extension assays, afRFC stimulated the processivity of afPoIB1 in afPCNA-dependent reactions. Although the afRFC complex showed significant DNA-dependent ATPase activity, which could be further stimulated by afPCNA, neither of the isolated afRFC subunits showed this activity. However, both the large and small afRFC subunits showed interaction with afPCNA. Furthermore, we demonstrate that ATP binding, but not hydrolysis, is needed to stimulate interactions of the afRFC complex with afPCNA and DNA.
机译:真核生物,原核生物和古细菌的复制性聚合酶使用环状DNA滑动夹获得生产力,该环状DNA滑动夹通过钳夹加载器[真核生物中的复制因子C(RFC)]装载到DNA上。在这项研究中,我们克隆了两个古细菌古菌的RFC同源物的两个亚基的基因。分别和作为复合体从大肠杆菌表达和纯化蛋白质。 afRFC亚基形成一个杂五聚体复合物,由一个大亚基的拷贝和四个小亚基的拷贝组成。为了分析afRFC的功能,我们还在大肠杆菌中表达了A.fulgidus PCNA同源物和B型聚合酶(PoIB1)。在引物延伸分析中,afRFC刺激了afPCNA依赖性反应中afPoIB1的持续合成能力。尽管afRFC复合物显示出显着的DNA依赖性ATPase活性,可以被afPCNA进一步刺激,但分离出的afRFC亚基均未显示出该活性。但是,无论大小的afRFC亚基都显示与afPCNA的相互作用。此外,我们证明,需要ATP结合而不是水解来刺激afRFCNA复合体与afPCNA和DNA的相互作用。

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