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The unstructured C-terminus of the τ subunit of Escherichia coli DNA polymerase III holoenzyme is the site of interaction with the α subunit

机译:大肠杆菌DNA聚合酶III全酶的τ亚基的非结构化C末端是与α亚基相互作用的位点

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摘要

The τ subunit of Escherichia coli DNA polymerase III holoenzyme interacts with the α subunit through its C-terminal Domain V, τC16. We show that the extreme C-terminal region of τC16 constitutes the site of interaction with α. The τC16 domain, but not a derivative of it with a C-terminal deletion of seven residues (τC16Δ7), forms an isolable complex with α. Surface plasmon resonance measurements were used to determine the dissociation constant (KD) of the α−τC16 complex to be ∼260 pM. Competition with immobilized τC16 by τC16 derivatives for binding to α gave values of KD of 7 μM for the α−τC16Δ7 complex. Low-level expression of the genes encoding τC16 and τC16▵7, but not τC16Δ11, is lethal to E. coli. Suppression of this lethal phenotype enabled selection of mutations in the 3′ end of the τC16 gene, that led to defects in α binding. The data suggest that the unstructured C-terminus of τ becomes folded into a helix–loop–helix in its complex with α. An N-terminally extended construct, τC24, was found to bind DNA in a salt-sensitive manner while no binding was observed for τC16, suggesting that the processivity switch of the replisome functionally involves Domain IV of τ.
机译:大肠杆菌DNA聚合酶III全酶的τ亚基通过其C端结构域VτC16与α亚基相互作用。我们表明,τC16的极端C端区域构成了与α相互作用的位点。 τC16结构域(但不是其衍生物)具有7个残基的C端缺失(τC16Δ7),与α形成了可分离的复合物。表面等离振子共振测量用于确定α-τC16复合物的解离常数(KD)为〜260 pM。 τC16衍生物与固定的τC16竞争与α的结合,得出α-τC16Δ7复合物的KD值为7μM。编码τC16和τC16▵7的基因的低水平表达,而不是τC16Δ11,对大肠杆菌具有致命性。抑制这种致死表型可以选择τC16基因3'端的突变,从而导致α结合缺陷。数据表明,τ的非结构化C末端折叠成与α复杂的螺旋-环-螺旋。发现N末端延伸的构建体τC24以盐敏感的方式结合DNA,而未观察到τC16的结合,表明复制体的持续性开关功能上涉及τ的结构域IV。

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