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Single-Molecule Atomic Force Spectroscopy Reveals that DnaD Forms Scaffolds and Enhances Duplex Melting

机译:单分子原子力光谱揭示了DnaD形成支架并增强了双链熔解

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摘要

The Bacillus subtilis DnaD is an essential DNA-binding protein implicated in replication and DNA remodeling. Using single-molecule atomic force spectroscopy, we have studied the interaction of DnaD and its domains with DNA. Our data reveal that binding of DnaD to immobilized single molecules of duplex DNA causes a marked reduction in the ‘end-to-end’ distance of the DNA in a concentration-dependent manner, consistent with previously reported DnaD-induced looping by scaffold formation. Native DnaD enhances partial melting of the DNA strands. The C-terminal domain (Cd) of DnaD binds to DNA and enhances partial duplex melting but does not cause DNA looping. The Cd-mediated melting is not as efficient as that caused by native DnaD. The N-terminal domain (Nd) does not affect significantly the DNA. A mixture of Nd and Cd fails to recreate the DNA looping effect of native DnaD but produces exactly the same effects as Cd on its own, consistent with the previously reported failure of the separated domains to form DNA-interacting scaffolds.
机译:枯草芽孢杆菌DnaD是一种必需的DNA结合蛋白,与复制和DNA重塑有关。使用单分子原子力光谱,我们研究了DnaD及其域与DNA的相互作用。我们的数据表明,DnaD与固定的双链DNA单分子结合会导致DNA的“端对端”距离显着降低,且呈浓度依赖性,这与先前报道的DnaD诱导的支架形成环相一致。天然DnaD增强了DNA链的部分融解。 DnaD的C末端域(Cd)与DNA结合并增强部分双链体解链,但不会引起DNA环化。 Cd介导的融解不如天然DnaD引起的融解有效。 N末端结构域(Nd)不会显着影响DNA。 Nd和Cd的混合物无法重现天然DnaD的DNA环化作用,但单独产生与Cd完全相同的作用,这与先前报道的分离结构域形成DNA相互作用支架的失败一致。

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