首页> 外文期刊>Biochemistry >Binding of SSB and RecA protein to DNA-containing stem loop structures: SSB ensures the polarity of RecA polymerization on single-stranded DNA.
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Binding of SSB and RecA protein to DNA-containing stem loop structures: SSB ensures the polarity of RecA polymerization on single-stranded DNA.

机译:SSB和RecA蛋白与含DNA的茎环结构的结合:SSB确保RecA在单链DNA上聚合的极性。

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Single-stranded DNA-binding proteins play an important role in homologous pairing and strand exchange promoted by the class of RecA-like proteins. It is presumed that SSB facilitates binding of RecA on to ssDNA by melting secondary structure, but direct physical evidence for the disruption of secondary structure by either SSB or RecA is still lacking. Using a series of oligonucleotides with increasing amounts of secondary structure, we show that stem loop structures impede contiguous binding of RecA and affect the rate of ATP hydrolysis. The electrophoretic mobility shift of a ternary complex of SSB-DNA-RecA and a binary complex of SSB-DNA are similar; however, the mechanism remains obscure. Binding of RecA on to stem loop is rapid in the presence of SSB or ATPgammaS and renders the complex resistant to cleavage by HaeIII, to higher amounts of competitor DNA or low temperature. The elongation of RecA filament in a 5' to 3' direction is halted at the proximal end of the stem. Consequently, RecA nucleates at the loop and cooperative binding propagates the RecA filament down the stem causing its disruption. The pattern of modification of thymine residues in the loop region indicates that RecA monomer is the minimum binding unit. Together, these results suggest that SSB plays a novel role in ensuring the directionality of RecA polymerization across stem loop in ssDNA. These observations have fundamental implications on the role of SSB in multiple aspects of cellular DNA metabolism.
机译:单链DNA结合蛋白在类RecA类蛋白促进的同源配对和链交换中起重要作用。推测SSB通过融化二级结构而促进RecA与ssDNA的结合,但是仍然缺乏直接物理证据证明SSB或RecA破坏二级结构。使用具有增加的二级结构量的一系列寡核苷酸,我们显示茎环结构阻碍RecA的连续结合并影响ATP水解的速率。 SSB-DNA-RecA的三元复合物和SSB-DNA的二元复合物的电泳迁移率变化相似。但是,该机制仍然不清楚。在存在SSB或ATPgammaS的情况下,RecA与茎环的结合迅速,并使复合物具有抗HaeIII裂解的能力,可抵抗更高量的竞争者DNA或低温。 RecA细丝在5'到3'方向的伸长在茎的近端停止。因此,RecA在环处成核,并且协作结合使RecA细丝沿茎向下传播,从而引起其破坏。环区域中胸腺嘧啶残基的修饰模式表明RecA单体是最小的结合单元。总之,这些结果表明,SSB在确保跨ssDNA的茎环的RecA聚合的方向性方面起着新颖的作用。这些观察对SSB在细胞DNA代谢的多个方面的作用具有根本意义。

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