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Analysis of ParB-centromere interactions by multiplex SPR imaging reveals specific patterns for binding ParB in six centromeres of Burkholderiales chromosomes and plasmids

机译:通过多重SPR成像分析ParB-着丝粒相互作用揭示了在Burkholderiales染色体和质粒的六个着丝粒中结合ParB的特定模式

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摘要

Bacterial centromeres–also called parS, are cis-acting DNA sequences which, together with the proteins ParA and ParB, are involved in the segregation of chromosomes and plasmids. The specific binding of ParB to parS nucleates the assembly of a large ParB/DNA complex from which ParA—the motor protein, segregates the sister replicons. Closely related families of partition systems, called Bsr, were identified on the chromosomes and large plasmids of the multi-chromosomal bacterium Burkholderia cenocepacia and other species from the order Burkholeriales. The centromeres of the Bsr partition families are 16 bp palindromes, displaying similar base compositions, notably a central CG dinucleotide. Despite centromeres bind the cognate ParB with a narrow specificity, weak ParB-parS non cognate interactions were nevertheless detected between few Bsr partition systems of replicons not belonging to the same genome. These observations suggested that Bsr partition systems could have a common ancestry but that evolution mostly erased the possibilities of cross-reactions between them, in particular to prevent replicon incompatibility. To detect novel similarities between Bsr partition systems, we have analyzed the binding of six Bsr parS sequences and a wide collection of modified derivatives, to their cognate ParB. The study was carried out by Surface Plasmon Resonance imaging (SPRi) mulitplex analysis enabling a systematic survey of each nucleotide position within the centromere. We found that in each parS some positions could be changed while maintaining binding to ParB. Each centromere displays its own pattern of changes, but some positions are shared more or less widely. In addition from these changes we could speculate evolutionary links between these centromeres.
机译:细菌着丝粒(也称为parS)是顺式作用的DNA序列,与蛋白质ParA和ParB一起参与染色体和质粒的分离。 ParB与parS的特异性结合使大型ParB / DNA复合体的组装成核,ParA(运动蛋白)从中分离出姐妹复制子。在多染色体细菌伯克霍尔德氏菌和来自伯克霍尔德氏菌的其他物种的染色体和大质粒上鉴定了密切相关的称为Bsr的分配系统家族。 Bsr分区家族的着丝粒是16 bp回文,显示相似的碱基组成,特别是中央CG二核苷酸。尽管着丝粒以狭窄的特异性结合同源的ParB,但是在少数不属于同一基因组的复制子的Bsr分配系统之间检测到弱的ParB-parS非同源相互作用。这些观察结果表明,Bsr分区系统可能具有共同的血统,但是进化过程却消除了它们之间交叉反应的可能性,特别是为了防止复制子不兼容。为了检测Bsr分区系统之间的新颖相似性,我们分析了六个Bsr parS序列和大量的修饰衍生物与它们的同源ParB的结合。该研究是通过表面等离振子共振成像(SPRi)多重分析进行的,从而能够对着丝粒内每个核苷酸位置进行系统的调查。我们发现在每个parS中可以更改某些位置,同时保持与ParB的绑定。每个着丝粒都显示出自己的变化模式,但是某些位置或多或少地共享。除了这些变化,我们还可以推测这些着丝粒之间的进化联系。

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