缺乏H-NS蛋白会导致大肠杆菌染色体复制和分离过程中DNA延伸且定位异常。
Lack of the H-NS Protein Results in Extended and Aberrantly Positioned DNA during Chromosome Replication and Segregation in Escherichia coli.
作者信息
Helgesen Emily, Fossum-Raunehaug Solveig, Skarstad Kirsten
机构信息
Department of Molecular Cell Biology, Institute for Cancer Research, Oslo University Hospital, Radiumhospitalet, Oslo, Norway.
Department of Molecular Cell Biology, Institute for Cancer Research, Oslo University Hospital, Radiumhospitalet, Oslo, Norway School of Pharmacy, Faculty of Mathematics and Natural Sciences, University of Oslo, Oslo, Norway.
出版信息
J Bacteriol. 2016 Mar 31;198(8):1305-16. doi: 10.1128/JB.00919-15. Print 2016 Apr.
UNLABELLED
The architectural protein H-NS binds nonspecifically to hundreds of sites throughout the chromosome and can multimerize to stiffen segments of DNA as well as to form DNA-protein-DNA bridges. H-NS has been suggested to contribute to the orderly folding of the Escherichia coli chromosome in the highly compacted nucleoid. In this study, we investigated the positioning and dynamics of the origins, the replisomes, and the SeqA structures trailing the replication forks in cells lacking the H-NS protein. In H-NS mutant cells, foci of SeqA, replisomes, and origins were irregularly positioned in the cell. Further analysis showed that the average distance between the SeqA structures and the replisome was increased by ∼100 nm compared to that in wild-type cells, whereas the colocalization of SeqA-bound sister DNA behind replication forks was not affected. This result may suggest that H-NS contributes to the folding of DNA along adjacent segments. H-NS mutant cells were found to be incapable of adopting the distinct and condensed nucleoid structures characteristic of E. coli cells growing rapidly in rich medium. It appears as if H-NS mutant cells adopt a “slow-growth” type of chromosome organization under nutrient-rich conditions, which leads to a decreased cellular DNA content.
IMPORTANCE
It is not fully understood how and to what extent nucleoid-associated proteins contribute to chromosome folding and organization during replication and segregation in Escherichia coli. In this work, we find in vivo indications that cells lacking the nucleoid-associated protein H-NS have a lower degree of DNA condensation than wild-type cells. Our work suggests that H-NS is involved in condensing the DNA along adjacent segments on the chromosome and is not likely to tether newly replicated strands of sister DNA. We also find indications that H-NS is required for rapid growth with high DNA content and for the formation of a highly condensed nucleoid structure under such conditions.
未标记
结构蛋白H-NS非特异性地结合于整个染色体上的数百个位点,并且能够多聚化以使DNA片段变硬,还能形成DNA-蛋白质-DNA桥。有人提出H-NS有助于大肠杆菌染色体在高度压缩的类核中有序折叠。在本研究中,我们调查了缺乏H-NS蛋白的细胞中复制起点、复制体以及跟随复制叉的SeqA结构的定位和动态变化。在H-NS突变细胞中,SeqA、复制体和复制起点的焦点在细胞内的定位不规则。进一步分析表明,与野生型细胞相比,SeqA结构与复制体之间的平均距离增加了约100纳米,而复制叉后结合SeqA的姐妹DNA的共定位不受影响。这一结果可能表明H-NS有助于DNA沿相邻片段折叠。我们发现H-NS突变细胞无法形成在丰富培养基中快速生长的大肠杆菌细胞特有的独特且浓缩的类核结构。在营养丰富的条件下,H-NS突变细胞似乎采用了一种“缓慢生长”型的染色体组织形式,这导致细胞DNA含量降低。
重要性
目前尚不完全清楚类核相关蛋白在大肠杆菌复制和分离过程中如何以及在多大程度上促进染色体折叠和组织。在这项工作中,我们在体内发现缺乏类核相关蛋白H-NS的细胞比野生型细胞具有更低程度的DNA浓缩。我们的工作表明,H-NS参与染色体上相邻片段的DNA浓缩,不太可能连接姐妹DNA的新复制链。我们还发现有迹象表明,在高DNA含量的快速生长以及在此类条件下形成高度浓缩的类核结构过程中,H-NS是必需的。
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