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Rate, origin, and bidirectionality of Caulobacter chromosome replication as determined by pulsed-field gel electrophoresis.

机译:通过脉冲场凝胶电泳确定的Caulobacter染色体复制的速率,起源和双向性。

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摘要

Cell division in Caulobacter crescentus yields progeny cells that differ with respect to cell structure and developmental program. Chromosome replication initiates in the daughter stalked cell but is repressed in the daughter swarmer cell until later in the cell cycle. To study cell-type-specific DNA initiation, chromosome replication was directly analyzed by pulsed-field gel electrophoresis. Analysis of Dra I restriction fragments of DNA taken at various times from synchronized cell cultures labeled with 2'-deoxy[3H]guanosine has allowed us to determine the origin of DNA replication, the rate and direction of fork movement, and the order of gene replication. The first labeled Dra I fragment to appear contains the site of replication initiation. Based on the correlation of the physical and genetic maps derived by Ely and Gerardot [Ely, B. & Gerardot, C. J. (1988) Gene 68, 323-333], the origin was localized to a 305-kilobase fragment containing the rrnA gene. Furthermore, the sequential replication through unmapped Dra I fragments has enabled us to localize their positions on the genome. The order of appearance of labeled restriction fragments revealed that the chromosome replicates bidirectionally at a fork movement rate of 21 kilobases per minute.
机译:新月形杆菌中的细胞分裂产生的后代细胞在细胞结构和发育程序方面有所不同。染色体复制始于子茎细胞,但在子群细胞中受到抑制,直到细胞周期后期。为了研究特定于细胞类型的DNA起始,通过脉冲场凝胶电泳直接分析了染色体复制。分析从2'-脱氧[3H]鸟苷标记的同步细胞培养物中在不同时间采集的DNA的Dra I限制性片段,这使我们能够确定DNA复制的起点,叉运动的速率和方向以及基因的顺序复制。出现的第一个标记的Dra I片段包含复制起始位点。基于Ely和Gerardot [Ely,B。和Gerardot,C.J。(1988)基因68,323-333]推导的物理图谱和遗传图谱的相关性,将起源定位于含有rrnA基因的305碱基的片段。此外,通过未映射的Dra I片段的顺序复制使我们能够定位它们在基因组上的位置。标记的限制性片段的出现顺序表明,染色体以21 km / min的分叉运动速率双向复制。

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  • 作者

    Dingwall, A; Shapiro, L;

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  • 年度 1989
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  • 原文格式 PDF
  • 正文语种 en
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