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双向DNA复制起点在天然基因座以及附加型扩增的小鼠腺苷脱氨酶基因座中的定位。

Localization of a bidirectional DNA replication origin in the native locus and in episomally amplified murine adenosine deaminase loci.

作者信息

Carroll S M, DeRose M L, Kolman J L, Nonet G H, Kelly R E, Wahl G M

机构信息

Gene Expression Laboratory, Salk Institute for Biological Studies, La Jolla, California 92037.

出版信息

Mol Cell Biol. 1993 May;13(5):2971-81. doi: 10.1128/mcb.13.5.2971-2981.1993.

Abstract

Gene amplification is frequently mediated by the initial production of acentric, autonomously replicating extrachromosomal elements. The 4,000 extrachromosomal copies of the mouse adenosine deaminase (ADA) amplicon in B-1/50 cells initiate their replication remarkably synchronously in early S phase and at approximately the same time as the single-copy chromosomal locus from which they were derived. The abundance of ADA sequences and favorable replication timing characteristics in this system led us to determine whether DNA replication initiates in ADA episomes within a preferred region and whether this region is the same as that used at the corresponding chromosomal locus prior to amplification. This study reports the detection and localization of a discrete set of DNA fragments in the ADA amplicon which label soon after release of synchronized B-1/50 cells into S phase. A switch in template strand complementarity of Okazaki fragments, indicative of the initiation of bidirectional DNA replication, was found to lie within the same region. This putative replication origin is located approximately 28.5 kbp upstream of the 5' end of the ADA gene. The same region initiated DNA replication in the single-copy ADA locus of the parental cells. These analyses provide the first evidence that the replication of episomal intermediates involved in gene amplification initiates within a preferred region and that the same region is used to initiate DNA synthesis within the native locus.

摘要

基因扩增通常由无着丝粒的自主复制染色体外元件的初始产生介导。B - 1/50细胞中小鼠腺苷脱氨酶(ADA)扩增子的4000个染色体外拷贝在早S期显著同步启动复制,且与它们所源自的单拷贝染色体位点大致同时启动。该系统中ADA序列的丰度和有利的复制时间特征促使我们确定DNA复制是否在ADA附加体的一个优选区域内起始,以及该区域是否与扩增前相应染色体位点所使用的区域相同。本研究报告了在ADA扩增子中一组离散DNA片段的检测和定位,这些片段在同步化的B - 1/50细胞释放到S期后不久就被标记。发现冈崎片段模板链互补性的转变,这表明双向DNA复制的起始,位于同一区域内。这个假定的复制起点位于ADA基因5'端上游约28.5 kbp处。同一区域在亲代细胞的单拷贝ADA位点启动DNA复制。这些分析提供了首个证据,表明参与基因扩增的附加体中间体的复制在一个优选区域内起始,并且同一区域用于在天然位点启动DNA合成。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/21ce/359690/141423766b51/molcellb00017-0348-a.jpg

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