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肿瘤细胞与正常细胞中DNA复制的差异活跃起源

Differentially active origins of DNA replication in tumor versus normal cells.

作者信息

Di Paola Domenic, Price Gerald B, Zannis-Hadjopoulos Maria

机构信息

McGill Cancer Center and Department of Biochemistry, McGill University, Montreal, Quebec, Canada.

出版信息

Cancer Res. 2006 May 15;66(10):5094-103. doi: 10.1158/0008-5472.CAN-05-3951.

DOI:10.1158/0008-5472.CAN-05-3951
PMID:16707432
Abstract

Previously, a degenerate 36 bp human consensus sequence was identified as a determinant of autonomous replication in eukaryotic cells. Random mutagenesis analyses further identified an internal 20 bp of the 36 bp consensus sequence as sufficient for acting as a core origin element. Here, we have located six versions of the 20 bp consensus sequence (20mer) on human chromosome 19q13 over a region spanning approximately 211 kb and tested them for ectopic and in situ replication activity by transient episomal replication assays and nascent DNA strand abundance analyses, respectively. The six versions of the 20mer alone were capable of supporting autonomous replication of their respective plasmids, unlike random genomic sequence of the same length. Furthermore, comparative analyses of the endogenous replication activity of these 20mers at their respective chromosomal sites, in five tumor/transformed and two normal cell lines, done by in situ chromosomal DNA replication assays, involving preparation of nascent DNA by the lambda exonuclease method and quantification by real-time PCR, showed that these sites coincided with chromosomal origins of DNA replication in all cell lines. Moreover, a 2- to 3-fold higher origin activity in the tumor/transformed cells by comparison to the normal cells was observed, suggesting a higher activation of these origins in tumor/transformed cell lines.

摘要

此前,一个36 bp的简并人类共有序列被确定为真核细胞中自主复制的决定因素。随机诱变分析进一步确定,36 bp共有序列中的一个20 bp内部片段足以作为核心起始元件。在此,我们在人类19号染色体q13上跨越约211 kb的区域定位了六个版本的20 bp共有序列(20聚体),并分别通过瞬时游离型复制试验和新生DNA链丰度分析对它们的异位和原位复制活性进行了测试。与相同长度的随机基因组序列不同,这六个版本的20聚体单独就能支持各自质粒的自主复制。此外,通过原位染色体DNA复制试验对这五个肿瘤/转化细胞系和两个正常细胞系中这些20聚体在其各自染色体位点的内源性复制活性进行比较分析,该试验通过λ外切核酸酶法制备新生DNA并通过实时PCR进行定量,结果表明这些位点与所有细胞系中的DNA复制染色体起始位点一致。此外,与正常细胞相比,在肿瘤/转化细胞中观察到起始活性高2至3倍,这表明在肿瘤/转化细胞系中这些起始位点的激活程度更高。

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