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Effect of transcriptional regulatory sequences on autonomous replication of plasmids in transient mammalian systems.

机译:转录调控序列对瞬时哺乳动物系统中质粒自主复制的影响。

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摘要

Transcriptional regulatory sequences often influence the efficiency of DNA replication, directly or indirectly, in bacteria, yeast, and animal virus systems. We have tested several transcriptional regulatory sequences for affecting DNA replication, based on pUC vector, in transient systems. Autonomous replication of transfected plasmids was assayed by PCR amplification of the fragments derived from the plasmids, which had replicated in mammalian cells. By this highly efficient method of detecting replicated molecules, pUC19, but not pUC18, showed a week replication activity in transfected cells. Nucleotide sequences around the HindIII site in pUC19 were required for replication. Monomers or dimers of the octamer transcription motif of the mouse immunoglobulin heavy chain gene, inserted in multicloning sites of pUC19, could stimulate replication, while the 4- or 6-mers did not, in contrast to the results on its transcription activity. Other transcriptional elements including AP1, HSE, and E2F also stimulated replication, but neither CRE nor Sp1 binding motif did. These results suggest that at least some of the transcriptional regulatory sequences function as-modulators of DNA replication as well as of transcription.
机译:转录调控序列通常直接或间接影响细菌,酵母和动物病毒系统中DNA复制的效率。我们已经在瞬时系统中基于pUC载体测试了几种影响DNA复制的转录调控序列。通过PCR扩增衍生自质粒的片段来检测转染质粒的自主复制,所述片段已在哺乳动物细胞中复制。通过这种检测复制分子的高效方法,pUC19(而非pUC18)在转染细胞中显示了一周的复制活性。复制需要pUC19中HindIII位点周围的核苷酸序列。小鼠免疫球蛋白重链基因的八聚体转录基序的单体或二聚体插入到pUC19的多克隆位点中,可以刺激复制,而4-或6-聚体则没有,这与其转录活性的结果相反。其他转录元件,包括AP1,HSE和E2F也刺激复制,但是CRE和Sp1结合基序都没有。这些结果表明,至少一些转录调节序列起着DNA复制以及转录调节剂的作用。

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