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烟草核糖核苷酸还原酶RNR1和RNR2 cDNA的分子特征及在同步化植物细胞中的细胞周期调控表达

Molecular characterization of tobacco ribonucleotide reductase RNR1 and RNR2 cDNAs and cell cycle-regulated expression in synchronized plant cells.

作者信息

Chabouté M E, Combettes B, Clément B, Gigot C, Philipps G

机构信息

Institut de Biologie Moléculaire des Plantes du CNRS, Université Louis Pasteur, Strasbourg, France.

出版信息

Plant Mol Biol. 1998 Nov;38(5):797-806. doi: 10.1023/a:1006083318906.

Abstract

Eukaryotic ribonucleotide reductase (RNR), the enzyme involved in the synthesis of the deoxyribonucleotides, consists of two R1 and R2 subunits whose activities and gene expression are differentially regulated during the cell cycle and are preferentially induced at the G1/S transition. We have isolated three cDNA clones from a tobacco S phase library, two encoding the large R1 subunit, the first cloned in plants, and one encoding the small R2 subunit. From Southern blot hybridization we deduce that RNR2 is encoded by a single-copy gene whereas RNR1 is encoded by a small multigene family. The level of RNR mRNA is cell-cycle regulated showing a maximum in S phase. In mid-S phase, RNR2 transcripts show a higher maximum level than RNR1 transcripts. Analysis of the effects of various cell cycle inhibitors added to freshly subcultured stationary phase cells leads to the conclusion that RNR gene induction at the entry of the cells into the cell cycle takes place in late G1-early S phase. Addition of DNA synthesis-blocking agents to cycling cells synchronized in mid-S phase resulted in an enhancement of RNR transcript level, thus suggesting that RNR gene expression may be linked to the DNA synthesis rate by a feedback-like regulatory mechanism.

摘要

真核核糖核苷酸还原酶(RNR)是参与脱氧核糖核苷酸合成的酶,由两个R1和R2亚基组成,其活性和基因表达在细胞周期中受到不同调节,并在G1/S期转换时优先被诱导。我们从烟草S期文库中分离出三个cDNA克隆,两个编码大的R1亚基,这是首次在植物中克隆到的,另一个编码小的R2亚基。通过Southern印迹杂交我们推断RNR2由单拷贝基因编码,而RNR1由一个小的多基因家族编码。RNR mRNA水平受细胞周期调节,在S期达到最高。在S期中期,RNR2转录本的最高水平高于RNR1转录本。对添加到新传代的静止期细胞中的各种细胞周期抑制剂的作用进行分析得出结论,细胞进入细胞周期时RNR基因的诱导发生在G1晚期-S期早期。向在S期中期同步化的循环细胞中添加DNA合成阻断剂导致RNR转录本水平升高,因此表明RNR基因表达可能通过一种类似反馈的调节机制与DNA合成速率相关联。

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