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在小鼠3T3细胞中,通过正义和反义RNA表达对DNA聚合酶β的调控异常会改变细胞生长。

Deregulation of DNA polymerase beta by sense and antisense RNA expression in mouse 3T3 cells alters cell growth.

作者信息

Zmudzka B Z, Wilson S H

机构信息

Laboratory of Biochemistry, National Cancer Institute, National Institutes of Health, Bethesda, Maryland 20892.

出版信息

Somat Cell Mol Genet. 1990 Jul;16(4):311-20. doi: 10.1007/BF01232459.

Abstract

DNA polymerase beta (beta-pol) and its mRNA are maintained at constitutive levels during the cell cycle and during stages of cell growth in culture. To study biological consequences of variations in the level of this DNA repair enzyme and/or its mRNA, we prepared expression vectors in which cDNA for human beta-pol is inserted under the control of a metallothionein promoter (pMT) in the sense and antisense orientation, respectively, and these vectors then were used for stable transformation of mouse 3T3 cells. Vectors also contained the mouse DHFR gene, such that culture of transformants in medium with increasing concentrations of methotrexate resulted in amplification of inserted DNA. The levels of sense and antisense transcripts are strongly increased by culture of transformants in medium with 65 microM Zn2+, although some expression is detected even without Zn2+ induction. After five days of induction, the beta-pol level was about threefold higher in sense cells and about 10-fold lower in antisense cells than in parallel cultures without induction. The antisense line has a threefold increased cell doubling time in the presence of 65 microM Zn2+ compared with the absence of Zn2+. Zn2+ (65 microM) induction for the sense line results in normal growth for the first three days and, thereafter, a complete cessation of growth. Yet, these blocked cells remain fully viable. The results indicate that sudden deregulation of beta-pol expression alters cell growth in mouse 3T3 cells.

摘要

DNA聚合酶β(β-pol)及其mRNA在细胞周期和培养的细胞生长阶段维持在组成水平。为了研究这种DNA修复酶及其mRNA水平变化的生物学后果,我们制备了表达载体,其中人β-pol的cDNA分别以正义和反义方向插入金属硫蛋白启动子(pMT)的控制下,然后将这些载体用于小鼠3T3细胞的稳定转化。载体还包含小鼠二氢叶酸还原酶(DHFR)基因,使得在含有浓度递增的甲氨蝶呤的培养基中培养转化体导致插入DNA的扩增。在含有65μM Zn2+的培养基中培养转化体可强烈增加正义和反义转录物的水平,尽管即使没有Zn2+诱导也能检测到一些表达。诱导五天后,与未诱导的平行培养物相比,正义细胞中的β-pol水平高约三倍,反义细胞中的β-pol水平低约10倍。与不存在65μM Zn2+相比,反义细胞系在存在65μM Zn2+时细胞倍增时间增加了三倍。对正义细胞系用65μM Zn2+诱导在最初三天导致正常生长,此后完全停止生长。然而,这些停滞的细胞仍然完全存活。结果表明,β-pol表达的突然失调会改变小鼠3T3细胞的生长。

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