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胸苷激酶信使核糖核酸的过表达消除了胸苷激酶酶活性的细胞周期调控。

Overexpression of thymidine kinase mRNA eliminates cell cycle regulation of thymidine kinase enzyme activity.

作者信息

Mikulits W, Hengstschläger M, Sauer T, Wintersberger E, Müllner E W

机构信息

Institute of Molecular Biology, Vienna Biocenter, University of Vienna, Austria.

出版信息

J Biol Chem. 1996 Jan 12;271(2):853-60. doi: 10.1074/jbc.271.2.853.

DOI:10.1074/jbc.271.2.853
PMID:8557696
Abstract

Expression of thymidine kinase (TK) enzyme activity and mRNA is strictly S phase-specific in primary cells. In contrast, DNA tumor virus-transformed cells have enhanced and constitutive levels of TK mRNA during the whole cell cycle. Their TK protein abundance, however, still increases at the G1-S transition and stays high throughout G2 until mitosis. Therefore, post-transcriptional control must account for the decoupling of TK mRNA from protein synthesis in G1. To characterize the underlying mechanism, we studied the consequences of TK mRNA abundance on the cell cycle-dependent regulation of TK activity in nontransformed cells. Constitutive as well as conditional human and mouse TK cDNA vectors were stably transfected into mouse fibroblasts, which were subsequently synchronized by centrifugal elutriation. Low constitutive TK mRNA expression still resulted in a fluctuation of TK activity with a pronounced maximum in S phase. This pattern of cell cycle-dependent TK activity variation reflected the one in primary cell but is caused by post-transcriptional control. Increasing overexpression of TK transcripts after hormonal induction compromised this regulation. At the highest constant mRNA levels, regulation of enzyme activity was totally abolished in each phase of the cell cycle. These data indicate that post-transcriptional regulation of TK is tightly coupled to the amount of mRNA; high concentrations apparently titrate a factor(s) required for repressing TK production during G1 and presumably also G2.

摘要

胸苷激酶(TK)酶活性和mRNA的表达在原代细胞中严格呈S期特异性。相比之下,DNA肿瘤病毒转化细胞在整个细胞周期中TK mRNA水平升高且持续存在。然而,它们的TK蛋白丰度在G1-S期转换时仍会增加,并在整个G2期直至有丝分裂时保持高水平。因此,转录后调控必定是G1期TK mRNA与蛋白质合成解偶联的原因。为了阐明潜在机制,我们研究了TK mRNA丰度对未转化细胞中TK活性的细胞周期依赖性调控的影响。组成型以及条件性人源和鼠源TK cDNA载体被稳定转染到小鼠成纤维细胞中,随后通过离心淘析使其同步化。低水平的组成型TK mRNA表达仍会导致TK活性波动,在S期有明显峰值。这种细胞周期依赖性TK活性变化模式反映了原代细胞中的情况,但却是由转录后调控引起的。激素诱导后TK转录本的过表达增加破坏了这种调控。在最高的恒定mRNA水平下,细胞周期各阶段的酶活性调控完全被消除。这些数据表明,TK的转录后调控与mRNA量紧密相关;高浓度显然会滴定G1期以及可能还有G2期抑制TK产生所需的一个或多个因子。

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Overexpression of thymidine kinase mRNA eliminates cell cycle regulation of thymidine kinase enzyme activity.胸苷激酶信使核糖核酸的过表达消除了胸苷激酶酶活性的细胞周期调控。
J Biol Chem. 1996 Jan 12;271(2):853-60. doi: 10.1074/jbc.271.2.853.
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Different regulation of thymidine kinase during the cell cycle of normal versus DNA tumor virus-transformed cells.
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Post-transcriptional repression of thymidine kinase expression during cell cycle and growth stimulation.细胞周期和生长刺激过程中胸苷激酶表达的转录后抑制
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Serum-responsive expression from the murine thymidine kinase promoter is specifically disrupted in a transformed cell line.在一个转化细胞系中,来自小鼠胸苷激酶启动子的血清反应性表达被特异性破坏。
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Posttranscriptional control of thymidine kinase messenger RNA accumulation in cells released from G0-G1 phase blocks.
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Evidence for transcriptional and post-transcriptional control of the cellular thymidine kinase gene.细胞胸苷激酶基因转录和转录后调控的证据。
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