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细胞胸苷激酶的诱导发生在mRNA水平。

Induction of cellular thymidine kinase occurs at the mRNA level.

作者信息

Stuart P, Ito M, Stewart C, Conrad S E

出版信息

Mol Cell Biol. 1985 Jun;5(6):1490-7. doi: 10.1128/mcb.5.6.1490-1497.1985.

DOI:10.1128/mcb.5.6.1490-1497.1985
PMID:2993867
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC366882/
Abstract

The thymidine kinase (TK) gene has been isolated from human genomic DNA. The gene was passaged twice by transfection of LTK- cells with human chromosomal DNA, and genomic libraries were made in lambda Charon 30 from a second-round TK+ transformant. When the library was screened with a human Alu probe, seven overlapping lambda clones from the human TK locus were obtained. None of the seven contained a functional TK gene as judged by transfection analysis, but several combinations of clones gave rise to TK+ colonies when cotransfected into TK- cells. A functional cDNA clone encoding the human TK gene has also been isolated. Using this cDNA clone as a probe in restriction enzyme/blot hybridization analyses, we have mapped the coding sequences and direction of transcription of the gene. We have also used a single-copy subclone from within the coding region to monitor steady-state levels of TK mRNA in serum-stimulated and simian virus 40-infected simian CV1 tissue culture cells. Our results indicate that the previously reported increase in TK enzyme levels seen after either treatment is paralleled by an equivalent increase in the steady-state levels of TK mRNA. In the case of simian virus 40-infected cells, the induction was delayed by 8 to 12 h, which is the length of time after infection required for early viral protein synthesis. In both cases, induction of TK mRNA coincides with the onset of DNA synthesis, but virally infected cells ultimately accumulate more TK mRNA than do serum-stimulated cells.

摘要

胸苷激酶(TK)基因已从人类基因组DNA中分离出来。通过用人染色体DNA转染LTK-细胞,该基因传代了两次,并从第二轮TK+转化体构建了λ噬菌体Charon 30基因组文库。当用人类Alu探针筛选该文库时,获得了来自人类TK基因座的7个重叠λ克隆。通过转染分析判断,这7个克隆中没有一个含有功能性TK基因,但将几个克隆组合共转染到TK-细胞中时,产生了TK+菌落。也分离出了一个编码人类TK基因的功能性cDNA克隆。使用这个cDNA克隆作为探针进行限制性内切酶/印迹杂交分析,我们已经绘制了该基因的编码序列和转录方向。我们还使用了编码区内的一个单拷贝亚克隆来监测血清刺激和猿猴病毒40感染的猿猴CV1组织培养细胞中TK mRNA的稳态水平。我们的结果表明,之前报道的在这两种处理后观察到的TK酶水平升高与TK mRNA稳态水平的等效升高相平行。在猿猴病毒40感染的细胞中,诱导延迟了8至12小时,这是感染后早期病毒蛋白合成所需的时间长度。在这两种情况下,TK mRNA的诱导都与DNA合成的开始同时发生,但病毒感染的细胞最终积累的TK mRNA比血清刺激的细胞更多。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/246d/366882/11bfc5e3a50d/molcellb00102-0307-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/246d/366882/10f95d7be2f0/molcellb00102-0305-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/246d/366882/275cead40c85/molcellb00102-0306-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/246d/366882/11bfc5e3a50d/molcellb00102-0307-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/246d/366882/10f95d7be2f0/molcellb00102-0305-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/246d/366882/275cead40c85/molcellb00102-0306-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/246d/366882/11bfc5e3a50d/molcellb00102-0307-a.jpg

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