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人类和鼠类c-myb基因内含子4中调控序列的存在。

Presence of regulatory sequences within intron 4 of human and murine c-myb genes.

作者信息

Seib T, Welter C, Engel M, Theisinger B, Dooley S

机构信息

Human Genetics Department, University of Saarland, Homburg, Germany.

出版信息

Biochim Biophys Acta. 1994 Oct 18;1219(2):285-92. doi: 10.1016/0167-4781(94)90050-7.

Abstract

The molecular mechanisms that modulate c-myb mRNA transcription in hematopoietic cells appear to involve intron regulatory sequences. We have characterized the fourth of ten introns from both human and murine c-myb genes in regard to nucleotide sequence and specific protein binding. For this approach complete genomic c-myb intron 4 fragments were isolated from mouse and human DNA using PCR amplification with flanking exon-primers derived from the mouse gene. Comparison of the obtained sequences revealed strong homology between the two species. Using crude nuclear protein extracts from mouse and human myb expressing cells (70Z/3B; Molt4) and gel shift experiments we found specific protein interaction for both introns and to determine the protein binding site in detail, we performed DNase I footprinting. Our results indicate that the binding factor is absent in control cell lines without c-myb transcriptional activity, suggesting a possible positive regulatory function of the DNA-protein complex. To confirm these findings we introduced the human c-myb intron 4 DNA sequence into the EcoRI site of the pCAT-Promoter plasmid and transfected Molt4 cells with this chimeric construct. The transient expression studies revealed that intron 4 sequences possess enhancer activity. Thus, we have demonstrated that intron 4 sequences can be important for the regulation of c-myb proto-oncogene expression.

摘要

调节造血细胞中c-myb mRNA转录的分子机制似乎涉及内含子调控序列。我们已经从核苷酸序列和特异性蛋白结合方面对人和小鼠c-myb基因的十个内含子中的第四个进行了表征。对于这种方法,使用源自小鼠基因的侧翼外显子引物通过PCR扩增从小鼠和人类DNA中分离出完整的基因组c-myb内含子4片段。对所得序列的比较揭示了这两个物种之间的高度同源性。使用来自表达小鼠和人类myb的细胞(70Z/3B;Molt4)的粗核蛋白提取物和凝胶迁移实验,我们发现两个内含子都有特异性蛋白相互作用,为了详细确定蛋白结合位点,我们进行了DNase I足迹实验。我们的结果表明,在没有c-myb转录活性的对照细胞系中不存在结合因子,这表明DNA-蛋白复合物可能具有正调控功能。为了证实这些发现,我们将人类c-myb内含子4 DNA序列引入pCAT-启动子质粒的EcoRI位点,并用这种嵌合构建体转染Molt4细胞。瞬时表达研究表明内含子4序列具有增强子活性。因此,我们已经证明内含子4序列对于c-myb原癌基因表达的调节可能很重要。

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