首页> 美国卫生研究院文献>Molecular and Cellular Biology >Dual bidirectional promoters at the mouse dhfr locus: cloning and characterization of two mRNA classes of the divergently transcribed Rep-1 gene.
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Dual bidirectional promoters at the mouse dhfr locus: cloning and characterization of two mRNA classes of the divergently transcribed Rep-1 gene.

机译:小鼠dhfr基因座上的双向双向启动子:不同转录的Rep-1基因的两个mRNA类的克隆和表征。

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摘要

The mouse dihydrofolate reductase gene (dhfr) is a housekeeping gene expressed under the control of a promoter region embedded in a CpG island--a region rich in unmethylated CpG dinucleotides. A divergent transcription unit exists immediately upstream of the dhfr gene which is coamplified with dhfr in some but not all methotrexate-resistant cell lines. We show that the promoter region for this gene pair consists of two bidirectional promoters, a major and minor promoter, which are situated within a 660-base-pair region upstream of the dhfr ATG translation initiation codon. The major promoter controls over 90% of dhfr transcription, while the minor promoter directs the transcription of the remaining dhfr mRNAs. The major promoter functions bidirectionally, transcribing a divergent 4.0-kilobase poly(A) mRNA (class A) in the direction opposite that of dhfr transcription. The predicted protein product of this mRNA is 105 kilodaltons. The minor promoter also functions bidirectionally, directing the transcription of at least two divergent RNAs (class B). These RNAs, present in quantities approximately 1/10 to 1/50 that of the class A mRNAs, are 4.4- and 1.6-kilobase poly(A) mRNAs. cDNAs representing both class A and class B mRNAs have been cloned from a mouse fibroblast cell line which has amplified the dhfr locus (3T3R500). DNA sequence analysis of these cDNAs reveals that the class A and class B mRNAs share, for the most part, the same exons. On the basis of S1 nuclease protection analysis of RNA preparations from several mouse tissues, both dhfr and divergent genes showed similar levels of expression but did show some specificity in start site utilization. Computer homology searches have revealed sequence similarity of the divergent transcripts with bacterial genes involved in DNA mismatch repair, and we therefore have named the divergently transcribed gene Rep-1.
机译:小鼠二氢叶酸还原酶基因(dhfr)是管家基因,在嵌入CpG岛的启动子区域的控制下表达,该区域富含未甲基化的CpG二核苷酸。 dhfr基因的上游紧邻存在一个发散的转录单位,该基因在某些但不是全部抗甲氨蝶呤的细胞系中与dhfr共扩增。我们显示该基因对的启动子区域由两个双向启动子,主要和次要启动子,位于dhfr ATG翻译起始密码子上游的660个碱基对区域内。主要启动子控制着超过90%的dhfr转录,而次要启动子则控制着其余dhfr mRNA的转录。主要启动子双向起作用,以与dhfr转录相反的方向转录不同的4.0碱基碱基的poly(A)mRNA(A类)。该mRNA的预测蛋白质产物为105千道尔顿。次要启动子还具有双向功能,指导至少两个不同的RNA(B类)的转录。这些RNA的数量约为A类mRNA的1/10至1/50,分别是4.4和1.6碱基碱基的poly(A)mRNA。已经从扩增dhfr基因座(3T3R500)的小鼠成纤维细胞系中克隆了代表A类和B类mRNA的cDNA。这些cDNA的DNA序列分析表明,A类和B类mRNA在很大程度上共享相同的外显子。根据几种小鼠组织中RNA制剂的S1核酸酶保护分析,dhfr和发散基因均显示相似的表达水平,但在起始位点利用中确实显示出某些特异性。计算机同源性搜索已经揭示了差异转录物与参与DNA错配修复的细菌基因的序列相似性,因此我们将其命名为差异转录基因Rep-1。

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