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VSG基因118由一个共转座的类RNA聚合酶I启动子转录。

VSG gene 118 is transcribed from a cotransposed pol I-like promoter.

作者信息

Shea C, Lee M G, Van der Ploeg L H

出版信息

Cell. 1987 Aug 14;50(4):603-12. doi: 10.1016/0092-8674(87)90033-x.

Abstract

To understand the control of differential variant cell surface glycoprotein (VSG) gene expression in T. brucei, we studied VSG gene and expression site transcription regulation. We show that the interchromosomal duplicative transposition of VSG gene 118, on an unusually large transposed segment, results in the transcriptional activation of a cotransposed RNA polymerase I-like (pol I) promoter, from which the VSG gene is transcribed. Transcription of VSG genes by pol I can therefore be regulated by DNA rearrangements that affect positional control of gene expression. A 5' cap is added in trans to the pol I-derived pre-mRNA, by addition of a pol II-derived 35 nucleotide mini-exon. A second gene (ESAG1) is located 25 kb upstream of the VSG 118 gene and is also transcribed. This expression site therefore contains at least two independently regulated genes. We discuss the putative importance of a nucleolar location for VSG gene and expression site transcription regulation.

摘要

为了解布氏锥虫中差异可变细胞表面糖蛋白(VSG)基因表达的调控机制,我们研究了VSG基因和表达位点的转录调控。我们发现,VSG基因118在一个异常大的转座片段上进行染色体间重复转座,导致一个共转座的RNA聚合酶I样(pol I)启动子的转录激活,VSG基因由此启动转录。因此,pol I对VSG基因的转录可通过影响基因表达位置控制的DNA重排来调控。通过添加一个来自pol II的35个核苷酸的小外显子,5'帽被反式添加到pol I衍生的前体mRNA上。第二个基因(ESAG1)位于VSG 118基因上游25 kb处,也被转录。因此,这个表达位点至少包含两个独立调控的基因。我们讨论了核仁定位对于VSG基因和表达位点转录调控的假定重要性。

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