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小鼠组蛋白基因的表达:转录进入3'基因间DNA以及H3基因3'端下游的隐蔽加工位点。

Expression of mouse histone genes: transcription into 3' intergenic DNA and cryptic processing sites downstream from the 3' end of the H3 gene.

作者信息

Chodchoy N, Levine B J, Sprecher C, Skoultchi A I, Marzluff W F

出版信息

Mol Cell Biol. 1987 Mar;7(3):1039-47. doi: 10.1128/mcb.7.3.1039-1047.1987.

Abstract

Introduction of the mouse histone H3.1 gene into tk- mouse L cells by cotransfection with the herpesvirus thymidine kinase gene resulted in the production of two mRNAs from the transfected gene, one with a normal 3' end and the other one with a longer 3'-untranslated region, ending at site X, which was poly(A)+. In contrast, the endogenous histone H3.1 gene only produced a single mRNA. The cryptic poly(A)+ site was only used when the histone H3.1 gene was transfected. To localize possible downstream cryptic processing sites, the hairpin loop at the end of the histone gene was deleted and the resulting deletions were introduced into L cells. Two major mRNAs were produced from this gene, one ending at site X and the major one ending at site Y, which was located 150 nucleotides before site X. Transcription extended downstream of site X efficiently in the endogenous gene, as judged by the extent of transcription of downstream sequences in isolated nuclei. Transcription extended downstream of site X in the transfected gene because the placement of a normal histone 3' end downstream of site X resulted in transcripts that ended at site X and longer transcripts that ended with the new histone 3' end. These results indicate that transcription may normally proceed a substantial distance past the hairpin loop (greater than 500 bases). The formation of the different 3' ends in these transfected genes was due to competition between different processing mechanisms.

摘要

通过与疱疹病毒胸苷激酶基因共转染,将小鼠组蛋白H3.1基因导入tk-小鼠L细胞,结果转染基因产生了两种mRNA,一种具有正常的3'末端,另一种具有更长的3'-非翻译区,在X位点终止,该位点是poly(A)+。相比之下,内源性组蛋白H3.1基因只产生一种mRNA。只有在转染组蛋白H3.1基因时,隐蔽的poly(A)+位点才会被使用。为了定位可能的下游隐蔽加工位点,删除了组蛋白基因末端的发夹环,并将产生的缺失片段导入L细胞。该基因产生了两种主要的mRNA,一种在X位点终止,主要的一种在Y位点终止,Y位点位于X位点之前150个核苷酸处。根据分离细胞核中下游序列的转录程度判断,内源性基因的转录有效地延伸到了X位点下游。转染基因的转录也延伸到了X位点下游,因为在X位点下游放置正常的组蛋白3'末端会导致转录本在X位点终止,以及以新的组蛋白3'末端终止的更长的转录本。这些结果表明,转录通常可能会在发夹环之后继续进行相当长的距离(超过500个碱基)。这些转染基因中不同3'末端的形成是由于不同加工机制之间的竞争。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3d67/365174/bc7ee88e807f/molcellb00075-0087-a.jpg

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