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酵母中人工核糖体RNA基因的转录

Transcription of an artificial ribosomal RNA gene in yeast.

作者信息

Kempers-Veenstra A E, van Heerikhuizen H, Musters W, Klootwijk J, Planta R J

出版信息

EMBO J. 1984 Jun;3(6):1377-82. doi: 10.1002/j.1460-2075.1984.tb01980.x.

Abstract

We constructed an artificial yeast rRNA gene and studied its transcription after introduction into a recipient yeast strain. The artificial gene comprised a fragment containing the sequence from position -207 to +128 relative to the site of initiation of Saccharomyces carlsbergensis 37S pre-rRNA, followed by a marker fragment from Spirodela oligorhiza chloroplast DNA and finally a fragment containing the sequence from position -36 to +101 relative to the 3' end of the 26S rRNA gene. The resulting construct was cloned into the yeast-Escherichia coli shuttle vector pJDB207. Both Northern blot hybridization and R-loop analysis of RNA from transformed Saccharomyces cerevisiae cells revealed a discrete transcript of the expected length. S1 nuclease mapping as well as primer extension analysis showed that the major proportion of the transcripts was initiated at exactly the same site as 37S pre-rRNA. These results show that the respective rDNA fragments contain the information for correct initiation of transcription and formation of the 3' end. A minor proportion of the transcripts was initiated at a number of sites between positions -1 and -100 upstream of the predominant start. The proportion and the pattern of these upstream starts is affected by the vector context of the artificial rRNA gene.

摘要

我们构建了一个人工酵母rRNA基因,并将其导入受体酵母菌株后研究其转录情况。该人工基因包含一个片段,其包含相对于卡尔酵母37S前体rRNA起始位点从-207至+128位置的序列,接着是来自少根紫萍叶绿体DNA的标记片段,最后是一个包含相对于26S rRNA基因3'末端从-36至+101位置序列的片段。将所得构建体克隆到酵母-大肠杆菌穿梭载体pJDB207中。对转化的酿酒酵母细胞的RNA进行Northern印迹杂交和R环分析,均揭示了预期长度的离散转录本。S1核酸酶图谱分析以及引物延伸分析表明,转录本的主要部分在与37S前体rRNA完全相同的位点起始。这些结果表明,各个rDNA片段包含转录正确起始和3'末端形成的信息。一小部分转录本在主要起始位点上游-1至-100位置之间的多个位点起始。这些上游起始的比例和模式受人工rRNA基因载体背景的影响。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d45d/557526/1067ae3bc69c/emboj00310-0162-a.jpg

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