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肺炎支原体rRNA操纵子的转录控制元件。

Transcription control elements of the Mycoplasma pneumoniae rRNA operon.

作者信息

Hyman H C, Gafny R, Glaser G, Razin S

机构信息

Department of Membrane and Ultrastructure Research, Hebrew University, Hadassah Medical School, Jerusalem, Israel.

出版信息

Isr J Med Sci. 1987 Jun;23(6):585-90.

PMID:2444563
Abstract

The single RNA operon of Mycoplasma pneumoniae was cloned into a lambda vector and subcloned into pBR322. This was carried out in order to enable the analysis of the transcription control regions of this operon. S1 nuclease mapping was used to locate the 5' ends of RNA transcripts synthesized from the operon. The 5' ends of the 23S, 16S, and a precursor RNA synthesized in vivo in M. pneumoniae were mapped on the DNA template. Preliminary in vitro transcription experiments using RNA polymerase of Escherichia coli led to the conclusion that E. coli recognizes one promoter in the 5' region of the M. pneumoniae rRNA operon. The startsite of the in vitro transcript seems to lie downstream from the 5' end of the M. pneumoniae precursor transcript. Preliminary sequencing of the 5' regions of the M. pneumoniae rRNA operon and of the M. capricolum rRNA B operon enabled their comparison to each other and to known sequences from other organisms.

摘要

肺炎支原体的单一RNA操纵子被克隆到一个λ载体中,然后亚克隆到pBR322中。这样做是为了能够分析该操纵子的转录控制区域。使用S1核酸酶图谱法来定位从该操纵子合成的RNA转录本的5'末端。在肺炎支原体体内合成的23S、16S和前体RNA的5'末端在DNA模板上进行了定位。使用大肠杆菌RNA聚合酶进行的初步体外转录实验得出结论,大肠杆菌识别肺炎支原体rRNA操纵子5'区域中的一个启动子。体外转录本的起始位点似乎位于肺炎支原体前体转录本5'末端的下游。对肺炎支原体rRNA操纵子和山羊支原体rRNA B操纵子的5'区域进行的初步测序,使得它们能够相互比较,并与来自其他生物体的已知序列进行比较。

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