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spo0B基因座的序列分析揭示了一个多顺反子转录单元。

Sequence analysis of the spo0B locus reveals a polycistronic transcription unit.

作者信息

Ferrari F A, Trach K, Hoch J A

出版信息

J Bacteriol. 1985 Feb;161(2):556-62. doi: 10.1128/jb.161.2.556-562.1985.

Abstract

A 2.3-kilobase pair EcoRI fragment containing the spo0B locus has been sequenced. The spo0B locus was shown to code for a protein of 22,542 daltons. Promoter distal to the spo0B locus, an open reading frame was uncovered which was preceded by a strong ribosome-binding site. S1 nuclease protection experiments revealed that both the spo0B locus and this open reading frame were part of the same transcript. A portion of the middle of the open reading frame was cloned in the integrative vector pJH101. Transformation of this plasmid into Bacillus subtilis 168 was only rarely successful, and those few colonies that arose consisted of cells that had lost the plasmid. The results suggested that the product of this open reading frame is essential for the growth of the bacterium. The regulation of the spo0B locus was studied by using translational spo0B-lacZ fusions in an integrative vector. These studies revealed that the spo0B locus was maximally expressed during vegetative growth. It was estimated that 50 to 100 copies of the protein are present during this period. Sequence analysis of the region upstream from the spo0B locus revealed another operon that contained a gene coding for a protein homologous to ribosomal protein L27 of Escherichia coli.

摘要

一个包含spo0B基因座的2.3千碱基对的EcoRI片段已被测序。结果显示,spo0B基因座编码一种分子量为22,542道尔顿的蛋白质。在spo0B基因座的启动子远端,发现了一个开放阅读框,其前面有一个很强的核糖体结合位点。S1核酸酶保护实验表明,spo0B基因座和这个开放阅读框都是同一转录本的一部分。开放阅读框中间的一部分被克隆到整合载体pJH101中。将该质粒转化到枯草芽孢杆菌168中很少成功,出现的少数菌落由丢失了质粒的细胞组成。结果表明,这个开放阅读框的产物对细菌的生长至关重要。通过在整合载体中使用翻译性spo0B-lacZ融合体来研究spo0B基因座的调控。这些研究表明,spo0B基因座在营养生长期间表达量最高。据估计,在此期间该蛋白质有50到100个拷贝。对spo0B基因座上游区域的序列分析揭示了另一个操纵子,其中包含一个编码与大肠杆菌核糖体蛋白L27同源的蛋白质的基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9ce5/214918/d30db50a37df/jbacter00225-0095-a.jpg

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