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枯草芽孢杆菌质粒pBD64的转录及克隆于其中的噬菌体SPO1基因的表达。

Transcription of Bacillis subtilis plasmid pBD64 and expression of bacteriophage SPO1 genes cloned therein.

作者信息

Curran J F, Stewart C R

出版信息

Virology. 1985 Apr 15;142(1):98-111. doi: 10.1016/0042-6822(85)90425-8.

Abstract

Plasmid pBD64, a vector which is useful for cloning in Bacillis subtilis (T. J. Gryczan, A. G. Shivakumar, and D. Dubnau (1980), J. Bacteriol. 141, 246-253), has at least three substantial transcription units. Two of these include the single EcoRI, XbaI, and BamHI sites, while the other includes the single BglII site. Each of these transcripts was synthesized in the counterclockwise direction, relative to the pBD64 restriction map. No transcripts were detected in the opposite direction. Infection by bacteriophage SPO1 caused a substantial decrease in each of these transcripts. No new pBD64 transcripts were detected during SPO1 infection. Various SPO1 genes, cloned at several of these pBD64 sites, were tested for expression by observing their capacity to complement SPO1 mutants. Several middle and late genes were expressed substantially, regardless of the orientation in which the fragments were inserted. Since transcription from the vector could cause expression only in one orientation, this argues that the necessary transcription originated at SPO1 promoters, and, thus, that SPO1 middle and late promoters can be active in thymine-containing DNA.

摘要

质粒pBD64是一种可用于在枯草芽孢杆菌中克隆的载体(T. J. 格里灿、A. G. 希瓦库马尔和D. 杜布瑙(1980年),《细菌学杂志》141卷,246 - 253页),它至少有三个主要转录单元。其中两个包含单一的EcoRI、XbaI和BamHI位点,另一个包含单一的BglII位点。相对于pBD64限制酶切图谱,这些转录本中的每一个都是沿逆时针方向合成的。未检测到相反方向的转录本。噬菌体SPO1感染导致这些转录本中的每一个都大幅减少。在SPO1感染期间未检测到新的pBD64转录本。通过观察克隆在这些pBD64位点中的几个位点上的各种SPO1基因互补SPO1突变体的能力来测试它们的表达情况。几个中期和晚期基因大量表达,无论片段插入的方向如何。由于来自载体的转录仅能在一个方向上导致表达,这表明必要的转录起源于SPO1启动子,因此,SPO1中期和晚期启动子在含胸腺嘧啶的DNA中可以是活跃的。

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Cloning and mapping of the SPO1 genome.SPO1基因组的克隆与定位
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Bacteriophage SPO1 middle transcripts.噬菌体SPO1中期转录本
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The genome of Bacillus subtilis bacteriophage SPO1.枯草芽孢杆菌噬菌体SPO1的基因组。
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