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Distortion in the spacer region of Pm during activation of middle transcription of phage Mu.

机译:噬菌体Mu的中间转录激活过程中Pm间隔区中的扭曲。

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摘要

Transcription from the middle promoter, Pm, of phage Mu is initiated by Escherichia coli RNA polymerase holoenzyme (E sigma 70; RNAP) and the phage-encoded activator, Mor. Point mutations in the spacer region between the -10 hexamer and the Mor binding site result in changes of promoter activity in vivo. These mutations are located at the junction between a rigid T-tract and adjacent, potentially deformable G + C-rich DNA segment, suggesting that deformation of the spacer region may play a role in the transcriptional activation of Pm. This prediction was tested by using dimethyl sulfate and potassium permanganate footprinting analyses. Helical distortion involving strand separation was detected at positions -32 to -34, close to the predicted interface between Mor and RNAP. Promoter mutants in which this distortion was not detected exhibited a lack of melting in the -12 to -1 region and reduced promoter activity in vivo. We propose that complexes containing the distortion represent stressed intermediates rather than stable open complexes and thus can be envisaged as a transition state in the kinetic pathway of Pm activation in which stored torsional energy could be used to facilitate melting around the transcription start point.
机译:噬菌体Mu中间启动子Pm的转录是由大肠杆菌RNA聚合酶全酶(E sigma 70; RNAP)和噬菌体编码的激活剂Mor启动的。 -10六聚体和Mor结合位点之间的间隔区中的点突变导致体内启动子活性的变化。这些突变位于刚性T束和相邻的,可能变形的富含G + C的DNA片段之间的交界处,表明间隔区的变形可能在Pm的转录激活中起作用。通过使用硫酸二甲酯和高锰酸钾足迹分析法测试了这一预测。在靠近Mor和RNAP的预测界面的位置-32至-34处检测到涉及链分离的螺旋形扭曲。未检测到这种畸变的启动子突变体在-12至-1区域缺乏解链,并且体内启动子活性降低。我们建议,包含变形的复合物代表受应力的中间体,而不是稳定的开放复合物,因此可以设想为Pm活化动力学路径中的过渡态,其中存储的扭转能可用于促进转录起点周围的熔解。

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