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Activation of the Promoter of the Fengycin Synthetase Operon by the UP Element

机译:UP元件激活凤霉素合成酶操纵子的启动子

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摘要

Bacillus subtilis F29-3 produces an antifungal peptidic antibiotic that is synthesized nonribosomally by fengycin synthetases. Our previous work established that the promoter of the fengycin synthetase operon is located 86 nucleotides upstream of the translational initiation codon of fenC. This investigation involved transcriptional fusions with a DNA fragment that contains the region between positions −105 and +80 and determined that deleting the region between positions −55 and −42 reduces the promoter activity by 64.5%. Transcriptional fusions in the B. subtilis DB2 chromosome also indicated that mutating the sequence markedly reduces the promoter activity. An in vitro transcription analysis confirmed that the transcription is inefficient when the sequence in this region is mutated. Electrophoretic mobility shift and footprinting analyses demonstrated that the C-terminal domain of the RNA polymerase α subunit binds to the region between positions −55 and −39. These results indicated that the sequence is an UP element. Finally, this UP element is critical for the production of fengycin, since mutating the UP sequence in the chromosome of B. subtilis F29-3 reduces the transcription of the fen operon by 85% and prevents the cells from producing enough fengycin to suppress the germination of Paecilomyces variotii spores on agar plates.
机译:枯草芽孢杆菌F29-3产生抗真菌肽类抗生素,它由丰霉素合成酶非核糖体合成。我们先前的工作确定了丰霉素合成酶操纵子的启动子位于fenC翻译起始密码子上游的86个核苷酸处。这项研究涉及与DNA片段的转录融合,该片段包含-105和+80位之间的区域,并确定删除位置-55和-42位之间的区域会使启动子活性降低64.5%。枯草芽孢杆菌DB2染色体中的转录融合还表明,突变序列会显着降低启动子活性。体外转录分析证实,当该区域中的序列发生突变时,转录效率低下。电泳迁移率迁移和足迹分析表明,RNA聚合酶α亚基的C末端结构域与位置-55和-39之间的区域结合。这些结果表明该序列是UP元件。最后,此UP元件对于生产丰霉素至关重要,因为突变枯草芽孢杆菌F29-3染色体中的UP序列可使fen操纵子的转录降低85%,并阻止细胞产生足够的丰霉素以抑制发芽。琼脂平板上的天花拟青霉孢子。

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