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Binding Sequences for RdgB, a DNA Damage-Responsive Transcriptional Activator, and Temperature-Dependent Expression of Bacteriocin and Pectin Lyase Genes in Pectobacterium carotovorum subsp. carotovorum▿ †

机译:绑定序列RdgB,一种DNA损伤响应转录激活剂,和细菌果胶杆菌亚种中细菌素和果胶裂解酶基因的温度依赖性表达。胡萝卜vor

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摘要

Pectobacterium carotovorum subsp. carotovorum strain Er simultaneously produces the phage tail-like bacteriocin carotovoricin (Ctv) and pectin lyase (Pnl) in response to DNA-damaging agents. The regulatory protein RdgB of the Mor/C family of proteins activates transcription of pnl through binding to the promoter. However, the optimal temperature for the synthesis of Ctv (23°C) differs from that for synthesis of Pnl (30°C), raising the question of whether RdgB directly activates ctv transcription. Here we report that RdgB directly regulates Ctv synthesis. Gel mobility shift assays demonstrated RdgB binding to the P0, P1, and P2 promoters of the ctv operons, and DNase I footprinting determined RdgB-binding sequences (RdgB boxes) on these and on the pnl promoters. The RdgB box of the pnl promoter included a perfect 7-bp inverted repeat with high binding affinity to the regulator (Kd [dissociation constant] = 150 nM). In contrast, RdgB boxes of the ctv promoters contained an imperfect inverted repeat with two or three mismatches that consequently reduced binding affinity (Kd = 250 to 350 nM). Transcription of the rdgB and ctv genes was about doubled at 23°C compared with that at 30°C. In contrast, the amount of pnl transcription tripled at 30°C. Thus, the inverse synthesis of Ctv and Pnl as a function of temperature is apparently controlled at the transcriptional level, and reduced rdgB expression at 30°C obviously affected transcription from the ctv promoters with low-affinity RdgB boxes. Pathogenicity toward potato tubers was reduced in an rdgB knockout mutant, suggesting that the RdgAB system contributes to the pathogenicity of this bacterium, probably by activating pnl expression.
机译:胡萝卜杆菌假单胞菌亚种。胡萝卜噬菌体菌株Er响应DNA破坏剂,同时产生噬菌体尾状细菌素胡萝卜素(Ctv)和果胶裂解酶(Pnl)。 Mor / C蛋白家族的调节蛋白RdgB通过与启动子结合来激活pnl的转录。但是,合成Ctv的最佳温度(23°C)与合成Pnl的最佳温度(30°C)不同,这引发了RdgB是否直接激活ctv转录的问题。在这里,我们报告RdgB直接调节Ctv合成。凝胶迁移率迁移分析证明了RdgB与ctv操纵子的P0,P1和P2启动子结合,并且DNase I足迹确定了这些和pnl启动子上的RdgB结合序列(RdgB框)。 pnl启动子的RdgB盒包含一个完美的7 bp反向重复序列,对调节剂具有很高的结合亲和力(Kd [解离常数] = 150 nM)。相反,ctv启动子的RdgB框包含不完全的反向重复序列,具有两个或三个错配,从而降低了结合亲和力(Kd = 250至350 nM)。与30°C相比,rdgB和ctv基因的转录在23°C时大约翻了一番。相反,在30℃下pnl转录的量增加了两倍。因此,Ctv和Pnl的逆合成与温度的关系显然在转录水平上受到控制,而rdgB表达在30°C降低明显影响了具有低亲和力RdgB盒的ctv启动子的转录。在rdgB基因敲除突变体中,马铃薯块茎的致病性降低,这表明RdgAB系统可能通过激活pnl表达而促进了这种细菌的致病性。

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