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Two Phenotype-Differentiated Acinetobacter baumannii Mutants That Survived in a Meropenem Selection Display Large Differences in Their Transcription Profiles

机译:在美罗培南选择中幸存的两个表型不同鲍曼不动杆菌突变体在其转录谱中显示出很大的差异。

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摘要

37662RM1 and 37662RM2 are two phenotypically different, carbapenem-resistant mutants of Acinetobacter baumannii 37662 isolate following selection with meropenem (MEM) at sub-inhibitory concentrations. 37662RM2 lacks capsule synthesis and shows dramatically increased biofilm formation, while 37662RM1 shows merely impaired capsule synthesis. Here we report that 37662RM1 and RM2 have transcription profiles that are different from those of their starting strain, 37662WT. There were far more differentially expressed genes in 37662RM2 than in 37662RM1. The capsule polysaccharide (CPS) synthesis-required genes (itrA2, gtr5, psaA, psaB, psaC, psaD, psaE, psaF, kpsS2, wzx, wzy, wza, wzb, and wzc) showed reduced transcription levels in 37662RM2, which may at least partially explain the loss of capsule synthesis. The csu operon genes responsible for pili assembly and their regulator genes bfmR-bfmS were over-expressed in 37662RM2. This result together with the established critical roles of these genes in biofilm formation provide solid evidence that up-regulation of csu and bfmR-bfmS should be considered responsible for the enhanced biofilm formation in 37662RM2. ISAba1 was found to insert into the intergenic region between the csu operon and the acrR gene and should be responsible for the significant up-regulation of acrR, which was proposed to be associated with biofilm formation. Genome sequencing revealed that the ISAba1 upstream blaOXA–508 (a new member of blaOXA–51-like) and acrR were duplicated, suggesting a replicative transposition event. Altogether, the phenotype divergence driven by MEM selection mainly occurs at the RNA level and the transposition of ISAba1 plays an important role in modulating gene expression to adapt to the environment.
机译:37662RM1和37662RM2是鲍曼不动杆菌37662分离株的两个表型不同,对碳青霉烯耐药的突变株,在亚抑制浓度下用美罗培南(MEM)选择后。 37662RM1缺乏胶囊合成,并且生物膜形成显着增加,而37662RM1仅显示胶囊合成受损。在这里,我们报告37662RM1和RM2具有不同于其起始菌株37662WT的转录谱。 37662RM2中的差异表达基因远多于37662RM1。胶囊多糖(CPS)合成所需的基因(itrA2,gtr5,psaA,psaB,psaC,psaD,psaE,psaF,kpsS2,wzx,wzy,wza,wzab,wzb和wzc)显示的转录水平降低了37662RM2,可能在至少部分解释了胶囊合成的损失。负责菌毛组装的csu操纵子基因及其调节基因bfmR- bfmS 在37662RM2中过表达。该结果以及这些基因在生物膜形成中已确立的关键作用提供了有力的证据,表明应 csu bfmR - bfmS 的上调被认为是造成37662RM2生物膜形成增强的原因。 IS Aba 1被发现插入 csu 操纵子和 acrR 基因之间的基因间区域,并应负责显着上调被认为与生物膜形成有关的 acrR 。基因组测序表明,IS Aba 1上游 bla OXA–508( bla OXA–51的新成员)和复制了acrR ,表明存在复制性转座事件。总之,由MEM选择驱动的表型差异主要发生在RNA水平,IS Aba 1的转座在调节基因表达以适应环境中起重要作用。

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