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Phylogenetically Novel LuxI/LuxR-Type Quorum Sensing Systems Isolated Using a Metagenomic Approach

机译:系统发育的新型LuxI / LuxR型群体感应系统,使用超基因组学方法进行分离

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A great deal of research has been done to understand bacterial cell-to-cell signaling systems, but there is still a large gap in our current knowledge because the majority of microorganisms in natural environments do not have cultivated representatives. Metagenomics is one approach to identify novel quorum sensing (QS) systems from uncultured bacteria in environmental samples. In this study, fosmid metagenomic libraries were constructed from a forest soil and an activated sludge from a coke plant, and the target genes were detected using a green fluorescent protein (GFP)-based Escherichia coli biosensor strain whose fluorescence was screened by spectrophotometry. DNA sequence analysis revealed two pairs of new LuxI family N-acyl-l-homoserine lactone (AHL) synthases and LuxR family transcriptional regulators (clones N16 and N52, designated AubI/AubR and AusI/AusR, respectively). AubI and AusI each produced an identical AHL, N-dodecanoyl-l-homoserine lactone (C12-HSL), as determined by nuclear magnetic resonance (NMR) and mass spectrometry. Phylogenetic analysis based on amino acid sequences suggested that AusI/AusR was from an uncultured member of the Betaproteobacteria and AubI/AubR was very deeply branched from previously described LuxI/LuxR homologues in isolates of the Proteobacteria. The phylogenetic position of AubI/AubR indicates that they represent a QS system not acquired recently from the Proteobacteria by horizontal gene transfer but share a more ancient ancestry. We demonstrated that metagenomic screening is useful to provide further insight into the phylogenetic diversity of bacterial QS systems by describing two new LuxI/LuxR-type QS systems from uncultured bacteria.
机译:为了理解细菌细胞间信号系统,已经进行了大量研究,但是由于自然环境中的大多数微生物都没有培养出代表性的细菌,因此我们目前的知识仍然存在很大差距。元基因组学是一种从环境样品中的未培养细菌中识别新型群体感应(QS)系统的方法。在这项研究中,由森林土壤和焦炭植物产生的活性污泥构建了fosmid宏基因组库,并使用基于绿色荧光蛋白(GFP)的大肠杆菌生物传感器菌株检测了目标基因,该菌株通过分光光度法进行了荧光筛选。 DNA序列分析揭示了两对新的LuxI家族N-酰基-1-高丝氨酸内酯(AHL)合酶和LuxR家族转录调节子(克隆N16和N52,分别命名为AubI / AubR和AusI / AusR)。通过核磁共振(NMR)和质谱法测定,AubI和AusI各自产生相同的AHL,N-十二烷酰基-1-高丝氨酸内酯(C12-HSL)。基于氨基酸序列的系统发育分析表明,AusI / AusR来自β变形杆菌的未培养成员,而AubI / AubR与先前描述的LuxI / LuxR同源蛋白在蛋白酶分离物中的分支非常深。 AubI / AubR的系统发育位置表明它们代表的QS系统不是最近通过水平基因转移从Proteobacteria获得的,但具有更古老的血统。我们通过描述来自未培养细菌的两个新的LuxI / LuxR型QS系统,证明了宏基因组学筛选可用于进一步深入了解细菌QS系统的系统发育多样性。

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