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Integrated Transcriptional Regulatory Network of Quorum Sensing Replication Control and SOS Response in Dinoroseobacter shibae

机译:柴犬嗜藻菌群体感应复制控制和SOS反应的整合转录调控网络

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摘要

Quorum sensing (QS) coordinates population wide gene expression of bacterial species. Highly adaptive traits like gene transfer agents (GTA), morphological heterogeneity, type 4 secretion systems (T4SS), and flagella are QS controlled in Dinoroseobacter shibae, a Roseobacter model organism. Its QS regulatory network is integrated with the CtrA phosphorelay that controls cell division in alphaproteobacteria. To elucidate the network topology, we analyzed the transcriptional response of the QS-negative D. shibae strain ΔluxI1 toward externally added autoinducer (AI) over a time period of 3 h. The signaling cascade is initiated by the CtrA phosphorelay, followed by the QS genes and other target genes, including the second messenger c-di-GMP, competence, flagella and pili. Identification of transcription factor binding sites in promoters of QS induced genes revealed the integration of QS, CtrA phosphorelay and the SOS stress response mediated by LexA. The concentration of regulatory genes located close to the origin or terminus of replication suggests that gene regulation and replication are tightly coupled. Indeed, addition of AI first stimulates and then represses replication. The restart of replication comes along with increased c-di-GMP levels. We propose a model in which QS induces replication followed by differentiation into GTA producing and non-producing cells. CtrA-activity is controlled by the c-di-GMP level, allowing some of the daughter cells to replicate again. The size of the GTA producing subpopulation is tightly controlled by QS via the AI Synthase LuxI2. Finally, induction of the SOS response allows for integration of GTA DNA into the host chromosome.
机译:群体感应(QS)协调细菌物种的全基因表达。高度适应性状,例如基因转移剂(GTA),形态异质性,4型分泌系统(T4SS)和鞭毛,在玫瑰菌模型生物芝芝中得到QS控制。它的QS监管网络与CtrA磷灰质集成在一起,该CtrA磷灰质可控制alpha变形细菌中的细胞分裂。为了阐明网络拓扑,我们在3小时的时间内分析了QS阴性芝士菌株luxlux对外部添加的自诱导子(AI)的转录反应。信号级联反应由CtrA磷酸化启动,然后是QS基因和其他靶基因,包括第二信使c-di-GMP,能力,鞭毛和菌毛。 QS诱导基因启动子中转录因子结合位点的鉴定揭示了QS,CtrA磷酸化和LexA介导的SOS应激反应的整合。位于复制起点或终点附近的调节基因的浓度表明基因调节和复制紧密结合。确实,添加AI首先会刺激然后抑制复制。复制的重新启动伴随着c-di-GMP水平的提高。我们提出了一个模型,其中QS诱导复制,然后分化为GTA生产细胞和非生产细胞。 CtrA活性受c-di-GMP水平控制,允许某些子细胞再次复制。 QS通过AI合酶LuxI2严格控制产生GTA的亚群的大小。最后,SOS反应的诱导允许将GTA DNA整合到宿主染色体中。

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