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RNAseq-based Transcriptome Analysis of Burkholderia glumae Quorum Sensing

机译:伯克霍尔德氏菌群体感应的基于RNAseq的转录组分析

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摘要

Burkholderia glumae causes rice grain rot and sheath rot by producing toxoflavin, the expression of which is regulated by quorum sensing (QS). The QS systems of B. glumae rely on N-octanoyl homoserine lactone, synthesized by TofI and its cognate receptor TofR, to activate the genes for toxoflavin biosynthesis and an IclR-type transcriptional regulator gene, qsmR. To understand genome-wide transcriptional profiling of QS signaling, we employed RNAseq of the wild-type B. glumae BGR1 with QS-defective mutant, BGS2 (BGR1 tofI::Ω) and QS-dependent transcriptional regulator mutant, BGS9 (BGR1 qsmR::Ω). A comparison of gene expression profiling among the wild-type BGR1 and the two mutants before and after QS onset as well as gene ontology (GO) enrichment analysis from differential expressed genes (DEGs) revealed that genes involved in motility were highly enriched in TofI-dependent DEGs, whereas genes for transport and DNA polymerase were highly enriched in QsmR-dependent DEGs. Further, a combination of pathways with these DEGs and phenotype analysis of mutants pointed to a couple of metabolic processes, which are dependent on QS in B. glumae, that were directly or indirectly related with bacterial motility. The consistency of observed bacterial phenotypes with GOs or metabolic pathways in QS-regulated genes implied that integration RNAseq with GO enrichment or pathways would be useful to study bacterial physiology and phenotypes.
机译:伯克霍尔德氏菌通过产生毒素黄素而导致水稻粒腐烂和鞘腐烂,其表达受群体感应(QS)调节。豆腐双歧杆菌的QS系统依赖于由TofI及其同源受体TofR合成的N-辛酰基高丝氨酸内酯来激活毒素黄素生物合成的基因和IclR型转录调节基因qsmR。为了了解QS信号的全基因组转录谱,我们使用了野生型芽孢杆菌BGR1的RNAseq,其具有QS缺陷型突变体BGS2(BGR1 tofI ::Ω)和QS依赖性转录调节子突变体BGS9(BGR1 qsmR: :Ω)。比较QS发作前后野生型BGR1与两个突变体之间的基因表达谱以及对差异表达基因(DEG)进行的基因本体(GO)富集分析,发现与运动有关的基因在TofI-中高度富集依赖的DEG,而运输和DNA聚合酶的基因高度依赖QsmR依赖的DEG。此外,具有这些DEG的途径和突变体的表型分析的组合指出了依赖于小球藻中QS的几个代谢过程,这些代谢过程直接或间接地与细菌运动相关。 QS调控基因中观察到的细菌表型与GO或代谢途径的一致性暗示,RNAseq与GO富集或途径的整合将对研究细菌生理学和表型有用。

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