抑制Phaeobacter inhibens DSM 17395对其262-kb编码抗生素合成的染色质缺失的全局响应

IF 0.1 4区 生物学 Q2 BIOTECHNOLOGY & APPLIED MICROBIOLOGY Microbial Physiology Pub Date : 2020-01-01 Epub Date: 2020-07-24 DOI:10.1159/000508591
Daniel Wünsch, Annemieke Strijkstra, Lars Wöhlbrand, Heike M Freese, Sabine Scheve, Christina Hinrichs, Kathleen Trautwein, Michael Maczka, Jörn Petersen, Stefan Schulz, Jörg Overmann, Ralf Rabus
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引用次数: 9

摘要

海洋alphaproteobacterium Phaeobacter inhibens DSM 17395是Roseobacter家族的一员,最近的研究表明,在删除其262 kb的编码tropodithitic acid (TDA)生物合成的染色质后,它可以显著促进生长。为了仔细研究Δ262突变体生长增强背后的代谢/调节适应,我们在以Casamino Acids为生长底物的过程控制生物反应器中研究了其与野生型相比的转录组和蛋白质组。基因组重测序显示,野生型和Δ262突变型之间只有少数额外的遗传变化(异源插入、噬菌体激活和几个点突变),尽管对所研究的生长生理没有可能的影响。研究发现,参与底物完全氧化为CO2的分解代谢网络的绝大多数转录物和蛋白质的丰度没有变化,这表明Δ262突变体对氨基酸的利用增强并不需要提高分解代谢网络中大多数酶的合成。同样,遗传信息处理和细胞过程的成分基本保持不变。相比之下,426个基因表现出差异表达,其中410个定位在3.2 mb染色体上,5个定位在65kb染色体上,11个定位在78kb染色体上。值得注意的是,作用于快速利用的Val、Ile和Leu的支链氨基转移酶IlvE上调。此外,从氨基酸和无机营养物(如磷酸盐)的几种摄取系统的转录本和蛋白质的丰度增加可以证明,转运体被重新配置。呼吸链的一些成分也被上调,这与Δ262突变体更高的呼吸速率有关。此外,在Δ262突变体中,与TDA生物合成相关的染色体编码转录物和蛋白质(例如,丝氨酸酰基转移酶CysE)被强烈下调。综上所述,这些观察结果反映了P. inhibens DSM 17395复制子对增强生长的适应性以及功能互联性。
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Global Response of Phaeobacter inhibens DSM 17395 to Deletion of Its 262-kb Chromid Encoding Antibiotic Synthesis.

The marine alphaproteobacterium Phaeobacter inhibens DSM 17395, a member of the Roseobacter group, was recently shown to markedly enhance growth upon deletion of its 262-kb chromid encoding biosynthesis of tropodithietic acid (TDA). To scrutinize the metabolic/regulatory adaptations that underlie enhanced growth of the Δ262 mutant, its transcriptome and proteome compared to the wild type were investigated in process-controlled bioreactors with Casamino Acids as growth substrate. Genome resequencing revealed only few additional genetic changes (a heterogenic insertion, prophage activation, and several point mutations) between wild type and Δ262 mutant, albeit with no conceivable effect on the studied growth physiology. The abundances of the vast majority of transcripts and proteins involved in the catabolic network for complete substrate oxidation to CO2 were found to be unchanged, suggesting that the enhanced amino acid utilization of the Δ262 mutant did not require elevated synthesis of most enzymes of the catabolic network. Similarly, constituents of genetic information processing and cellular processes remained mostly unchanged. In contrast, 426 genes displayed differential expression, of which 410 were localized on the 3.2-Mb chromosome, 5 on the 65-kb chromid, and 11 on the 78-kb chromid. Notably, the branched-chain amino transferase IlvE acting on rapidly utilized Val, Ile, and Leu was upregulated. Moreover, the transportome was reconfigured, as evidenced from increased abundances of transcripts and proteins of several uptake systems for amino acids and inorganic nutrients (e.g., phosphate). Some components of the respiratory chain were also upregulated, which correlates with the higher respiration rates of the Δ262 mutant. Furthermore, chromosomally encoded transcripts and proteins that are peripherally related to TDA biosynthesis (e.g., the serine acyl transferase CysE) were strongly downregulated in the Δ262 mutant. Taken together, these observations reflect adaptations to enhanced growth as well as the functional interconnectivity of the replicons of P. inhibens DSM 17395.

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