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Distinct transcriptional regulation of the two Escherichia coli transhydrogenases PntAB and UdhA

机译:两种大肠杆菌转氢酶PntAB和UdhA的不同转录调控

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摘要

Transhydrogenases catalyse interconversion of the redox cofactors NADH and NADPH, thereby conveying metabolic flexibility to balance catabolic NADPH formation with anabolic or stress-based consumption of NADPH. Escherichia coli is one of the very few microbes that possesses two isoforms: the membrane-bound, proton-translocating transhydrogenase PntAB and the cytosolic, energy-independent transhydrogenase UdhA. Despite their physiological relevance, we have only fragmented information on their regulation and the signals coordinating their counteracting activities. Here we investigated PntAB and UdhA regulation by studying transcriptional responses to environmental and genetic perturbations. By testing pntAB and udhA GFP reporter constructs in the background of WT E. coli and 62 transcription factor mutants during growth on different carbon sources, we show distinct transcriptional regulation of the two transhydrogenase promoters. Surprisingly, transhydrogenase regulation was independent of the actual catabolic overproduction or underproduction of NADPH but responded to nutrient levels and growth rate in a fashion that matches the cellular need for the redox cofactors NADPH and/or NADH. Specifically, the identified transcription factors Lrp, ArgP and Crp link transhydrogenase expression to particular amino acids and intracellular concentrations of cAMP. The overall identified set of regulators establishes a primarily biosynthetic role for PntAB and link UdhA to respiration.
机译:转氢酶催化氧化还原辅助因子NADH和NADPH的相互转化,从而传达代谢灵活性,以平衡分解代谢NADPH的形成与合成代谢或基于压力的NADPH的消耗。大肠杆菌是具有两种同工型的极少数微生物之一:膜结合的质子易位转氢酶PntAB和胞质,能量独立的转氢酶UdhA。尽管它们具有生理相关性,但我们仅零碎地了解了它们的调控和协调其抵消活动的信号。在这里,我们通过研究对环境和遗传扰动的转录反应,研究了PntAB和UdhA的调控。通过在不同碳源上生长期间在野生型大肠杆菌和62个转录因子突变体的背景下测试pntAB和udhA GFP报告基因构建体,我们显示了两种转氢酶启动子的独特转录调控。出人意料的是,转氢酶的调节与NADPH的实际分解代谢的过量生产或生产不足无关,但以与细胞对氧化还原辅因子NADPH和/或NADH的需求相匹配的方式对营养水平和生长速率作出响应。具体而言,鉴定出的转录因子Lrp,ArgP和Crp将转氢酶的表达与特定氨基酸和cAMP的细胞内浓度联系起来。整体确定的调节剂组为PntAB建立了主要的生物合成作用,并将UdhA与呼吸联系起来。

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