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Upregulated Transcription of Plasmid and Chromosomal Ribulose Monophosphate Pathway Genes Is Critical for Methanol Assimilation Rate and Methanol Tolerance in the Methylotrophic Bacterium Bacillus methanolicus

机译:质粒和染色体核糖单磷酸通路基因的上调转录对于甲基营养细菌甲醇芽孢杆菌的甲醇吸收速率和甲醇耐受性至关重要

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摘要

The natural plasmid pBM19 carries the key mdh gene needed for the oxidation of methanol into formaldehyde by Bacillus methanolicus. Five more genes, glpX, fba, tkt, pfk, and rpe, with deduced roles in the cell primary metabolism, are also located on this plasmid. By using real-time PCR, we show that they are transcriptionally upregulated (6- to 40-fold) in cells utilizing methanol; a similar induction was shown for two chromosomal genes, hps and phi. These seven genes are involved in the fructose bisphosphate aldolase/sedoheptulose bisphosphatase variant of the ribulose monophosphate (RuMP) pathway for formaldehyde assimilation. Curing of pBM19 causes higher methanol tolerance and reduced formaldehyde tolerance, and the methanol tolerance is reversed to wild-type levels by reintroducing mdh. Thus, the RuMP pathway is needed to detoxify the formaldehyde produced by the methanol dehydrogenase-mediated conversion of methanol, and the in vivo transcription levels of mdh and the RuMP pathway genes reflect the methanol tolerance level of the cells. The transcriptional inducer of hps and phi genes is formaldehyde, and not methanol, and introduction of multiple copies of these two genes into B. methanolicus made the cells more tolerant of growth on high methanol concentrations. The recombinant strain also had a significantly higher specific growth rate on methanol than the wild type. While pBM19 is critical for growth on methanol and important for formaldehyde detoxification, the maintenance of this plasmid represents a burden for B. methanolicus when growing on mannitol. Our data contribute to a new and fundamental understanding of the regulation of B. methanolicus methylotrophy.
机译:天然质粒pBM19携带了甲醇芽孢杆菌将甲醇氧化成甲醛所需的关键mdh基因。在该质粒上还定位了在细胞初级代谢中具有推论作用的另外五个基因glpX,fba,tkt,pfk和rpe。通过使用实时PCR,我们显示它们在利用甲醇的细胞中被转录上调(6至40倍)。对两个染色体基因hps和phi显示了相似的诱导。这七个基因参与了果糖二磷酸醛缩酶(RuMP)途径中的果糖二磷酸醛缩醛醛缩酶/七羟庚二糖双磷酸酶变体,以甲醛同化。 pBM19的固化导致更高的甲醇耐受性和降低的甲醛耐受性,并且通过重新引入mdh将甲醇耐受性逆转至野生型水平。因此,需要RuMP途径来解毒由甲醇脱氢酶介导的甲醇转化所产生的甲醛,并且mdh和RuMP途径基因的体内转录水平反映了细胞的甲醇耐受水平。 hps和phi基因的转录诱导物是甲醛,而不是甲醇,并且将这两个基因的多个拷贝引入甲醇双歧杆菌使细胞在高甲醇浓度下更能耐受生长。重组菌株在甲醇上的比生长速率也明显高于野生型。虽然pBM19对在甲醇上生长至关重要,对甲醛解毒也很重要,但当在甘露醇上生长时,该质粒的维持代表了甲醇芽孢杆菌的负担。我们的数据有助于对甲醇芽孢杆菌甲基营养的调节有了新的基础性认识。

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