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Transcriptional Profiling of Methyltransferase Genes during Growth of Methanosarcina mazei on Trimethylamine

机译:三甲胺上甲烷甲烷八叠球菌生长过程中甲基转移酶基因的转录谱分析

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摘要

The genomic expression patterns of Methanosarcina mazei growing with trimethylamine were measured in comparison to those of cells grown with methanol. We identified a total of 72 genes with either an increased level (49 genes) or a decreased level (23 genes) of mRNA during growth on trimethylamine with methanol-grown cells as the control. Major differences in transcript levels were observed for the mta, mtb, mtt, and mtm genes, which encode enzymes involved in methane formation from methanol and trimethylamine, respectively. Other differences in mRNA abundance were found for genes encoding enzymes involved in isopentenyl pyrophosphate synthesis and in the formation of aromatic amino acids, as well as a number of proteins with unknown functions. The results were verified by in-depth analysis of methyltransferase genes using specific primers for real-time quantitative reverse transcription-PCR (RT-PCR). The monitored transcript levels of genes encoding corrinoid proteins involved in methyl group transfer from methylated C1 compounds (mtaC, mtbC, mttC, and mtmC) indicated increased amounts of mRNA from the mtaBC1, mtaBC2, and mtaBC3 operons in methanol-grown cells, whereas mRNA of the mtb1-mtt1 operon was found in high concentrations during trimethylamine consumption. The genes of the mtb1-mtt1 operon encode methyltransferases that are responsible for sequential demethylation of trimethylamine. The analysis of product formation of trimethylamine-grown cells at different optical densities revealed that large amounts of dimethylamine and monomethylamine were excreted into the medium. The intermediate compounds were consumed only in the very late exponential growth phase. RT-PCR analysis of key genes involved in methanogenesis led to the conclusion that M. mazei is able to adapt to changing trimethylamine concentrations and the consumption of intermediate compounds. Hence, we assume that the organism possesses a regulatory network for optimal substrate utilization.
机译:与用甲醇生长的细胞相比,测量了用三甲胺生长的马氏甲烷八叠球菌的基因组表达模式。我们确定了总共72个基因,其中以甲醇生长的细胞为对照,在三甲胺上生长期间,mRNA的水平升高(49个基因)或水平降低(23个基因)。分别在mta,mtb,mtt和mtm基因上观察到转录水平的主要差异,它们分别编码与甲醇和三甲胺形成甲烷有关的酶。在编码参与异戊烯基焦磷酸合成,芳香族氨基酸形成以及许多功能未知的蛋白质的酶的基因中,发现了mRNA丰度的其他差异。通过使用实时荧光定量逆转录PCR(RT-PCR)的特异性引物对甲基转移酶基因进行深入分析,验证了结果。监测从甲基化的C1化合物(mtaC,mtbC,mttC和mtmC)甲基转移涉及的编码类海藻蛋白的基因的转录水平监测表明,在甲醇生长的细胞中,来自mtaBC1,mtaBC2和mtaBC3操纵子的mRNA量增加了,而mRNA在三甲胺消耗期间发现高浓度的mtb1-mtt1操纵子。 mtb1-mtt1操纵子的基因编码负责三甲胺顺序去甲基化的甲基转移酶。对三甲胺生长的细胞在不同光密度下的产物形成的分析表明,大量的二甲胺和单甲胺被排泄到培养基中。中间体化合物仅在指数增长后期才被消耗。对参与甲烷生成的关键基因进行RT-PCR分析得出结论:马氏甲烷八叠球菌能够适应不断变化的三甲胺浓度和中间化合物的消耗。因此,我们假设该生物体具有用于最佳底物利用的调控网络。

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