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Comparative transcriptomics and transcriptional regulation analysis of enhanced laccase production induced by co-culture of Pleurotus eryngii var. ferulae with Rhodotorula mucilaginosa

机译:增强型曲氏植物红细胞增强漆酶生产的比较转基因组和转录调控分析。 Ferulae与rhodotorula mucilaginosa

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The co-culturing of Pleurotus eryngii var. ferulae and Rhodotorula mucilaginosa was confirmed in our previous studies to be an efficient strategy to improve laccase production by submerged fermentation. To determine the possible regulation principles underlying this behaviour, comparative transcriptomic analysis was performed on P. eryngii var. ferulae to investigate the differential expression of genes in co-culture. RNA-seq analysis showed that genes concerning xenobiotic biodegradation and expenditure of energy were upregulated. However, genes related to oxidative stress were downregulated. In addition, the transcription levels of laccase isoenzymes were not consistent in the co-culture system: 3 laccase genes (lacc1, lacc2, lacc12) were upregulated, and 3 laccase genes (lacc4, lacc6, lacc9) were downregulated. The enhancement in laccase activity can be due to upregulation of a laccase heterodimer encoded by the genes lacc2 and ssPOXA3a (or ssPOXA3b), whose expression levels were increased by 459% and 769% (or 585% for ssPOXA3b) compared with those of a control, respectively. beta-Carotene produced by R. mucilaginosa upregulated the transcription of lacc2 only. Combining these results with an analysis of cis-acting responsive elements indicated that four transcription factors (TFs) had potential regulatory effects on the transcription of laccase genes. It was supposed that TFa regulated lacc transcription by binding with methyl jasmonate and heat shock response elements. The expression of TFb, TFc, and TFd was regulated by beta-carotene. However, beta-carotene had no effect on TFa expression. These results provide a possible mechanism for the regulation of laccase gene transcription in the co-culture system and are also beneficial for the future intensification of fungal laccase production.
机译:Pleurotus eryngii var的共同培养。在我们以前的研究中证实Furulae和rhodotorula粘菌菌病毒是通过淹没发酵改善漆酶生产的有效策略。为了确定这种行为的可能调节原理,对P.Eryngii VAR进行比较转录组分析。 Forula探讨了共培养中基因的差异表达。 RNA-SEQ分析表明,关于异败生物降解和能量支出的基因被上调。然而,下调与氧化应激相关的基因。另外,在共培养系统中,漆酶同工酶的转录水平不一致:上调3漆基因(LACC1,LAC2,LAC112),下调3个漆基因(LACC4,LACC6,LACC9)。漆酶活性的增强可以是由于基因LACC2和SSPOXA3A(或SSPOXA3B)编码的漆酶异二聚体的上调,其表达水平与控制器相比,其表达水平增加了459%和769%(或SSPOXA3B的585%) , 分别。由R. Mucilaginosa产生的β-胡萝卜素仅升高了LACC2的转录。将这些结果与CIS作用响应元件的分析相结合,表明四种转录因子(TFS)对漆酶基因的转录具有潜在的调节作用。假设TFA调节LACC转录通过与茉莉甲酸甲酯和热休克响应元件结合。 TFB,TFC和TFD的表达由β-胡萝卜素调节。然而,β-胡萝卜素对TFA表达没有影响。这些结果提供了调节共培养系统中LACACAS基因转录的可能机制,也有利于未来真菌漆酶生产的强化。

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