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Kinetic transcriptome analysis reveals an essentially intact induction system in a cellulase hyper-producer Trichoderma reesei strain

机译:动力学转录组分析揭示了纤维素酶高产里氏木霉菌株中基本完整的诱导系统

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Background The filamentous fungus Trichoderma reesei is the main industrial cellulolytic enzyme producer. Several strains have been developed in the past using random mutagenesis, and despite impressive performance enhancements, the pressure for low-cost cellulases has stimulated continuous research in the field. In this context, comparative study of the lower and higher producer strains obtained through random mutagenesis using systems biology tools (genome and transcriptome sequencing) can shed light on the mechanisms of cellulase production and help identify genes linked to performance. Previously, our group published comparative genome sequencing of the lower and higher producer strains NG 14 and RUT C30. In this follow-up work, we examine how these mutations affect phenotype as regards the transcriptome and cultivation behaviour. Results We performed kinetic transcriptome analysis of the NG 14 and RUT C30 strains of early enzyme production induced by lactose using bioreactor cultivations close to an industrial cultivation regime. RUT C30 exhibited both earlier onset of protein production (3 h) and higher steady-state productivity. A rather small number of genes compared to previous studies were regulated (568), most of them being specific to the NG 14 strain (319). Clustering analysis highlighted similar behaviour for some functional categories and allowed us to distinguish between induction-related genes and productivity-related genes. Cross-comparison of our transcriptome data with previously identified mutations revealed that most genes from our dataset have not been mutated. Interestingly, the few mutated genes belong to the same clusters, suggesting that these clusters contain genes playing a role in strain performance. Conclusions This is the first kinetic analysis of a transcriptomic study carried out under conditions approaching industrial ones with two related strains of T. reesei showing distinctive cultivation behaviour. Our study sheds some light on some of the events occurring in these strains following induction by lactose. The fact that few regulated genes have been affected by mutagenesis suggests that the induction mechanism is essentially intact compared to that for the wild-type isolate QM6a and might be engineered for further improvement of T. reesei. Genes from two specific clusters might be potential targets for such genetic engineering.
机译:背景技术丝状真菌里氏木霉是主要的工业纤维素分解酶生产商。过去使用随机诱变已经开发了几种菌株,尽管性能有了显着提高,但低成本纤维素酶的压力刺激了该领域的持续研究。在这种情况下,通过使用系统生物学工具(基因组和转录组测序)通过随机诱变获得的较低和较高生产者菌株的比较研究可以阐明纤维素酶的产生机制,并有助于鉴定与性能相关的基因。先前,我们的小组发表了较低和较高生产者菌株NG 14和RUT C30的比较基因组测序。在这项后续工作中,我们研究了这些突变如何影响转录组和培养行为的表型。结果我们使用接近工业培养方案的生物反应器,对乳糖诱导的早期酶产生的NG 14和RUT C30菌株进行了动力学转录组分析。 RUT C30既显示出较早的蛋白质生成时间(3小时),又显示出更高的稳态生产率。与以前的研究相比,受到调控的基因数量很少(568),其中大多数是针对NG 14菌株的(319)。聚类分析突出显示了某些功能类别的相似行为,使我们能够区分诱导相关基因和生产力相关基因。我们的转录组数据与先前鉴定出的突变的交叉比较表明,我们数据集中的大多数基因尚未突变。有趣的是,少数突变基因属于相同的簇,表明这些簇包含在菌株性能中起作用的基因。结论这是一项转录组学研究的第一个动力学分析,该研究是在接近工业化的条件下,用两种相关的里氏木霉菌株进行的,它们表现出独特的栽培特性。我们的研究揭示了这些菌株在乳糖诱导后发生的一些事件。很少有受调控的基因受到诱变影响的事实表明,与野生型分离株QM6a相比,该诱导机制基本上是完整的,并且可能被工程化以进一步改良里氏木霉。来自两个特定簇的基因可能是此类基因工程的潜在目标。

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