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CLR-4,一种新型的酿酒酵母中纤维素酶基因表达的保守转录因子。

CLR-4, a novel conserved transcription factor for cellulase gene expression in ascomycete fungi.

机构信息

Key Laboratory of Systems Microbial Biotechnology, Tianjin Institute of Industrial Biotechnology, Chinese Academy of Sciences, Tianjin, 300308, China.

出版信息

Mol Microbiol. 2019 Feb;111(2):373-394. doi: 10.1111/mmi.14160. Epub 2018 Nov 25.

DOI:10.1111/mmi.14160
PMID:30474279
Abstract

Fungal degradation of lignocellulosic biomass requires various (hemi-)cellulases and is an important part of the natural carbon cycle. Although induction of cellulases has been described for some saprobic filamentous fungi, the regulation of cellulase transcription is complex and many aspects are still poorly understood. Here, we identified and characterized the novel cellulase regulation factor NcCLR-4 in Neurospora crassa and its ortholog MtCLR-4 in Myceliophthora thermophila. Deletion of CLR-4 resulted in similarly defective cellulolytic enzyme production and activities. Transcriptome analyses of ΔNcclr-4/ΔMtclr-4 revealed the down-regulation of genes encoding (hemi-)cellulases and pivotal regulators (clr-1, clr-2 and xyr-1) and key genes in the cAMP signaling pathway such as adenylate cyclase Nccr-1. Intracellular cAMP levels were markedly lower in ΔNcclr-4/ΔMtclr-4 than in wild-type during cellulose utilization. In electrophoretic mobility shift (EMSA) and DNase I footprinting assays, NcCLR-4/MtCLR-4 can directly bound to the promoters of Nccr-1/Mtcr-1 (encoding adenylyl cyclase). EMSAs also demonstrated that NcCLR-4/MtCLR-4 could directly bound to clr-1 (encoding a key cellulase regulator), Mtclr-2 and Mtxyr-1 (encoding biomass deconstruction regulators). These findings about the novel cellulase expression regulators NcCLR-4 and MtCLR-4 enrich our understanding of how cellulose degradation is regulated and provide new targets for engineering fungi to deconstruct plant biomass in biorefineries.

摘要

真菌对木质纤维素生物质的降解需要各种(半)纤维素酶,是自然碳循环的重要组成部分。尽管已经描述了一些腐生丝状真菌中纤维素酶的诱导,但纤维素酶转录的调控非常复杂,许多方面仍知之甚少。在这里,我们鉴定并表征了粗糙脉孢菌中的新型纤维素酶调控因子 NcCLR-4 及其在嗜热毁丝霉中的同源物 MtCLR-4。CLR-4 的缺失导致类似的纤维素酶生产和活性缺陷。ΔNcclr-4/ΔMtclr-4 的转录组分析显示,编码(半)纤维素酶和关键调控因子(clr-1、clr-2 和 xyr-1)以及 cAMP 信号通路中关键基因(如腺苷酸环化酶 Nccr-1)的基因下调。与野生型相比,ΔNcclr-4/ΔMtclr-4 在利用纤维素时细胞内 cAMP 水平明显降低。在电泳迁移率变动(EMSA)和 DNase I 足迹分析中,NcCLR-4/MtCLR-4 可以直接与 Nccr-1/Mtcr-1(编码腺苷酸环化酶)的启动子结合。EMSA 还表明,NcCLR-4/MtCLR-4 可以直接与 clr-1(编码关键纤维素酶调控因子)、Mtclr-2 和 Mtxyr-1(编码生物质解构调控因子)结合。这些关于新型纤维素表达调控因子 NcCLR-4 和 MtCLR-4 的发现丰富了我们对纤维素降解如何调控的理解,并为工程真菌在生物炼制厂中解构植物生物质提供了新的目标。

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