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金针菇菌柄组织硬化过程中细胞壁合成相关MYB基因家族的全基因组鉴定及FfMYB13调控分析

Genome-wide identification of the MYB gene family and FfMYB13 regulation analysis in cell wall synthesis underlying tissue toughening process of yellow Flammulina filiformis stipes.

作者信息

Zhang Benfeng, Wei Xuyang, Xi Linhao, Qiao Yingli, Chang Mingchang, Deng Bing, Liu Jingyu

机构信息

College of Food Science and Engineering, Shanxi Agricultural University, Taigu 030801, Shanxi, China; Key Laboratory of Shanxi Province for Loess Plateau Edible Fungi, Taigu 030801, Shanxi, China.

College of Food Science and Engineering, Shanxi Agricultural University, Taigu 030801, Shanxi, China.

出版信息

Int J Biol Macromol. 2025 Feb;288:138660. doi: 10.1016/j.ijbiomac.2024.138660. Epub 2024 Dec 11.

DOI:10.1016/j.ijbiomac.2024.138660
PMID:39672422
Abstract

MYB transcription factors (TFs) play important roles in fungal growth, development, stress response, and secondary metabolism. Cell wall glycan remodeling induced by oxidative damage levels is vital for stipe quality during mature stage of yellow Flammulina filiformis fruiting bodies. In this study, we identified 15 F. filiformis MYB (FfMYB) that are ranging from 28.43 kDa-172.3 kDa, with an average of 73.51 kDa. These FfMYB genes were unevenly distributed among six chromosomes. Phylogenetic analysis indicated that 15 FfMYBs were closely related to existing model fungi, while they were more distant from Arabidopsis thaliana. Based on expression analysis, a MYB TF termed FfMYB13 were isolated and identified as a potential regulator binding the promoter of Ff-FeSOD1, which was negatively correlated with tissue toughening of yellow F. filiformis stipes. The data of DAP-seq analysis suggested that the downstream target genes of FfMYB13 were significantly enriched in cell wall metabolism. The result of EMSA and dual luciferase report experiments demonstrated that FfMYB13 served as an upstream transcriptional regulatory factor that activates four cell wall synthesis metabolism related genes, FfKRE6, Ffgas1, FfHYD-1, and FfGFA1. Moreover, FfMYB13 might negatively influence tissue toughening in the inhibition of oxidative damage by activating Ff-FeSOD1.

摘要

MYB转录因子在真菌的生长、发育、应激反应和次级代谢中发挥着重要作用。氧化损伤水平诱导的细胞壁聚糖重塑对金针菇子实体成熟阶段的菌柄品质至关重要。在本研究中,我们鉴定了15个金针菇MYB(FfMYB),其分子量范围为28.43 kDa至172.3 kDa,平均为73.51 kDa。这些FfMYB基因在6条染色体上分布不均。系统发育分析表明,15个FfMYB与现有模式真菌密切相关,而与拟南芥的关系较远。基于表达分析,分离并鉴定了一个名为FfMYB13的MYB转录因子,它是一个潜在的调节因子,可结合Ff-FeSOD1的启动子,该启动子与金针菇菌柄的组织硬化呈负相关。DAP-seq分析数据表明,FfMYB13的下游靶基因在细胞壁代谢中显著富集。EMSA和双荧光素酶报告实验结果表明,FfMYB13作为上游转录调节因子,激活了4个与细胞壁合成代谢相关的基因FfKRE6、Ffgas1、FfHYD-1和FfGFA1。此外,FfMYB13可能通过激活Ff-FeSOD1来抑制氧化损伤,从而对组织硬化产生负面影响。

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