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Profiling and Quantifying Differential Gene Transcription Provide Insights into Ganoderic Acid Biosynthesis in Ganoderma lucidum in Response to Methyl Jasmonate

机译:分析和定量差异基因转录提供了灵芝响应茉莉酸甲酯灵芝灵长酸生物合成的见解。

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摘要

Ganoderma lucidum is a mushroom with traditional medicinal properties that has been widely used in China and other countries in Eastern Asia. Ganoderic acids (GA) produced by G. lucidum exhibit important pharmacological activities. Previous studies have demonstrated that methyl jasmonate (MeJA) is a potent inducer of GA biosynthesis and the expression of genes involved in the GA biosynthesis pathway in G. lucidum. To further explore the mechanism of GA biosynthesis, cDNA-Amplified Fragment Length Polymorphism (cDNA-AFLP) was used to identify genes that are differentially expressed in response to MeJA. Using 64 primer combinations, over 3910 transcriptionally derived fragments (TDFs) were obtained. Reliable sequence data were obtained for 390 of 458 selected TDFs. Ninety of these TDFs were annotated with known functions through BLASTX searching the GenBank database, and 12 annotated TDFs were assigned into secondary metabolic pathways by searching the KEGGPATHWAY database. Twenty-five TDFs were selected for qRT-PCR analysis to confirm the expression patterns observed with cDNA-AFLP. The qRT-PCR results were consistent with the altered patterns of gene expression revealed by the cDNA-AFLP technique. Additionally, the transcript levels of 10 genes were measured at the mycelium, primordia, and fruiting body developmental stages of G. lucidum. The greatest expression levels were reached during primordia for all of the genes except cytochrome b2 reached its highest expression level in the mycelium stage. This study not only identifies new candidate genes involved in the regulation of GA biosynthesis but also provides further insight into MeJA-induced gene expression and secondary metabolic response in G. lucidum.
机译:灵芝是一种具有传统药用特性的蘑菇,已在中国和东亚其他国家广泛使用。灵芝产生的灵芝酸(GA)具有重要的药理活性。先前的研究表明,茉莉酸甲酯(MeJA)是灵芝GA生物合成和灵芝中GA生物合成途径相关基因表达的有效诱导剂。为了进一步探索GA生物合成的机制,使用cDNA扩增片段长度多态性(cDNA-AFLP)来鉴定响应MeJA差异表达的基因。使用64种引物组合,获得了超过3910个转录衍生片段(TDF)。获得了458个所选TDF中的390个的可靠序列数据。通过BLASTX搜索GenBank数据库,对90种这些TDF进行了已知功能的注释,并通过搜索KEGGPATHWAY数据库,将12种带注释的TDF分配给了次级代谢途径。选择了二十五个TDF进行qRT-PCR分析,以确认用cDNA-AFLP观察到的表达模式。 qRT-PCR结果与cDNA-AFLP技术揭示的基因表达改变模式一致。此外,在灵芝的菌丝体,原基和子实体发育阶段测量了10个基因的转录水平。除细胞色素b2在菌丝期达到最高表达水平外,所有基因均在原基期达到最大表达水平。这项研究不仅鉴定了参与GA生物合成调控的新候选基因,而且还进一步了解了由MeJA诱导的灵芝中的基因表达和次级代谢反应。

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