Integration of DNA Methylation, MicroRNAome, Degradome and Transcriptome Provides Insights into Petunia Anther Development.

IF 4 2区 生物学 Q2 CELL BIOLOGY Plant and Cell Physiology Pub Date : 2025-01-29 DOI:10.1093/pcp/pcae126
Yuanzheng Yue, Wuwei Zhu, Jiahui Wang, Tengteng Wang, Lisha Shi, Hannah Rae Thomas, Huirong Hu, Lianggui Wang
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Abstract

Petunia hybrida is an annual herb flower that is prevalently cultivated both in public landscaping and home gardening. Anthers are vital reproductive organs for plants, but the molecular mechanism controlling petunia anther development remains elusive. In this work, we combined DNA methylation, microRNAome, degradome and transcriptome data to generate a comprehensive resource focused on exploring the complex molecular mechanism of petunia anther development. This study shows that DNA methylation could have an important impact in repressing the anther-expressed genes in the late stages of anther maturation. A total of 8,096 anther-preferential genes and 149 microRNAs (miRNAs) were identified that highly expressed in the five typical petunia anther developmental stages. Gene Ontology enrichment analysis of differentially expressed genes as well as miRNAs target genes revealed that metabolic, cellular and single-organism processes were significantly activated during the anther maturation processes. Moreover, a co-expression regulatory network for five typical anther development stages was constructed based on transcriptomic data, in which two hub transcription factors, PhERF48 and PhMS1, were demonstrated to be important regulatory genes for male fertility. Furthermore, two DNA demethylase proteins (PhDME and PhDML3) and three methyl-CpG-binding-domain proteins (PhMBD2, PhMBD3 and PhMBD4) were identified as potential critical DNA methylation regulators in petunia anther development. Our results provide new knowledge regarding the regulatory mechanism of petunia anther development, which will support the breeding of novel sterile petunia lines in the future.

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整合 DNA 甲基化、MicroRNA 组、降解组和转录组有助于深入了解矮牵牛花药的发育。
矮牵牛花是一种一年生草本花,普遍种植在公共景观和家庭园艺中。花药是植物重要的生殖器官,但控制矮牵牛花药发育的分子机制尚不清楚。在这项工作中,我们将DNA甲基化、microRNAome、降解组和转录组数据结合起来,形成了一个全面的资源,专注于探索矮牵牛花药发育的复杂分子机制。该研究表明,DNA甲基化可能对花药成熟后期花药表达基因的抑制有重要影响。在5个典型矮牵牛花药发育阶段共鉴定出8096个花药优先基因和149个microRNAs (miRNAs)高表达。差异表达基因和miRNAs靶基因的基因本体富集分析显示,在花药成熟过程中,代谢、细胞和单生物过程被显著激活。此外,基于转录组学数据,构建了5个典型花药发育阶段的共表达调控网络,其中两个枢纽转录因子PhERF48和PhMS1是重要的雄性生殖调控基因。进一步,鉴定出两个DNA去甲基化酶蛋白(PhDME和PhDML3)和三个甲基- cpg结合域蛋白(PhMBD2, PhMBD3和PhMBD4)是牵牛花花药发育中潜在的关键DNA甲基化调节因子。研究结果为矮牵牛花药发育的调控机制提供了新的认识,为矮牵牛不育新品系的选育提供了依据。
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来源期刊
Plant and Cell Physiology
Plant and Cell Physiology 生物-细胞生物学
CiteScore
8.40
自引率
4.10%
发文量
166
审稿时长
1.7 months
期刊介绍: Plant & Cell Physiology (PCP) was established in 1959 and is the official journal of the Japanese Society of Plant Physiologists (JSPP). The title reflects the journal''s original interest and scope to encompass research not just at the whole-organism level but also at the cellular and subcellular levels. Amongst the broad range of topics covered by this international journal, readers will find the very best original research on plant physiology, biochemistry, cell biology, molecular genetics, epigenetics, biotechnology, bioinformatics and –omics; as well as how plants respond to and interact with their environment (abiotic and biotic factors), and the biology of photosynthetic microorganisms.
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