Multi-omics analysis reveals the positive impact of differential chloroplast activity during in vitro regeneration of barley.

IF 3.9 2区 生物学 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY Plant Molecular Biology Pub Date : 2024-11-13 DOI:10.1007/s11103-024-01517-x
Parul Sirohi, Chanderkant Chaudhary, Mayank Sharma, Ravi Bodampalli Anjanappa, Suchi Baliyan, Ritika Vishnoi, Sumit Kumar Mishra, Reeku Chaudhary, Bhairavnath Waghmode, Anuj Kumar Poonia, Hugo Germain, Debabrata Sircar, Harsh Chauhan
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Abstract

Existence of potent in vitro regeneration system is a prerequisite for efficient genetic transformation and functional genomics of crop plants. In this study, two contrasting cultivars differencing in their in vitro regeneration efficiency were identified. Tissue culture friendly cultivar Golden Promise (GP) and tissue culture resistant DWRB91(D91) were selected as contrasting cultivars to investigate the molecular basis of regeneration efficiency through multiomics analysis. Transcriptomics analysis revealed 1487 differentially expressed genes (DEGs), in which 795 DEGs were upregulated and 692 DEGs were downregulated in the GP-D91 transcriptome. Genes encoding proteins localized in chloroplast and involved in ROS generation were upregulated in the embryogenic calli of GP. Moreover, proteome analysis by LC-MS/MS revealed 3062 protein groups and 16,989 peptide groups, out of these 1586 protein groups were differentially expressed proteins (DEPs). Eventually, GC-MS based metabolomics analysis revealed the higher activity of plastids and alterations in key metabolic processes such as sugar metabolism, fatty acid biosynthesis, and secondary metabolism. TEM analysis also revealed differential plastid development. Higher accumulation of sugars, amino acids and metabolites corresponding to lignin biosynthesis were observed in GP as compared to D91. A comprehensive examination of gene expression, protein profiling and metabolite patterns unveiled a significant increase in the genes encompassing various functions, such as ion homeostasis, chlorophyll metabolic process, ROS regulation, and the secondary metabolic pathway.

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多组学分析揭示了大麦离体再生过程中叶绿体活动差异的积极影响。
强大的体外再生系统是作物植物高效遗传转化和功能基因组学的先决条件。本研究确定了两个体外再生效率不同的对比栽培品种。研究选择了对组织培养友好的栽培品种Golden Promise(GP)和对组织培养抗性强的栽培品种DWRB91(D91)作为对比栽培品种,通过多组学分析研究再生效率的分子基础。转录组学分析发现了1487个差异表达基因(DEGs),其中795个DEGs在GP-D91转录组中上调,692个DEGs在GP-D91转录组中下调。编码叶绿体中定位蛋白和参与 ROS 生成的基因在 GP 的胚胎胼胝体中上调。此外,通过 LC-MS/MS 进行的蛋白质组分析发现了 3062 个蛋白质组和 16 989 个肽组,其中 1586 个蛋白质组为差异表达蛋白质(DEPs)。最后,基于 GC-MS 的代谢组学分析显示,质体的活性更高,糖代谢、脂肪酸生物合成和次级代谢等关键代谢过程也发生了改变。TEM 分析也揭示了质体发育的差异。与 D91 相比,在 GP 中观察到糖类、氨基酸和与木质素生物合成相应的代谢物有更高的积累。通过对基因表达、蛋白质分析和代谢物模式的全面研究发现,涵盖各种功能的基因显著增加,如离子平衡、叶绿素代谢过程、ROS 调节和次级代谢途径。
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来源期刊
Plant Molecular Biology
Plant Molecular Biology 生物-生化与分子生物学
自引率
2.00%
发文量
95
审稿时长
1.4 months
期刊介绍: Plant Molecular Biology is an international journal dedicated to rapid publication of original research articles in all areas of plant biology.The Editorial Board welcomes full-length manuscripts that address important biological problems of broad interest, including research in comparative genomics, functional genomics, proteomics, bioinformatics, computational biology, biochemical and regulatory networks, and biotechnology. Because space in the journal is limited, however, preference is given to publication of results that provide significant new insights into biological problems and that advance the understanding of structure, function, mechanisms, or regulation. Authors must ensure that results are of high quality and that manuscripts are written for a broad plant science audience.
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Proteomic and metabolomic insights into the mechanisms of calcium-mediated salt stress tolerance in hemp. Multi-omics analysis reveals the positive impact of differential chloroplast activity during in vitro regeneration of barley. Publisher Correction: Alternative splicing and deletion in S-RNase confer stylar-part self-compatibility in the apple cultivar 'Vered'. Transcriptomic responses of Solanum tuberosum cv. Pirol to arbuscular mycorrhiza and potato virus Y (PVY) infection. DArTseq genotyping facilitates identification of Aegilops biuncialis chromatin introgressed into bread wheat Mv9kr1.
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