Evaluation of reference genes for qRT-PCR studies in the colchicine producing Gloriosa superba L.

IF 1.7 4区 生物学 Q4 BIOTECHNOLOGY & APPLIED MICROBIOLOGY Plant Biotechnology Reports Pub Date : 2023-05-18 DOI:10.1007/s11816-023-00840-x
Nekha Johnson, Diana Rodriguez Diaz, Sivakumar Ganapathy, John S Bass, Toni M Kutchan, Abdul L Khan, Albert B Flavier
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Abstract

The flame lily, Gloriosa superba L., is one of the two primary sources of the anti-inflammatory drug, colchicine. Previous studies have shown that a higher level of colchicine production occurs in the rhizomes than in leaves and roots. Earlier precursor feeding and transcriptome analysis of G. superba have provided a putative pathway and candidate genes involved in colchicine biosynthesis. Comparative analysis of expression levels of candidate pathway genes in different tissues of G. superba using quantitative real-time reverse transcription-polymerase chain reaction (qRT-PCR) can reveal highly expressed genes in the rhizome compared to other tissues which could suggest roles of the gene products in colchicine biosynthesis. Normalization is an important step in effectively analyzing differential gene expression by qRT-PCR with broader applications. The current study selected candidate reference genes from the transcriptome datasets and analyzed them to determine the most stable genes for normalization of colchicine biosynthesis-related genes. Using RefFinder, one stable reference gene, UBC22, was selected to normalize gene expression levels of candidate methyltransferase (MT) genes in the leaves, roots, and rhizomes of G. superba. With UBC22 as reference gene, the methyltransferases, GsOMT1, GsOMT3, and GsOMT4 showed significantly higher expression levels in the rhizome of G. superba, while MT31794 was more highly expressed in the roots. In conclusion, the current results showed a viable reference gene expression analysis system that could help elucidate colchicine biosynthesis and its exploitation for increased production of the drug in G. superba.

Supplementary information: The online version contains supplementary material available at 10.1007/s11816-023-00840-x.

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用于生产秋水仙碱的超级球藻qRT-PCR研究的参考基因的评价。
火焰百合,Gloriosa superba L.,是抗炎药秋水仙碱的两个主要来源之一。先前的研究表明,根状茎中秋水仙碱的产生水平高于叶和根。木荷的早期前体喂养和转录组分析提供了参与秋水仙碱生物合成的假定途径和候选基因。使用定量实时逆转录聚合酶链反应(qRT-PCR)对候选途径基因在超级稻不同组织中的表达水平进行比较分析,可以揭示与其他组织相比在根茎中高表达的基因,这可能表明基因产物在秋水仙碱生物合成中的作用。标准化是通过qRT-PCR有效分析差异基因表达的重要步骤,具有更广泛的应用。目前的研究从转录组数据集中选择了候选参考基因,并对其进行了分析,以确定秋水仙碱生物合成相关基因正常化的最稳定基因。使用RefFinder,选择一个稳定的参考基因UBC22来标准化超级稻叶片、根和根茎中候选甲基转移酶(MT)基因的基因表达水平。以UBC22为参考基因,甲基转移酶GsOMT1、GsOMT3和GsOMT4在超级根中表现出显著更高的表达水平,而MT31794在根中的表达更高。总之,目前的结果显示了一个可行的参考基因表达分析系统,该系统可以帮助阐明秋水仙碱的生物合成及其在木荷中增加药物产量的利用。补充信息:在线版本包含补充材料,网址为10.1007/s11816-023-00840-x。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Plant Biotechnology Reports
Plant Biotechnology Reports 生物-生物工程与应用微生物
CiteScore
4.10
自引率
4.20%
发文量
72
审稿时长
>12 weeks
期刊介绍: Plant Biotechnology Reports publishes original, peer-reviewed articles dealing with all aspects of fundamental and applied research in the field of plant biotechnology, which includes molecular biology, genetics, biochemistry, cell and tissue culture, production of secondary metabolites, metabolic engineering, genomics, proteomics, and metabolomics. Plant Biotechnology Reports emphasizes studies on plants indigenous to the Asia-Pacific region and studies related to commercialization of plant biotechnology. Plant Biotechnology Reports does not exclude studies on lower plants including algae and cyanobacteria if studies are carried out within the aspects described above.
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