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De novo transcriptome sequencing of radish ( Raphanus sativus L.) fleshy roots: analysis of major genes involved in the anthocyanin synthesis pathway

机译:萝卜(Raphanus sativus L.)肉质根的从头转录组测序:花色苷合成途径中涉及的主要基因分析

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The HongXin radish (Raphanus sativus L.), which contains the natural red pigment (red radish pigment), is grown in the Fuling district of Chongqing City. However, the molecular mechanisms underlying anthocyanin synthesis for the formation of natural red pigment in the fleshy roots of HongXin radish are not well studied. De novo transcriptome of HX-1 radish, as well as that of the advanced inbred lines HX-2 and HX-3 were characterized using next generation sequencing (NGS) technology. In total, approximately 66.22 million paired-end reads comprising 34, 927 unigenes (N50?=?1, 621?bp) were obtained. Based on sequence similarity search with known proteins, total of 30, 127 (about 86.26%) unigenes were identified. Additionally, functional annotation and classification of these unigenes indicated that most of the unigenes were predominantly enriched in the metabolic process-related terms, especially for the biosynthetic pathways of secondary metabolites. Moreover, majority of the anthocyanin biosynthesis-related genes (ABRGs) involved in the regulation of anthocyanin biosynthesis were identified by targeted search for their annotation. Subsequently, the expression of 15 putative ABRGs involved in the anthocyanin synthesis-related pathways were validated using quantitative real-time polymerase chain reaction (qRT-PCR). Of those, RsPAL2, RsCHS-B2, RsDFR1, RsDFR2, RsFLS, RsMT3 and RsUFGT73B2-like were identified significantly associated with anthocyanin biosynthesis. Especially for RsDFR1, RsDFR2 and RsFLS, of those, RsDFR1 and RsDFR2 were highest enriched in the HX-3 and WG-3, but RsFLS were down-regulated in HX-3 and WG-3. We proposed that the transcripts of RsDFR1, RsDFR2 and RsFLS might be act as key regulators in anthocyanin biosynthesis pathway. The assembled radish transcript sequences were analysed to identify the key ABRGs involved in the regulation of anthocyanin biosynthesis. Additionally, the expression patterns of candidate ABRGs involved in the anthocyanin biosynthetic pathway were validated by qRT-PCR. We proposed that the transcripts of RsDFR1, RsDFR2 and RsFLS might be acted as key regulators in anthocyanin biosynthesis pathway. This study will enhance our understanding of the biosynthesis and metabolism of anthocyanin in radish.
机译:含有天然红色素(红萝卜色素)的红心萝卜(Raphanus sativus L.)生长在重庆市ling陵区。然而,尚未深入研究花青素合成在红心萝卜肉质根中形成天然红色素的分子机制。使用下一代测序(NGS)技术表征了HX-1萝卜以及高级自交系HX-2和HX-3的从头转录组。总共获得了约6622万对配对读段,包括34、927个单基因(N50α=?1,621?bp)。基于与已知蛋白质的序列相似性搜索,总共鉴定出30、127(约86.26%)个单基因。此外,这些单基因的功能注释和分类表明,大多数单基因主要富含代谢过程相关的术语,尤其是次生代谢物的生物合成途径。此外,大多数花色苷生物合成相关基因(ABRGs)涉及花色苷生物合成的调控是通过有针对性的搜索来识别的。随后,使用定量实时聚合酶链反应(qRT-PCR)验证了花色苷合成相关途径中涉及的15种假定的ABRG的表达。其中,RsPAL2,RsCHS-B2,RsDFR1,RsDFR2,RsFLS,RsMT3和RsUFGT73B2-like与花色苷的生物合成显着相关。特别是对于RsDFR1,RsDFR2和RsFLS,其中RsDFR1和RsDFR2在HX-3和WG-3中的富集程度最高,而RsFLS在HX-3和WG-3中的表达却被下调。我们提出,RsDFR1,RsDFR2和RsFLS的转录本可能是花色苷生物合成途径中的关键调控因子。分析组装的萝卜转录物序列,以鉴定参与花色苷生物合成调控的关键ABRG。另外,通过qRT-PCR验证了涉及花色苷生物合成途径的候选ABRG的表达模式。我们提出,RsDFR1,RsDFR2和RsFLS的转录本可能是花色苷生物合成途径中的关键调控因子。这项研究将增进我们对萝卜中花色苷生物合成和代谢的了解。

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