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Identifying and characterizing genes and transcription factors involved in coloration of apple fruit

机译:鉴定和表征涉及苹果果实着色的基因和转录因子

摘要

Apple (Malus × domestica Borkh.) is one of the most highly cultivated fruit crops grown around the world and apple consumption has been increasing over the years. One of the most important determinants of fruit quality is skin color. Red coloration in apple fruit is attributed to anthocyanin accumulation. Anthocyanins are encoded by structural genes, in the anthocyanin biosynthetic pathway, which are highly regulated by transcription factors. In this thesis, studies were conducted to identify and characterize structural genes and associated transcription factors involved in the anthocyanin biosynthetic pathway. Three genes encoding apple anthocyanin reductase gene (MdANR) were isolated, designated as MdANR1, MdANR2a, and MdANR2b. It is found that MdANR2a, and MdANR2b are in fact allelic. MdANR1 and MdANR2 were mapped to the apple linkage map on linkage groups (LG) 10 and 5, respectively. The functionality of MdANR gene was investigated following its overexpression in tobacco and found to influence flower color pigmentation and pattern. Overexpression of MdANR influenced other genes in the flavonoid biosynthesis pathway by down-regulating chalcone isomerase (CHI), dihydroflavonol reductase (DFR), and leucoanthocyanidin reductase (LAR) genes. Moreover, the observed loss of flower color in transgenic tobacco lines was attributed to reduction of anthocyanin pigments. This was likely due to down-regulation of tobacco CHI and DFR genes that are important in anthocyanin production. In addition, a new floral pigmented pattern was generated by incomplete inhibition of anthocyanin production. As expected, the epicatechin accumulated at higher levels in transgenic tobacco than in wild-type tobacco. However, higher amounts of catechin but lower levels of LAR, responsible for synthesis of catechin, were found in transgenic lines when compared to wild-type tobacco. Thus, it has been proposed that ANR plays a redundant role to that of LAR. A novel MYB transcription factor (TF) gene, designated as MdMYB11, was isolated and genetically mapped onto LG15 of the apple genetic map. Alignment of deduced amino acid sequences of MdMYB11 to those of other R2R3 MYB TFs revealed that this new apple transcription factor contains the R2R3 conserved domain. Moreover, this TF is highly similar to Arabidopsis MYB subgroup 4, such as AtMYB3, 4, and 6, by which they negatively regulate genes involved in monolignol biosynthesis. Functional analysis of MdMYB11 was conducted via ectopic expression in tobacco. Expression of MdMYB11 increased anthocyanin production in tobacco flowers by inducing several anthocyanin biosynthesis pathway genes, particularly those of CHI, chalcone synthase (CHS), and UDP-glucose: flavonoid 3-o-glucosyltransferase (UFGT). In addition, this TF functioned as a repressor of both cinnamate-4-hydroxylase (C4H) and 4-coumaroyl:CoA-ligase (4CL) genes, both important in lignin biosynthesis, and possibly contributing to modulation of floral morphogenesis. Moreover, transgenic flowers had longer styles than those of wild-type flowers, suggesting that the MdMYB11 gene might be involved in pistil development. New candidate TF genes regulating apple fruit coloration were identified following global gene expression analysis of the apple transcriptome using an apple microarray. Comparison of gene expression in fruit peel of apple cv. Red Delicious subjected to continuous ‘dark treatment’ versus dark-grown fruit subjected to ‘14 h-light-exposure’ identified 815 genes that were modulated. Following annotation (to the Arabidopsis Gene Ontology), these genes were classified into 19 categories, and were mostly involved in primary metabolism (17%) and transcription (12%). Of these, 18 genes encoded for putative TFs. Further identification of color-related TFs was conducted by comparison of expression profiles of fruit of red skinned apple cv. Red Delicious and non-red skinned apple cv. Golden Delicious, and using quantitative real-time (RT)-PCR (qRT-PCR). Two putative TF genes were found to be expressed at higher levels in fruit of ‘Red Delicious’ than that in ‘Golden Delicious’, thus suggesting that these TFs might be involved in fruit coloration. Altogether, these findings have provided novel information and knowledge of the role(s) of genes and transcription factors involved in the anthocyanin biosynthesis pathway. Moreover, the regulator mechanism of fruit coloration has been further elucidated following transcriptome analysis of the apple genome and functional analysis of selected genes and transcription factors.
机译:苹果(Malus×domestica Borkh。)是世界上种植率最高的水果作物之一,多年来苹果的消费量一直在增加。水果质量的最重要决定因素之一是肤色。苹果果实中的红色可归因于花青素的积累。花青素由花青素生物合成途径中的结构基因编码,该结构基因受转录因子高度调控。本论文进行了研究,以鉴定和表征花色苷生物合成途径中涉及的结构基因和相关的转录因子。分离了三个编码苹果花色苷还原酶基因(MdANR)的基因,分别命名为MdANR1,MdANR2a和MdANR2b。发现MdANR2a和MdANR2b实际上是等位基因。 MdANR1和MdANR2分别映射到链接组(LG)10和5上的苹果链接图。在烟草中过量表达MdANR基因后,对其功能进行了研究,发现其影响花的色素沉着和花型。 MdANR的过表达通过下调查尔酮异构酶(CHI),二氢黄酮醇还原酶(DFR)和无色花色素还原酶(LAR)基因影响类黄酮生物合成途径中的其他基因。此外,在转基因烟草品系中观察到的花色损失归因于花色苷色素的减少。这可能是由于在花色苷生产中很重要的烟草CHI和DFR基因的下调。此外,由于不完全抑制花青素的产生,产生了新的花色素图案。如所期望的,表儿茶素在转基因烟草中的积累水平高于野生型烟草。但是,与野生型烟草相比,在转基因品系中发现了负责儿茶素合成的较高儿茶素含量但较低的LAR。因此,已经提出,ANR对LAR起着多余的作用。分离出一个新的MYB转录因子(TF)基因,命名为MdMYB11,并将其遗传定位到苹果遗传图谱的LG15上。 MdMYB11推导的氨基酸序列与其他R2R3 MYB TF的氨基酸序列比对显示,该新的苹果转录因子包含R2R3保守域。而且,该TF与拟南芥MYB亚组4如AtMYB3、4和6高度相似,它们通过它们负调控与单木酚生物合成有关的基因。通过烟草中的异位表达对MdMYB11进行功能分析。 MdMYB11的表达通过诱导几个花色苷生物合成途径基因,特别是CHI,查尔酮合酶(CHS)和UDP-葡萄糖:类黄酮3-o-葡萄糖基转移酶(UFGT)的花色苷生物合成途径基因,增加了烟草花中花色苷的产生。此外,此TF可以同时充当肉桂酸4-羟化酶(C4H)和4-香豆酰基:CoA-连接酶(4CL)基因的阻遏物,两者在木质素生物合成中很重要,并可能有助于调节花的形态发生。而且,转基因花的样式比野生型花的样式更长,这表明MdMYB11基因可能参与了雌蕊的发育。在使用苹果微阵列对苹果转录组进行整体基因表达分析之后,确定了调节苹果果实着色的新候选TF基因。苹果cv果皮中基因表达的比较。与“黑暗”水果经历“ 14 h光照”相比,“红色美味”进行了连续的“黑暗处理”,鉴定出了815个被调制的基因。在注释之后(拟南芥基因本体论),这些基因被分为19类,并且主要参与初级代谢(17%)和转录(12%)。在这些基因中,有18个为假定的TF编码。通过比较红皮苹果cv果实的表达谱,进一步鉴定了与颜色相关的TF。红色美味和非红色皮肤的苹果简历。 Golden Delicious,并使用定量实时(RT)-PCR(qRT-PCR)。发现两个假定的TF基因在“红色美味”的果实中表达的水平高于“金色美味”的果实,因此表明这些TF可能与果实的着色有关。总而言之,这些发现为花色苷生物合成途径中涉及的基因和转录因子的作用提供了新颖的信息和知识。此外,在对苹果基因组进行转录组分析以及对选定基因和转录因子的功能分析之后,进一步阐明了水果着色的调节机制。

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    Vimolmangkang Sornkanok;

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  • 年度 2011
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  • 原文格式 PDF
  • 正文语种 {"code":"en","name":"English","id":9}
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