叶片原生质体来源的紫花苜蓿细胞胚胎发生能力诱导相关基因的鉴定与表征

M. Domoki , J. Györgyey , J. Bíró , T.P. Pasternak , Á. Zvara , S. Bottka , L.G. Puskás , D. Dudits , A. Fehér
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引用次数: 28

摘要

在初始培养基中2,4-二氯苯氧乙酸(2,4- d)浓度的影响下,紫花苜蓿叶片原生质体来源的细胞可以发育成体细胞胚胎。为了揭示胚胎发生能力建立过程中基因表达的变化,我们使用基于pcr的cDNA减法方法比较了分别在1 μM和10 μM 2,4- d存在下发育的细胞类型在第一次细胞分裂时(培养第4天)的基因表达变化。虽然减法效率相对较低,但采用额外的差异筛选步骤可以鉴定出38个10 μM 2,4- d上调转录本。对相应的基因/蛋白进行注释,并选择各种功能基团的代表进行更详细的基因表达分析。采用实时荧光定量PCR (RT-QPCR)方法测定所选基因在2,4- d处理叶片及体细胞胚发生全过程中的相对表达量。基因表达模式证实,除1个基因外,11个研究基因和阳性对照叶子叶1 (MsLEC1)基因均可诱导2,4- d。这些基因在体细胞胚发生的早期诱导期和后期胚分化期表现出不同的表达模式。编码gst转移酶、PR10发病相关蛋白、细胞分裂相关核糖体(S3a)蛋白、arf型小GTPase和核小体组装因子家族SET蛋白的基因不仅在体细胞胚胎诱导过程中,而且在体细胞胚胎分化过程中也表现出较高的相对表达。这可能表明这些基因的表达与体细胞胚胎发生过程中的发育转变(分化和去分化)有关。
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Identification and characterization of genes associated with the induction of embryogenic competence in leaf-protoplast-derived alfalfa cells

Alfalfa leaf protoplast-derived cells can develop into somatic embryos depending on the concentration of 2,4-dichlorophenoxyacetic acid (2,4-D) in the initial culture medium. In order to reveal gene expression changes during the establishment of embryogenic competence, we compared the cell types developed in the presence of 1 and 10 μM 2,4-D, respectively, at the time of their first cell divisions (fourth day of culture) using a PCR-based cDNA subtraction approach. Although the subtraction efficiency was relatively low, applying an additional differential screening step allowed the identification of 38 10 μM 2,4-D up-regulated transcripts. The corresponding genes/proteins were annotated and representatives of various functional groups were selected for more detailed gene expression analysis. Real-time quantitative PCR (RT-QPCR) analysis was used to determine relative expression of the selected genes in 2,4-D-treated leaves as well as during the whole process of somatic embryogenesis. Gene expression patterns confirmed 2,4-D inducibility for all but one of the 11 investigated genes as well as for the positive control leafy cotyledon1 (MsLEC1) gene. The characterized genes exhibited differential expression patterns during the early induction phase and the late embryo differentiation phase of somatic embryogenesis. Genes coding for a GST-transferase, a PR10 pathogenesis-related protein, a cell division-related ribosomal (S3a) protein, an ARF-type small GTPase and the nucleosome assembly factor family SET protein exhibited higher relative expression not only during the induction of somatic embryogenesis but at the time of somatic embryo differentiation as well. This may indicate that the expression of these genes is associated with developmental transitions (differentiation as well as de-differentiation) during the process of somatic embryogenesis.

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