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Molecular characterization and expression analysis of SERK1 and SERK2 in Brassica napus L.: implication for microspore embryogenesis and plant regeneration

机译:甘蓝型油菜SERK1和SERK2的分子表征和表达分析:对小孢子胚胎发生和植物再生的影响

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Little is known about regulatory role of somatic embryogenesis-related kinase (SERK) genes family in the induction of microspore embryogenesis, development and plant regeneration. In this study, the expression of two SERK genes (SERK1 and SERK2) was assessed during the microspore embryogenesis and plantlet regeneration in Brassica napus L. The BnSERK1 was severely up-regulated 1-5 days following microspore culture and its expression drastically decreased in the globular-heart and also torpedo staged microspore-derived embryos (MDEs). In addition, high levels of BnSERK1 transcript were detected in the MDE maturation phase and in the roots and shoots of the regenerated plantlets which indicates a broader role(s) of BnSERK1 in the organ formation, rather than being specific to the embryogenesis. Results of partial sequencing indicated that the BnSERK1 shares a conserved serine-threonine kinase catalytic domain and exhibited 95 % similarity with AtSERK1, CsSERK1, BrSERK1, NaSERK1, and NbSERK1. A steady increase in the expression of BnSERK2 was observed during the MDE initiation and development so that, the highest expression was noted in the MDE maturation phase i.e., late cotyledonary MDEs. Our results also indicated low amounts of BnSERK2 transcript at the onset of rhyzogenesis but significantly higher expression in the developing roots. In contrast, the BnSERK2 strongly up-regulated during the both initially and developed shoots. The BnSERK2 shares highly conserved LRR-RLK domain when compared with different species tested so that, high homology (100 %) was noticed with BrSERK2. Based on our findings, MDE formation and plantlet regeneration seem to be correlated with both BnSERK1 and BnSERK2 expression.
机译:关于体细胞胚发生相关激酶(SERK)基因家族在诱导小孢子胚发生,发育和植物再生中的调控作用知之甚少。在这项研究中,评估了两个甘蓝型油菜小孢子胚胎发生和植株再生过程中的两个SERK基因(SERK1和SERK2)的表达。BnSERK1在小孢子培养后1-5天被严重上调,在小孢子培养中BnSERK1的表达急剧下降。球状心和鱼雷分阶段的小孢子衍生胚胎(MDE)。此外,在MDE成熟期以及再生小植株的根和芽中检测到高水平的BnSERK1转录物,这表明BnSERK1在器官形成中的作用更为广泛,而不是特定于胚胎发生。部分测序的结果表明,BnSERK1共有一个保守的丝氨酸-苏氨酸激酶催化结构域,并与AtSERK1,CsSERK1,BrSERK1,NaSERK1和NbSERK1表现出95%的相似性。在MDE的启动和发育过程中观察到BnSERK2表达的稳定增加,因此,在MDE成熟阶段,即子叶后期的MDE中,表达最高。我们的研究结果还表明,在发根发生初期,BnSERK2转录物的含量较低,但在发育中的根中表达明显较高。相比之下,BnSERK2在最初和发育的芽期间均强烈上调。与测试的不同物种相比,BnSERK2具有高度保守的LRR-RLK结构域,因此与BrSERK2的同源性很高(100%)。根据我们的发现,MDE的形成和小植株的再生似乎与BnSERK1和BnSERK2的表达都相关。

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