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首页> 外文期刊>Physiologia plantarum >Screening of UV-B-induced genes from apple peels by SSH: possible involvement of MdCOP1-mediated signaling cascade genes in anthocyanin accumulation.
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Screening of UV-B-induced genes from apple peels by SSH: possible involvement of MdCOP1-mediated signaling cascade genes in anthocyanin accumulation.

机译:通过SSH从苹果果皮中筛选UV-B诱导的基因:MdCOP1介导的信号级联基因可能参与花色苷的积累。

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Suppression subtractive hybridization (SSH) was employed to identify candidate genes involved in red coloration in apple peel with the ultraviolet (UV)-B-treated "Mutsu". After reverse Northern blotting verification, nearly 80 clones were successfully sequenced. Large portions of the expressed sequence tags (ESTs) are well characterized anthocyanin biosynthesis-related genes, such as chalcone synthase (11A5), flavonol synthase (12F3), anthocyanidin synthase (11H5) and UDP-glycosyl transferase (14A12) whose presence proved the success of SSH. Eight ESTs were selected for quantitative real-time polymerase chain reaction analysis and their expressions were all elevated in "Induction", further confirming the reliability of the SSH library. One EST, 11F4 (CONSTITUTIVE PHOTOMORPHOGENIC 1: COP1) with putative function in light signal relay was further analyzed in "Mutsu" and "Tsugaru", along with MdHY5 (ELONGATED HYPOCOTYL 5: the downstream target of COP1), MdMYB22 (a possible flavonol-specific activator under the regulation of HY5, belonging to the SG7/PRODUCTION OF FLAVONOL GLYCOSIDES family) and MdMYBA. Results showed that MdCOP1, MdHY5, MdMYB22 and MdMYBA were all UV-B inducible genes and anthocyanin accumulation occurred after their increased expressions. Moreover, their expressions and anthocyanin content were enhanced under UV-B plus 17 degrees C treatment. The presence of G box, a known consensus binding site of HY5, in the MdMYBA promoter region implicated that it could be regulated by MdHY5, which was verified by the result of the yeast one-hybrid analysis. Our data suggested that UV-B irradiation would induce the utmost upstream light signaling factor, MdCOP1, which activates MdHY5 signaling by binding to the promoter regions of MdMYBs, and finally leads to the red coloration of apple peels.
机译:使用抑制消减杂交(SSH)来鉴定与紫外线(B)处理的“ Mutsu”在苹果果皮中红色相关的候选基因。经过反向Northern印迹验证后,成功测序了近80个克隆。表达序列标签(EST)的大部分是花色苷生物合成相关基因的特征明确的基因,例如查尔酮合酶(11A5),黄酮醇合酶(12F3),花色素苷合酶(11H5)和UDP-糖基转移酶(14A12) SSH成功​​。选择了8个EST用于定量实时聚合酶链反应分析,并且它们的表达在“诱导”中均升高,进一步证实了SSH文库的可靠性。在“ Mutsu”和“ Tsugaru”中进一步分析了一种在光信号中继中具有推定功能的EST,11F4(组成型光生化1:COP1),以及MdHY5(ELONGATED HYPOCOTYL 5:COP1的下游靶标),MdMYB22(可能的黄酮醇) HY5调控下的特定激活剂,属于SG7 /黄酮糖苷生产家族)和MdMYBA。结果表明,MdCOP1,MdHY5,MdMYB22和MdMYBA均为UV-B诱导基因,表达增加后出现花青素积聚。此外,在UV-B加17℃处理下,它们的表达和花色苷含量增加。 MdMYBA启动子区域中存在一个已知的HY5共有共识结合位点G box,暗示它可能受MdHY5调控,这一点已通过酵母单杂交分析的结果得到证实。我们的数据表明,UV-B辐射将诱导最大的上游光信号传导因子MdCOP1,该因子通过与MdMYBs的启动子区域结合而激活MdHY5信号传导,并最终导致苹果皮呈红色。

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