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首页> 外文期刊>Journal of Experimental Botany >Characterization of the wheat gene encoding a grain-specific lipid transfer protein TdPR61, and promoter activity in wheat, barley and rice
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Characterization of the wheat gene encoding a grain-specific lipid transfer protein TdPR61, and promoter activity in wheat, barley and rice

机译:编码谷物特异性脂质转移蛋白TdPR61的小麦基因的特征以及在小麦,大麦和水稻中的启动子活性

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摘要

The TaPR61 gene from bread wheat encodes a lipid transfer protein (LTP) with a hydrophobic signal peptide, predicted to direct the TaPR61 protein to the apoplast. Modelling of TaPR61 revealed the presence of an internal cavity which can accommodate at least two lipid molecules. The full-length gene, including the promoter sequence of a TaPR61 orthologue, was cloned from a BAC library of Triticum durum. Quantitative RT-PCR analysis revealed the presence of TaPR61 and TdPR61 mainly in grain. A transcriptional TdPR61 promoter–GUS fusion was stably transformed into wheat, barley, and rice. The strongest GUS expression in all three plants was found in the endosperm transfer cells, the embryo surrounding region (ESR), and in the embryo. The promoter is strong and has similar but not identical spatial patterns of activity in wheat, barley, and rice. These results suggest that the TdPR61 promoter will be a useful tool for improving grain quality by manipulating the quality and quantity of nutrient/lipid uptake to the endosperm and embryo. Mapping of regions important for the promoter function using transient expression assays in developing embryos resulted in the identification of two segments important for promoter activation in embryos. The putative cis-elements from the distal segment were used as bait in a yeast 1-hybrid (Y1H) screen of a cDNA library prepared from the liquid part of the wheat multinucleate syncytium. A transcription factor isolated in the screen is similar to BES1/BLZ1 from Arabidopsis, which is known to be a key transcriptional regulator of the brassinosteroid signalling pathway.
机译:面包小麦的TaPR61基因编码带有疏水信号肽的脂质转移蛋白(LTP),预计可将TaPR61蛋白引导至质外体。 TaPR61的模型揭示了内部空腔的存在,该内部空腔可以容纳至少两个脂质分子。从硬粒小麦的BAC文库中克隆了包括TaPR61直向同源物的启动子序列在内的全长基因。定量RT-PCR分析显示TaPR61和TdPR61主要存在于谷物中。转录的TdPR61启动子– GUS融合体稳定地转化为小麦,大麦和水稻。在胚乳转移细胞,胚胎周围区域(ESR)和胚胎中发现了所有三种植物中最强的GUS表达。该启动子很强,并且在小麦,大麦和水稻中具有相似但不相同的活性空间模式。这些结果表明,TdPR61启动子将通过控制胚乳和胚芽的营养/脂质摄取的质量和数量,成为改善谷物质量的有用工具。在发育中的胚胎中使用瞬时表达测定法分析对启动子功能重要的区域,导致鉴定了对胚胎中的启动子激活重要的两个区段。从小麦多核合胞体的液体部分制备的cDNA文库的酵母1杂交(Y1H)筛选中,来自远端的推定顺式元件用作诱饵。在筛选中分离出的转录因子类似于拟南芥中的BES1 / BLZ1,已知它是油菜素类固醇信号通路的关键转录调节因子。

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