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MOLECULAR CLONING AND EXPRESSION ANALYSIS OF PEROXIDASE GENES FROM WHEAT

机译:小麦过氧化物酶基因的分子克隆和表达分析

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A PCR-based screening approach was used to isolate genomic clones from wheat encoding peroxidase isozymes. Three complete genes (pox1, pox2 and pox4) and one truncated gene (pox3) were characterized. The nucleotide sequences predicted mature proteins of 31 kDa, in which all the highly conserved motifs of secreted plant peroxidases were preserved. The coding region s showed 73-83% DNA sequence identity, with the highest level of similarity noted for the tandemly oriented pox2 and pox3. Expression of respective pox genes in various tissues of wheat was assessed by the RT-PCR technique, which showed that all four genes are active. The primary pox1 mRNA was spliced to remove three introns, whereas processing of the other pox transcripts involved only two intervening sequences. Splicing occurred at consensus GU/AG splice sites except for the first introns of pox1, pox2 and pox4 transcripts, where processing took place at unusual GC donor sites. The RNA analysis suggested that the pox1, pox2 and pox4 genes are predominantly expressed in roots. Lower levels of expression were found for pox4 and pox3 in leaves. Infection of wheat by the powdery mildew fungus selectively induced expression of pox2 in leaves.
机译:基于PCR的筛选方法用于从编码过氧化物酶同工酶的小麦中分离基因组克隆。表征了三个完整基因(pox1,pox2和pox4)和一个截短基因(pox3)。核苷酸序列预测了31 kDa的成熟蛋白,其中分泌的植物过氧化物酶的所有高度保守的基序都得以保留。编码区显示73-83%的DNA序列同一性,对于串联定向的pox2和pox3具有最高的相似度。通过RT-PCR技术评估了小麦各组织中pox基因的表达,结果表明这四个基因均具有活性。最初的pox1 mRNA被剪接去除三个内含子,而其他pox转录本的加工仅涉及两个插入序列。剪接发生在共有的GU / AG剪接位点,但pox1,pox2和pox4转录本的第一个内含子除外,它们在不寻常的GC供体位点进行加工。 RNA分析表明pox1,pox2和pox4基因主要在根中表达。发现叶中pox4和pox3的表达水平较低。白粉病真菌对小麦的感染选择性诱导了pox2在叶片中的表达。

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