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Molecular cloning and promoter analysis of the specific salicylic acid biosynthetic pathway gene phenylalanine ammonia-lyase (AaPAL1) from Artemisia annua

机译:青蒿特异水杨酸生物合成途径基因苯丙氨酸解氨酶(AaPAL1)的分子克隆和启动子分析

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摘要

Phenylalanine ammonia-lyase (PAL) is the key enzyme in the biosynthetic pathway of salicylic acid (SA). In this study, a full-length cDNA of PAL gene (named as AaPAL1) was cloned from Artemisia annua. The gene contains an open reading frame of 2,151 bps encoding 716 amino acids. Comparative and bioinformatics analysis revealed that the polypeptide protein of AaPAL1 was highly homologous to PALs from other plant species. Southern blot analysis revealed that it belonged to a gene family with three members. Quantitative RT-PCR analysis of various tissues of A. annua showed that AaPAL1 transcript levels were highest in the young leaves. A 1160-bp promoter region was also isolated resulting in identification of distinct cis-regulatory elements including W-box, TGACG-motif, and TC-rich repeats. Quantitative RT-PCR indicated that AaPAL1 was upregulated by salinity, drought, wounding, and SA stresses, which were corroborated positively with the identified cis-elements within the promoter region. AaPAL1 was successfully expressed in Escherichia. coli and the enzyme activity of the purified AaPAL1 was approximately 287.2 U/mg. These results substantiated the involvement of AaPAL1 in the phenylalanine pathway.
机译:苯丙氨酸氨裂解酶(PAL)是水杨酸(SA)生物合成途径中的关键酶。在这项研究中,从青蒿中克隆了PAL基因的全长cDNA(命名为AaPAL1)。该基因包含一个2,151 bps的开放阅读框,编码716个氨基酸。比较和生物信息学分析表明,AaPAL1的多肽蛋白与其他植物物种的PAL高度同源。 Southern印迹分析显示它属于具有三个成员的基因家族。桔梗各组织的定量RT-PCR分析表明,AaPAL1转录水平在幼叶中最高。还分离了一个1160 bp的启动子区域,从而鉴定出不同的顺式调控元件,包括W-box,TGACG-motif和TC-rich重复序列。定量RT-PCR表明,盐度,干旱,创伤和SA胁迫会上调AaPAL1的表达,与启动子区域内已确定的顺式元素呈正相关。 AaPAL1在大肠杆菌中成功表达。大肠埃希菌和纯化的AaPAL1的酶活性约为287.2 U / mg。这些结果证实了AaPAL1参与苯丙氨酸途径。

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