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影响crepenynic酸生物合成的高山还阳参脂肪酸去饱和酶的克隆与转录分析。

Cloning and transcriptional analysis of Crepis alpina fatty acid desaturases affecting the biosynthesis of crepenynic acid.

作者信息

Nam Jeong-Won, Kappock T Joseph

机构信息

Department of Chemistry, Washington University in St Louis, One Brookings Drive, Campus Box 1134, St Louis, MO 63130-4899, USA.

出版信息

J Exp Bot. 2007;58(6):1421-32. doi: 10.1093/jxb/erm005. Epub 2007 Feb 27.

DOI:10.1093/jxb/erm005
PMID:17329262
Abstract

Crepis alpina acetylenase is a variant FAD2 desaturase that catalyses the insertion of a triple bond at the Delta12 position of linoleic acid, forming crepenynic acid in developing seeds. Seeds contain a high level of crepenynic acid but other tissues contain none. Using reverse transcriptase-coupled PCR (RT-PCR), acetylenase transcripts were identified in non-seed C. alpina tissues, which were highest in flower heads. To understand why functional expression of the acetylenase is limited to seeds, genes that affect acetylenase activity by providing substrate (FAD2) or electrons (cytochrome b5), or that compete for substrate (FAD3), were cloned. RT-PCR analysis indicated that the availability of a preferred cytochrome b5 isoform is not a limiting factor. Developing seeds co-express acetylenase and FAD2 isoform 2 (FAD2-2) at high levels. Flower heads co-express FAD2-3 and FAD3 at high levels, and FAD2-2 and acetylenase at moderate levels. FAD2-3 was not expressed in developing seed. Real-time RT-PCR absolute transcript quantitation showed 10(4)-fold higher acetylenase expression in developing seeds than in flower heads. Collectively, the results show that both the acetylenase expression level and the co-expression of other desaturases may contribute to the tissue specificity of crepenynate production. Helianthus annuus contains a Delta12 acetylenase in a polyacetylene biosynthetic pathway, so does not accumulate crepenynate. Real-time RT-PCR analysis showed relatively strong acetylenase expression in young sunflowers. Acetylenase transcription is observed in both species without accumulation of the enzymatic product, crepenynate. Functional expression of acetylenase appears to be affected by competition and collaboration with other enzymes.

摘要

高山还阳参乙炔酶是一种变异的FAD2去饱和酶,它催化在亚油酸的Δ12位置插入一个三键,在发育中的种子中形成crepenynic酸。种子中含有高水平的crepenynic酸,但其他组织中没有。使用逆转录酶偶联PCR(RT-PCR),在高山还阳参的非种子组织中鉴定出了乙炔酶转录本,其在花头中含量最高。为了理解为什么乙炔酶的功能表达仅限于种子,克隆了通过提供底物(FAD2)或电子(细胞色素b5)来影响乙炔酶活性的基因,或者与底物竞争的基因(FAD3)。RT-PCR分析表明,一种优选的细胞色素b5同工型的可用性不是限制因素。发育中的种子高水平共表达乙炔酶和FAD2同工型2(FAD2-2)。花头高水平共表达FAD2-3和FAD3,中等水平共表达FAD2-2和乙炔酶。FAD2-3在发育中的种子中不表达。实时RT-PCR绝对转录本定量显示,发育中的种子中乙炔酶的表达比花头中高10^4倍。总体而言,结果表明乙炔酶的表达水平以及其他去饱和酶的共表达都可能导致crepenynate产生的组织特异性。向日葵在聚乙炔生物合成途径中含有一种Δ12乙炔酶,因此不会积累crepenynate。实时RT-PCR分析显示,年轻向日葵中乙炔酶表达相对较强。在这两个物种中都观察到了乙炔酶转录,但没有酶产物crepenynate的积累。乙炔酶的功能表达似乎受到与其他酶的竞争和协作的影响。

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