首页> 外文OA文献 >Accumulation of ricinoleic, lesquerolic, and densipolic acids in seeds of transgenic Arabidopsis plants that express a fatty acyl hydroxylase cDNA from castor bean.
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Accumulation of ricinoleic, lesquerolic, and densipolic acids in seeds of transgenic Arabidopsis plants that express a fatty acyl hydroxylase cDNA from castor bean.

机译:转基因拟南芥植物种子中蓖麻油酸,间苯二酚和戊二酸的积累,这些基因表达了蓖麻子中的脂肪酰基羟化酶cDNA。

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摘要

A cDNA encoding the oleate 12-hydroxylase from castor bean (Ricinus communis L.) has previously been shown to direct the synthesis of small amounts of ricinoleic acid (12-hydroxyoctadec-cis-9-enoic acid) in seeds of transgenic tobacco plants. Expression of the cDNA under control of the Brassica napus napin promoter in transgenic Arabidopsis thaliana plants resulted in the accumulation of up to 17% of seed fatty acids as ricinoleate and two novel fatty acids that have been identified by gas chromatography-mass spectrometry as lesquerolic (14-hydroxyeicos-cis-11-enoic acid) and densipolic (12-hydroxyoctadec-cis-9,15-dienoic acid) acids. Traces of auricolic acid were also observed. These results suggest that either the castor hydroxylase can utilize oleic acid and eicosenoic acid as substrates for ricinoleic and lesquerolic acid biosynthesis, respectively, or Arabidopsis contains an elongase that accepts ricinoleic acid as a substrate. These observations are also consistent with indirect biochemical evidence that an n-3 desaturase is capable of converting ricinoleic acid to densipolic acid. Expression of the castor hydroxylase also caused enhanced accumulation of oleic acid and a corresponding decrease in the levels of polyunsaturated fatty acids. Since the steady-state level of mRNA for the oleate-12 desaturase was not affected, it appears that the presence of the hydroxylase, directly or indirectly, causes posttranscriptional inhibition of desaturation.
机译:先前已经显示了编码来自蓖麻子(Ricinus communis L.)的油酸酯12-羟化酶的cDNA指导在转基因烟草植物种子中合成少量蓖麻油酸(12-羟基十八烷基-顺式-9-烯酸)。在甘蓝型油菜napin启动子控制下的cDNA在转基因拟南芥植物中的表达导致高达17%的种子脂肪酸如蓖麻油酸酯和两种新脂肪酸的积累,这两种新脂肪酸已通过气相色谱-质谱法鉴定为lesquerolic( 14-羟基二十烷基-顺式-十一烯酸)和戊二酸(12-羟基十八烷基-顺式-9,15-二烯酸)酸。还观察到痕量的金甲酸。这些结果表明,蓖麻羟化酶可以利用油酸和二十碳烯酸分别作为蓖麻油酸和去油芥酸生物合成的底物,或者拟南芥含有接受蓖麻油酸作为底物的延长酶。这些观察结果也与间接生化证据一致,即n-3去饱和酶能够将蓖麻油酸转化为癸二酸。蓖麻羟化酶的表达还引起油酸积累的增加和多不饱和脂肪酸水平的相应降低。由于不影响油酸酯12去饱和酶的mRNA稳态水平,因此似乎直接或间接存在羟化酶会导致转录后抑制去饱和作用。

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    Broun, P; Somerville, C;

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  • 年度 1997
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