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首页> 外文期刊>Journal of Plant Physiology >On the specificity of lipid hydroperoxide fragmentation by fatty acid hydroperoxide lyase from Arabidopsis thaliana
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On the specificity of lipid hydroperoxide fragmentation by fatty acid hydroperoxide lyase from Arabidopsis thaliana

机译:拟南芥中脂肪酸氢过氧化物裂解酶对脂质氢过氧化物片段化的特异性

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Fatty acid hydroperoxide lyase (HPL) is a membrane associated P450 enzyme that cleaves fatty acid hydroperoxides into aldehydes and omega-oxo fatty acids. One of the major products of this reaction is (3Z)-hexenal. It is a constituent of many fresh smelling fruit aromas. For its biotechnological production and because of the lack of structural data on the HPL enzyme family, we investigated the mechanistic reasons for the substrate specificity of HPL by using various structural analogues of HPL substrates. To approach this 13-HPL from Arabidopsis thaliana was cloned and expressed in E. coli utilising a His-Tag expression vector. The fusion protein was purified by affinity chromatography from the E. coli membrane fractions and its pH optimum was detected to be pH 7.2. Then, HPL activity against the respective (9S)- and (13S)-hydroperoxides derived either from linoleic, alpha-linolenic or gamma-linolenic acid, respectively, as well as that against the corresponding methyl esters was analysed. Highest enzyme activity was observed with the (13S)-hydroperoxide of alpha-linolenic acid (13alpha-HPOT) followed by that with its methyl ester. Most interestingly, when the hydroperoxy isomers of gamma-linolenic acid were tested as substrates, 9gamma-HPOT and not 13gamma-HPOT was found to be a better substrate of the enzyme. Taken together from these studies on the substrate specificity it is concluded that At13HPL may not recognise the absolute position of the hydroperoxy group within the substrate, but shows highest activities against substrates with a (1Z,4S,5E,7Z)-4-hydroperoxy-1,5,7-triene motif. Thus, At13HPL may not only be used for the production of C-6-derived volatiles, but depending on the substrate may be further used for the production of C-9-derived volatiles as well.
机译:脂肪酸氢过氧化物裂解酶(HPL)是一种与膜相关的P450酶,可将脂肪酸氢过氧化物裂解为醛和ω-氧代脂肪酸。该反应的主要产物之一是(3Z)-己烯醛。它是许多新鲜闻到的水果香气的成分。对于其生物技术生产以及由于缺乏HPL酶家族的结构数据,我们通过使用HPL底物的各种结构类似物研究了HPL底物特异性的机理。为了接近此,拟南芥的13-HPL被克隆并利用His-Tag表达载体在大肠杆菌中表达。通过亲和色谱法从大肠杆菌膜级分纯化融合蛋白,并检测其最适pH为pH 7.2。然后,分析了HPL对分别衍生自亚油酸,α-亚麻酸或γ-亚麻酸的(9S)-和(13S)-氢过氧化物的活性,以及​​对相应的甲酯的活性。用α-亚麻酸的(13S)-氢过氧化物(13α-HPOT)观察到最高的酶活性,然后是其甲酯。最有趣的是,当将γ-亚麻酸的氢过氧异构体作为底物进行测试时,发现9gamma-HPOT而非13gamma-HPOT是该酶的更好底物。从这些对底物特异性的研究中得出的结论是,At13HPL可能无法识别底物中氢过氧基团的绝对位置,但显示出对具有(1Z,4S,5E,7Z)-4-氢过氧- 1,5,7-三烯基序。因此,At13HPL不仅可以用于生产C-6来源的挥发物,而且取决于底物,还可以进一步用于生产C-9来源的挥发物。

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