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大豆(Glycine max)组织中的过氧化物酶和其他过氧化物代谢活性

Hydroperoxide Lyase and Other Hydroperoxide-Metabolizing Activity in Tissues of Soybean, Glycine max.

机构信息

Seed Biosynthesis Research, National Center For Agricultural Utilization Research, Peoria, Illinois 61604.

出版信息

Plant Physiol. 1991 Nov;97(3):1059-72. doi: 10.1104/pp.97.3.1059.

Abstract

Hydroperoxide lyase (HPLS) activity in soybean (Glycine max) seed/seedlings, leaves, and chloroplasts of leaves required detergent solubilization for maximum in vitro activity. On a per milligram of protein basis, more HPLS activity was found in leaves, especially chloroplasts, than in seeds or seedlings. The total yield of hexanal from 13(S)-hydroperoxy-cis-9,trans-11-octadecadienoic acid (13S-HPOD) from leaf or chloroplast preparations was 58 and 66 to 85%, respectively. Because of significant competing hydroperoxide-metabolizing activities from other enzymes in seed/seedling preparations, the hexanal yields from this source were lower (36-56%). Some of the products identified from the seed or seedling preparations indicated that the competing activity was mainly due to both a hydroperoxide peroxygenase and reactions catalyzed by lipoxygenase. Different HPLS isozyme compositions in the seed/seedling versus the leaf/chloroplast preparations were indicated by differences in the activity as a function of pH, the K(m) values, relative V(max) with 13S-HPOD and 13(S)-hydroperoxy-cis-9,trans-11,cis-15-octadecatrienoic acid (13S-HPOT), and the specificity with different substrates. With regard to the latter, both seed/seedling and chloroplast HPLS utilized the 13S-HPOD and 13S-HPOT substrates, but only seeds/seedlings were capable of metabolizing 9(S)-hydroperoxy-trans-10,cis-12-octadecadienoic acid into 9-oxononanoic acid, isomeric nonenals, and 4-hydroxynonenal. From 13S-HPOD and 13S-HPOT, the products were identified as 12-oxo-cis-9-dodecenoic acid, as well as hexanal from 13S-HPOD and cis-3-hexenal from 13S-HPOT. In seed preparations, there was partial isomerization of the cis-3 or cis-9 into trans-2 or trans-10 double bonds, respectively.

摘要

大豆种子/幼苗、叶片和叶绿体中的过氧化物酶(HPLS)活性需要去污剂增溶才能达到最大体外活性。以每毫克蛋白质为基础,叶片,尤其是叶绿体中的 HPLS 活性高于种子或幼苗。从 13(S)-羟基顺-9,反-11-十八碳二烯酸(13S-HPOD)产生的己醛的总产量来自叶片或叶绿体制剂分别为 58%和 66%至 85%。由于种子/幼苗制剂中其他酶的过氧化物代谢活性的显著竞争,该来源的己醛产率较低(36-56%)。从种子或幼苗制剂中鉴定出的一些产物表明,竞争活性主要归因于过氧化物过氧化物酶和脂氧合酶催化的反应。种子/幼苗与叶片/叶绿体制剂中不同的 HPLS 同工酶组成表明,活性随 pH 变化、K(m) 值、相对 V(max) 与 13S-HPOD 和 13(S)-羟基顺-9,反-11,顺-15-十八碳三烯酸(13S-HPOT)的关系以及不同底物的特异性不同。关于后者,种子/幼苗和叶绿体 HPLS 均利用 13S-HPOD 和 13S-HPOT 底物,但只有种子/幼苗能够将 9(S)-羟基反式-10,顺式-12-十八碳二烯酸代谢为 9-氧代壬酸、异构壬醛和 4-羟基壬醛。从 13S-HPOD 和 13S-HPOT 中,产物被鉴定为 12-氧代顺式-9-十二烯酸,以及来自 13S-HPOD 的己醛和顺式-3-己烯醛来自 13S-HPOT。在种子制剂中,顺式-3 或顺式-9 分别部分异构化为反式-2 或反式-10 双键。

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