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Characteristics of a Membrane-Associated Lipoxygenase in Tomato Fruit

机译:番茄果实膜相关脂氧合酶的特性

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摘要

Microsomal membranes isolated from the pericarp of maturegreen tomato (Lycopersicon esculentum) fruit rapidly metabolize exogenous radiolabeled linoleic acid into fatty acid oxidation products at 22°C. The reaction is strongly inhibited by n-propyl gallate, an inhibitor of lipoxygenase. The membranes also rapidly metabolize 16:0/18:2* phosphatidylcholine into radiolabeled oxidation products that comigrate on TLC plates with those formed from free linoleic acid. At 30°C, the formation of fatty acid oxidation products from 16:0/18:2* phosphatidylcholine is slower, and there is an initial accumulation of radiolabeled linoleic acid that is not evident at 22°C, which can be attributed to the action of lipolytic acyl hydrolase. Radiolabeled phosphatidic acid and diacylglycerol are also formed during metabolism of 16:0/18:2* phosphatidylcholine by the microsomal membranes, and there is no breakdown of either linoleic acid or phosphatidylcholine by heat-denatured membranes. When Triton X-100 treated membranes were used, the same patterns of metabolite formation from radiolabeled linoleic acid and 16:0/18:2* phosphatidylcholine were observed. Thus, the enzymes mediating the breakdown of these radiolabeled compounds appear to be tightly associated with the membranes. Collectively, the data indicate that there is a lipoxygenase associated with microsomal membranes from tomato fruit that utilizes free fatty acid substrate released from phospholipids. The microsomal lipoxygenase is strongly active over a pH range of 4.5 to 8.0, comprises approximately 38% of the total (microsomal plus soluble) lipoxygenase activity in the tissue, has an apparent Km of 0.52 millimolar and an apparent Vmax of 0.186 millimoles per minute per milligram of protein. The membranous enzyme also cross-reacts with polyclonal antibodies raised against soybean lipoxygenase-1 and has an apparent molecular mass of 100 kilodaltons.
机译:从成熟绿色番茄(Lycopersicon esculentum)果实的果皮中分离出的微粒体膜在22°C时迅速代谢外源性放射性标记的亚油酸为脂肪酸氧化产物。该反应被脂氧合酶抑制剂没食子酸正丙酯强烈抑制。膜还迅速将16:0/18:2 * 磷脂酰胆碱代谢为放射性标记的氧化产物,这些氧化产物在TLC板上与游离的亚油酸形成的迁移。在30°C时,由16:0/18:2 * 磷脂酰胆碱形成脂肪酸氧化产物的速度较慢,并且放射性标记的亚油酸的初始积累在22°C时不明显。 ,这可以归因于脂解酰基水解酶的作用。微粒体膜在16:0/18:2 * 磷脂酰胆碱的代谢过程中也会形成放射性标记的磷脂酸和二酰基甘油,热变性膜不会降解亚油酸或磷脂酰胆碱。当使用Triton X-100处理过的膜时,观察到由放射性标记的亚油酸和16:0/18:2 * 磷脂酰胆碱形成的代谢产物的模式相同。因此,介导这些放射性标记化合物分解的酶似乎与膜紧密结合。总体而言,数据表明存在与来自番茄果实的微粒体膜相关的脂氧化酶,其利用从磷脂释放的游离脂肪酸底物。微粒体脂氧合酶在4.5至8.0的pH范围内具有强活性,约占组织中总(微粒体与可溶性)脂氧合酶活性的38%,表观Km为0.52毫摩尔,表观Vmax为每分钟每分钟0.186毫摩尔毫克蛋白质。膜酶还与针对大豆脂氧合酶-1的多克隆抗体发生交叉反应,表观分子量为100道尔顿。

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