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人黄嘌呤脱氢酶/黄嘌呤氧化酶蛋白的器官分布及分子形式

Organ distribution and molecular forms of human xanthine dehydrogenase/xanthine oxidase protein.

作者信息

Sarnesto A, Linder N, Raivio K O

机构信息

Children's Hospital, University of Helsinki, Finland.

出版信息

Lab Invest. 1996 Jan;74(1):48-56.

PMID:8569197
Abstract

Xanthine dehydrogenase/xanthine oxidase (XDH/XO) is a major cytoplasmic source of superoxide radicals and hydrogen peroxide, and it is considered important in the pathogenesis of ischemia-reperfusion damage. Because little is known about the enzyme in human tissues, the aims of this study were to purify human XDH/XO and to produce Ab for detection of the protein in Western blots and for quantification by ELISA. We purified human milk XDH/XO, produced Ab for Western blotting and ELISA of the protein, and evaluated the molecular forms and activity-protein relationships in human tissues. The molecular size of the purified protein under nondenaturing conditions was approximately 300 kd. On SDS-PAGE, it was fragmented into four main bands of 143, 125, 87, and 59 kd. Ab recognized bands of similar size in Western blots of the purified preparation and human milk. In fresh liver homogenates treated with anti-proteases, the three largest bands were observed; in the intestine, only the two largest were observed. Serum, brain, heart, and skeletal muscle were negative, whereas some lung and kidney samples showed one faint band of 143 kd. Trypsin treatment of the enzyme converted the large molecular-weight bands into smaller bands, as did incubation of a liver homogenate without anti-proteases. XDH/XO protein concentrations (ng/mg total protein) were 146 +/- 70 in liver and 556 +/- 320 in intestine and less than 5 ng/ml in serum. The relationship of activity to protein (2.7-3.0 mumol/min/mg XDH/XO protein) was constant in liver and intestine during development. We conclude that 1) human XDH/XO has molecular size and subunit structure similar to other mammalian enzymes; 2) the polypeptide chain is unstable, also in the intact cell, despite retained activity; and 3) the amount of inactive XDH/XO in human liver and intestine is apparently small.

摘要

黄嘌呤脱氢酶/黄嘌呤氧化酶(XDH/XO)是超氧阴离子自由基和过氧化氢的主要胞质来源,并且被认为在缺血再灌注损伤的发病机制中起重要作用。由于对人体组织中的这种酶了解甚少,本研究的目的是纯化人XDH/XO并制备抗体,用于蛋白质印迹法检测该蛋白以及通过酶联免疫吸附测定进行定量分析。我们纯化了人乳中的XDH/XO,制备了用于该蛋白蛋白质印迹法和酶联免疫吸附测定的抗体,并评估了人体组织中的分子形式和活性与蛋白质的关系。在非变性条件下纯化蛋白的分子大小约为300kd。在十二烷基硫酸钠-聚丙烯酰胺凝胶电泳上,它被裂解为143、125、87和59kd的四条主要条带。抗体在纯化制剂和人乳的蛋白质印迹中识别出大小相似的条带。在用抗蛋白酶处理的新鲜肝匀浆中,观察到三条最大的条带;在肠道中,仅观察到两条最大的条带。血清、脑、心脏和骨骼肌呈阴性,而一些肺和肾样本显示出一条143kd的淡条带。用胰蛋白酶处理该酶可将大分子条带转化为较小的条带,未用抗蛋白酶处理的肝匀浆孵育也会如此。肝脏中XDH/XO蛋白浓度(ng/毫克总蛋白)为146±70,肠道中为556±320,血清中小于5ng/ml。在发育过程中,肝脏和肠道中活性与蛋白质的关系(2.7 - 3.0微摩尔/分钟/毫克XDH/XO蛋白)保持恒定。我们得出结论:1)人XDH/XO具有与其他哺乳动物酶相似的分子大小和亚基结构;2)尽管保留了活性,但多肽链不稳定,在完整细胞中也是如此;3)人肝脏和肠道中无活性的XDH/XO量显然很少。

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