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分离的犬心脏线粒体自身抗原位点的鉴定

Characterization of autoantigenic sites on isolated dog heart mitochondria.

作者信息

Kelley R E, Olson M S, Pinckard R N

出版信息

Biochim Biophys Acta. 1975 Sep 2;401(3):370-85. doi: 10.1016/0005-2736(75)90237-0.

Abstract
  1. Anti-heart mitochondria autoantibodies were developed in serum from dogs following experimental myocardial infarction. 2. Heart mitochondria frozen and thawed repeatedly in a sucrose/Tris-chloride buffer retained both their functional integrity as measured by the respiratory control ratio and their ability to serve as an antigen in a complement fixation test. Mitochondria frozen and thawed in a potassium chloride/Tris-chloride buffer lost both their functional integrity and their autoantigenic activity after one freeze-thaw cycle. 3. Extraction of the heart mitochondria with acetone/water mixtures to remove phospholipids from the membrane led to a complete loss of the ability of the mitochondria to react in the complement fixation test but did not affect the ability of the membranes to bind autoantibody in absorption experiments. 4. Treatment of the mitochondrial membranes with increasing concentrations of trypsin caused a loss of up to approximately 50% of the membrane protein with a gradual decrease in the autoantigenic activity of the membrane without impairment of the ability of the membrane to bind autoantibody. 5. Removal of up to 90% of the sialic acid of the mitochondrial membrane with neuraminidase resulted in a considerable increase in the complement-fixing autoantigenic activity of the membrane without changing the apparent ability of the membrane to bind autoantibody in absorption experiments. 6. Exposure of mitochondrial membranes to autoantibody and complement caused an inhibition of both an inner mitochondrial membrane enzyme, i.e. cytochrome oxidase (48%) and an outer mitochondrial membrane enzyme, i.e. NADH cytochrome c reductase (rotenone insensitive) (37%).
摘要
  1. 在实验性心肌梗死后的犬血清中产生了抗心脏线粒体自身抗体。2. 在蔗糖/三氯化物缓冲液中反复冻融的心脏线粒体,其呼吸控制率所测定的功能完整性以及在补体结合试验中作为抗原的能力均得以保留。在氯化钾/三氯化物缓冲液中冻融的线粒体,经过一次冻融循环后,其功能完整性和自身抗原活性均丧失。3. 用丙酮/水混合物提取心脏线粒体以去除膜中的磷脂,导致线粒体在补体结合试验中反应的能力完全丧失,但在吸收实验中不影响膜结合自身抗体的能力。4. 用浓度不断增加的胰蛋白酶处理线粒体膜,导致膜蛋白损失高达约50%,膜的自身抗原活性逐渐降低,但不损害膜结合自身抗体的能力。5. 用神经氨酸酶去除线粒体膜高达90%的唾液酸,导致膜的补体结合自身抗原活性显著增加,而在吸收实验中不改变膜结合自身抗体的明显能力。6. 线粒体膜暴露于自身抗体和补体后,导致线粒体内膜酶即细胞色素氧化酶(48%)和线粒体外膜酶即NADH细胞色素c还原酶(鱼藤酮不敏感)(37%)均受到抑制。

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