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人血小板的凝血酶受体:糖蛋白I的凝血酶结合及抗凝血酶特性

Thrombin receptors of human platelets: thrombin binding and antithrombin properties of glycoprotein I.

作者信息

Ganguly P, Gould N L

出版信息

Br J Haematol. 1979 May;42(1):137-45. doi: 10.1111/j.1365-2141.1979.tb03706.x.

Abstract

Washed human platelets were solubilized and the proteins were separated by preparative gel electrophoresis in the presence of sodium dodecyl sulphate. The gel was cut into slices and the effect of the eluted proteins on the clotting of fibrinogen by thrombin was evaluated. The isolate from only one gel slice strongly inhibited the clotting of fibrinogen. The prolongation of the clotting time was dependent on the concentration of the protein and reached a plateau around 5 microgram. Gel electrophoresis of this isolate showed a prominent glycoprotein with an apparent Mr=150 000. Gel filtration studies with [125I]thrombin showed that the protein isolate bound a significant amount of thrombin which could be displaced with unlabelled thrombin. Another preparation from the same gel or purified gamma-globulin did not bind thrombin or prolong the clotting time of fibrinogen. Glycoprotein I was isolated from human platelets by affinity chromatography on lectin-Sepharose columns. The isolated glycoprotein prolonged the clotting of fibrinogen and bound [125I]thrombin which could be displaced by unlabelled thrombin. It is proposed that the high affinity receptor of thrombin on human platelets is glycoprotein I. In addition, the antithrombin activity of intact platelets is due to binding of thrombin to this glycoprotein.

摘要

将洗涤过的人血小板溶解,蛋白质在十二烷基硫酸钠存在下通过制备性凝胶电泳进行分离。将凝胶切成薄片,并评估洗脱蛋白质对凝血酶使纤维蛋白原凝结的影响。仅从一个凝胶切片中分离出的物质强烈抑制纤维蛋白原的凝结。凝血时间的延长取决于蛋白质的浓度,在约5微克时达到平台期。该分离物的凝胶电泳显示出一种明显的糖蛋白,表观分子量为150000。用[125I]凝血酶进行的凝胶过滤研究表明,该蛋白质分离物结合了大量的凝血酶,未标记的凝血酶可将其置换。来自同一凝胶的另一种制剂或纯化的γ-球蛋白不结合凝血酶,也不延长纤维蛋白原的凝血时间。通过凝集素-琼脂糖柱亲和层析从人血小板中分离出糖蛋白I。分离出的糖蛋白延长了纤维蛋白原的凝结时间,并结合了[125I]凝血酶,未标记的凝血酶可将其置换。有人提出,人血小板上凝血酶的高亲和力受体是糖蛋白I。此外,完整血小板的抗凝血酶活性是由于凝血酶与该糖蛋白的结合。

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