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凝血酶诱导聚集的人血小板的解聚

Deaggregation of human platelets aggregated by thrombin.

作者信息

Kinlough-Rathbone R L, Perry D W, Packham M A, Mustard J F

出版信息

Thromb Haemost. 1985 Feb 18;53(1):42-4.

PMID:2986309
Abstract

Human platelets that have undergone the release reaction do not deaggregate readily. We examined conditions under which washed human platelets can be deaggregated after they have undergone an extensive release reaction induced by thrombin (1 or 5 U/ml). To make fibrinogen receptors unavailable, either CP/CPK (or apyrase) was used to remove released ADP, or PGE1 was used to increase cAMP. Chymotrypsin was used to digest proteins that might link platelets, and heparin to interact with released proteins and interfere with their binding to platelets and to each other. Individually, none of these caused deaggregation; heparin did not inhibit the effect of thrombin because no antithrombin III was present. Platelets exposed to thrombin (1 U/ml) which was neutralized at 90 sec by hirudin, could be deaggregated by combinations of CP/CPK (or apyrase) and chymotrypsin, or PGE1 and chymotrypsin. When a higher concentration of thrombin was used (5 U/ml) these combinations caused platelets to deaggregate only when heparin was added before thrombin induced the release reaction. Thus, when extensive release occurs three mechanisms may come into play to link human platelets: one that requires the fibrinogen receptor; a heparin-sensitive reaction that may involve the binding of released proteins; and a linkage that can be disrupted only by proteolysis, providing the other two mechanisms are also inhibited.

摘要

经历释放反应后的人血小板不易解聚。我们研究了在凝血酶(1或5 U/ml)诱导广泛释放反应后,洗涤过的人血小板能够解聚的条件。为了使纤维蛋白原受体无法发挥作用,要么使用CP/CPK(或腺苷三磷酸双磷酸酶)去除释放的ADP,要么使用前列腺素E1增加环磷酸腺苷(cAMP)。使用胰凝乳蛋白酶消化可能连接血小板的蛋白质,使用肝素与释放的蛋白质相互作用并干扰它们与血小板之间以及彼此之间的结合。单独使用这些方法均未导致解聚;由于不存在抗凝血酶III,肝素并未抑制凝血酶的作用。暴露于凝血酶(1 U/ml)且在90秒时被水蛭素中和的血小板,可通过CP/CPK(或腺苷三磷酸双磷酸酶)与胰凝乳蛋白酶的组合,或前列腺素E1与胰凝乳蛋白酶的组合实现解聚。当使用更高浓度的凝血酶(5 U/ml)时,只有在凝血酶诱导释放反应前加入肝素,这些组合才会使血小板解聚。因此,当发生广泛释放时,可能有三种机制参与连接人血小板:一种需要纤维蛋白原受体;一种对肝素敏感的反应,可能涉及释放蛋白的结合;还有一种连接只能通过蛋白水解来破坏,前提是另外两种机制也受到抑制。

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