通过测定丝状肌动蛋白和检测膜改变来测定血小板活化。

Acta histochemica. Supplementband Pub Date : 1991-01-01
P Spangenberg, D Tschöpe, J Esser, B Schwippert, B Kehrel, P Rösen, F A Gries
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引用次数: 0

摘要

凝血酶刺激人凝胶过滤血小板在未搅拌系统(无聚集)导致肌动蛋白聚合。随着肌动蛋白聚合,活化标记物(cd63 -糖蛋白53,一种53 kD溶酶体蛋白和cd62 -GMP 140,一种140 kD α颗粒蛋白)在血小板膜上增加,以及血小板反应蛋白单克隆抗体的特异性结合(p10)。因此,两种检测方法并行运行,并能灵敏地指示血小板活化。我们的数据还表明,当血小板受到凝血酶的挑战并涉及细胞骨架结构的重组时,颗粒融合后的亚细胞结构暴露是一个非常早期的事件。细胞松弛素E完全抑制凝血素诱导的肌动蛋白聚合和血小板聚集,但仅部分抑制凝血素诱导的cd63暴露。激活标记cd62和p10不受影响。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Determination of platelet activation by assaying filamentous actin and detecting membrane alterations.

Thrombin stimulation of human gel-filtered platelets in an unstirred system (without aggregation) results in actin polymerisation. Concomitantly with actin polymerisation the activation markers (CD 63--glycoprotein 53, a 53 kD lysosomal protein and CD 62--GMP 140, a 140 kD alpha granule protein) increase on the platelet membrane as well as the specific binding of monoclonal antibodies to thrombospondin (P 10). Consequently, both assays run in parallel and indicate sensitively platelet activation. Our data also indicate that exposure of subcellular structures following granule fusion is a very early event when platelets are challenged by thrombin and involve a reorganisation of cytoskeletal structures. Cytochalasin E inhibits completely the thrombin-induced actin polymerisation and the platelet aggregation but only partially the thrombin-induced exposure of CD 63. The activation markers CD 62 and P 10 were not influenced.

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