首页> 美国卫生研究院文献>Biophysical Journal >Dynamics of platelet glycoprotein IIb-IIIa receptor expression and fibrinogen binding. II. Quantal activation parallels platelet capture in stir-associated microaggregation.
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Dynamics of platelet glycoprotein IIb-IIIa receptor expression and fibrinogen binding. II. Quantal activation parallels platelet capture in stir-associated microaggregation.

机译:血小板糖蛋白IIb-IIIa受体表达和纤维蛋白原结合的动力学。二。量子活化与搅拌相关的微聚集中的血小板捕获平行。

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摘要

There is broad agreement that platelet aggregation is generally dependent on fibrinogen (Fg) binding to the glycoprotein (GP) IIb-IIIa receptor expressed on the activated platelet surface. We therefore compared rates and extents of aggregation and of fibrinogen receptor expression and specific Fg binding to activated platelets, as a function of ADP concentration. Human citrated platelet-rich plasma (diluted 10-fold) was stirred with adenosine diphosphate (ADP) for 10 s or 2 min to measure rates and extent of aggregation, respectively, determined from the decrease in the total number of particles. The number of fibrinogen receptors and bound Fg were measured from mean fluorescence values obtained with FITC-labeled IgM monoclonal antibody PAC1 and the IgG monoclonal antibody, 9F9, respectively, using flow cytometry as presented in part I (Frojmovic et al., 1994). Because flow cytometric and aggregation measurements were routinely determined at room temperature and 37 degrees C, respectively, we also compared and found temperature-independent initial rates of aggregation. The fraction of platelets with fluorescence values above one critical threshold value, corresponding to maximally "activated" platelets (P*), increased with increasing activator concentration and correlated linearly with the fraction of platelets recruited into aggregates for ADP (r > 0.9). Aggregation was not rate-limited by fibrinogen receptor expression or by Fg binding. It appears that each platelet expresses its maximal Fg receptors at a critical ADP concentration, i.e., occupancy of ADP receptors. This, in turn, leads to rapid Fg occupancy and capture of such "quantally activated" platelets into aggregates.
机译:人们普遍认为,血小板凝集通常取决于纤维蛋白原(Fg)与活化血小板表面表达的糖蛋白(GP)IIb-IIIa受体的结合。因此,我们比较了ADP浓度的函数,聚集率,纤维蛋白原受体表达和特异性Fg与活化血小板结合的速率和程度。将人柠檬酸化的富含血小板的血浆(稀释10倍)与二磷酸腺苷(ADP)搅拌10 s或2分钟,分别测量凝聚速率和聚集程度,该速率和程度由颗粒总数的减少确定。纤维蛋白原受体的数目和结合的Fg分别由流式细胞术从FITC标记的IgM单克隆抗体PAC1和IgG单克隆抗体9F9获得的平均荧光值进行测量,方法见第I部分(Frojmovic等,1994)。因为流式细胞仪和聚集物的测量分别是在室温和37摄氏度下常规确定的,所以我们也比较并发现了与温度无关的初始聚集率。荧光值高于一个临界阈值的血小板比例对应于最大“激活”的血小板(P *),随活化剂浓度的增加而增加,并且与募集到ADP聚集物中的血小板比例成线性相关(r> 0.9)。聚集不受纤维蛋白原受体表达或Fg结合的速率限制。似乎每个血小板都在临界ADP浓度即ADP受体占有率时表达其最大的Fg受体。反过来,这导致快速的Fg占用,并将这种“定量激活的”血小板捕获为聚集体。

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