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纤维蛋白原与其血小板受体的结合。

The binding of fibrinogen to its platelet receptor.

作者信息

Marguerie G A, Ardaillou N, Cherel G, Plow E F

出版信息

J Biol Chem. 1982 Oct 25;257(20):11872-5.

PMID:6288701
Abstract

Specific receptors for fibrinogen can be induced on platelets by a variety of stimuli. In this study, two independent approaches have implicated the D domain of fibrinogen in its interaction with the platelet. Immunochemically purified Fab fragments of anti-fibrinogen and anti-D inhibited 125I-fibrinogen binding to platelets in a dose-dependent fashion and platelet aggregation. In contrast, Fab fragments of anti-E produced only a slight inhibition of fibrinogen binding and nonimmune Fab fragments had no effect. Fibrinogen was digested with plasmin in the presence of 5 mM calcium and fragment D and E of Mr 100,000 and 50,000, respectively, were isolated. This D fragment inhibited 125I-fibrinogen binding to platelets in a concentration-dependent fashion, whereas the E fragment was ineffective. With 125I-fibrinogen at 0.17 microM, nonlabeled fibrinogen inhibited binding by 50% at 0.7 microM, whereas 170 microM fragment D was required to produce 50% inhibition. D fragment of Mr 80,000, generated in the absence of calcium, was noninhibitory. These observations provide strong evidence for the participation of the D domain in the binding of fibrinogen by its platelet receptor and suggest that the recognition site is lost in the conversion of the Mr 100,000 to 80,000 D species.

摘要

多种刺激可诱导血小板产生纤维蛋白原的特异性受体。在本研究中,两种独立的方法表明纤维蛋白原的D结构域参与其与血小板的相互作用。免疫化学纯化的抗纤维蛋白原和抗D的Fab片段以剂量依赖方式抑制125I-纤维蛋白原与血小板的结合及血小板聚集。相比之下,抗E的Fab片段仅对纤维蛋白原结合产生轻微抑制,非免疫Fab片段则无作用。在5 mM钙存在下用纤溶酶消化纤维蛋白原,分别分离出分子量为100,000和50,000的片段D和E。该D片段以浓度依赖方式抑制125I-纤维蛋白原与血小板的结合,而E片段无作用。对于0.17 microM的125I-纤维蛋白原,未标记的纤维蛋白原在0.7 microM时抑制结合50%,而产生50%抑制则需要170 microM的片段D。在无钙条件下产生的分子量为80,000的D片段无抑制作用。这些观察结果为D结构域参与纤维蛋白原与其血小板受体的结合提供了有力证据,并表明在分子量为100,000的D片段转化为80,000的D片段过程中识别位点丢失。

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