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蛋白质二硫键异构酶介导血小板聚集和分泌。

Protein disulphide isomerase mediates platelet aggregation and secretion.

作者信息

Essex D W, Li M

机构信息

Department of Medicine, State University of New York, Health Science Center at Brooklyn, 11203, USA.

出版信息

Br J Haematol. 1999 Mar;104(3):448-54. doi: 10.1046/j.1365-2141.1999.01197.x.

Abstract

Platelet surface thiols and disulphides play an important role in platelet responses. Agents that reduce disulphide bonds expose the fibrinogen receptor in platelets and activate the purified glycoprotein (GP) IIbIIIa receptor. Protein disulphide isomerase (PDI), an enzyme that rearranges disulphides bonds, is found on the platelet surface where it is catalytically active. We investigated the role of PDI in platelet responses using (1) rabbit anti-PDI IgG specific for PDI, (2) a competing substrate (scrambled ribonuclease A), and (3) the PDI inhibitor, bacitracin. Fab fragments of the rabbit anti-PDI IgG inhibited platelet responses to the agonists tested (ADP and collagen), whereas Fab fragments prepared identically from normal rabbit IgG had no inhibitory effect. Scrambled ribonuclease A blocked platelet aggregation and secretion, but native ribonuclease A did not. When biphasic platelet aggregation was examined using platelets in citrated plasma, the principle effect of bacitracin was on second phase or irreversible aggregation responses and the accompanying secretion. Using flow cytometry and an antibody specific for activated GPIIbIIIa (PAC-1), the rabbit anti-PDI Fab fragments substantially inhibited activation of GPIIbIIIa when added before, but not after, platelet activation. In summary, we have demonstrated that protein disulphide isomerase mediates platelet aggregation and secretion, and that it activates GPIIbIIIa, suggesting this receptor as the target of the enzyme.

摘要

血小板表面的硫醇和二硫键在血小板反应中起重要作用。还原二硫键的试剂会使血小板中的纤维蛋白原受体暴露,并激活纯化的糖蛋白(GP)IIbIIIa受体。蛋白二硫键异构酶(PDI)是一种可重排二硫键的酶,存在于血小板表面并具有催化活性。我们使用(1)对PDI具有特异性的兔抗PDI IgG、(2)一种竞争性底物( scrambled核糖核酸酶A)和(3)PDI抑制剂杆菌肽,研究了PDI在血小板反应中的作用。兔抗PDI IgG的Fab片段抑制了血小板对所测试激动剂(ADP和胶原)的反应,而用正常兔IgG以相同方式制备的Fab片段则没有抑制作用。 scrambled核糖核酸酶A可阻断血小板聚集和分泌,但天然核糖核酸酶A则不能。当使用枸橼酸盐血浆中的血小板检测双相血小板聚集时,杆菌肽的主要作用是作用于第二相或不可逆聚集反应以及伴随的分泌。使用流式细胞术和针对活化GPIIbIIIa的特异性抗体(PAC-1),兔抗PDI Fab片段在血小板活化之前而非之后添加时,可显著抑制GPIIbIIIa的活化。总之,我们已经证明蛋白二硫键异构酶介导血小板聚集和分泌,并激活GPIIbIIIa,提示该受体是该酶的作用靶点。

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