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血小板凝集蛋白p37通过与膜糖蛋白IV结合导致血小板凝集。

Platelet agglutinating protein p37 causes platelet agglutination through its binding to membrane glycoprotein IV.

作者信息

Lian E C, Siddiqui F A, Jamieson G A, Tandon N N

机构信息

Medical Service, Veterans Administration Medical Center, Miami, Florida 33125.

出版信息

Thromb Haemost. 1991 Jan 23;65(1):102-6.

PMID:2024231
Abstract

A 37 kDa platelet agglutinating protein (PAP p37) has previously been shown to be present in a subset of patients with thrombotic thrombocytopenic purpura and has been purified from their plasma. Using solubilized platelet membrane proteins from normal donors, it was shown by Western blotting that 125I-p37 bound to a membrane protein of 97 kDa (red/unred). Furthermore, the same protein was identified by reverse immunoblotting in which purified p37 was electrophoresed, transferred to the nitrocellulose sheet and incubated with solubilized normal platelet membrane proteins. The complex formed between p37 and the membrane protein was identified by autoradiography using polyclonal and monoclonal (OKM5) anti-GPIV antibodies, but was not detected by polyclonal antibody to GPIIIa. Similar studies with purified platelet GPIV under both reducing and non-reducing conditions demonstrated the binding of 125I-p37. Polyclonal and monoclonal antibodies to GPIV completely inhibited the platelet agglutination induced by TTP plasma containing p37, however, normal rabbit IgG, rabbit anti-GPIIIa IgG, and murine monoclonal anti-GPIIb/IIIa (10E5) antibodies had no effect. These data indicate that platelet GPIV is the receptor site for PAP p37.

摘要

先前已证明,一种37 kDa的血小板凝集蛋白(PAP p37)存在于一部分血栓性血小板减少性紫癜患者中,并且已从他们的血浆中纯化出来。利用来自正常供体的可溶性血小板膜蛋白,通过蛋白质免疫印迹法显示,125I-p37与一种97 kDa的膜蛋白(红色/未染色)结合。此外,通过反向免疫印迹法鉴定出了相同的蛋白,即在该方法中,将纯化的p37进行电泳,转移至硝酸纤维素膜上,然后与可溶性正常血小板膜蛋白一起孵育。利用多克隆抗体和单克隆(OKM5)抗GPIV抗体通过放射自显影法鉴定出了p37与膜蛋白之间形成的复合物,但未被抗GPIIIa多克隆抗体检测到。在还原和非还原条件下对纯化的血小板GPIV进行的类似研究证明了125I-p37的结合。抗GPIV多克隆抗体和单克隆抗体完全抑制了含p37的血栓性血小板减少性紫癜血浆诱导的血小板凝集,然而,正常兔IgG、兔抗GPIIIa IgG和鼠抗GPIIb/IIIa单克隆抗体(10E5)则没有作用。这些数据表明血小板GPIV是PAP p37的受体位点。

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