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血小板在全血中以及在存在免疫复合物或聚集的IgG的情况下与C1q的相互作用。

Platelet interactions with C1q in whole blood and in the presence of immune complexes or aggregated IgG.

作者信息

Peerschke E I, Ghebrehiwet B

机构信息

Department of Pathology, SUNY, Stony Brook 11794-7300.

出版信息

Clin Immunol Immunopathol. 1992 Apr;63(1):45-50. doi: 10.1016/0090-1229(92)90092-3.

Abstract

Previous studies identified specific receptors for C1q on human blood platelets in purified systems using monomeric C1q. To assess the physiologic potential of platelet C1q receptors, C1q binding was evaluated in whole blood and in the presence of immune complexes or aggregated IgG. Blood was obtained from healthy volunteers and collected directly into EDTA (1 vol 100mM EDTA:9 vol whole blood) and purified, 125I-labeled C1q or 125I-C1q associated with albumin-anti-albumin immune complexes. Samples were incubated at 22 or 37 degrees C for 60 min, and total cell bound C1q and platelet associated C1q were quantified. Platelet-bound, monomeric C1q or immune complex-associated C1q represented 40-50% of total peripheral blood cell-associated C1q. C1q binding was unaffected by the incubation temperature, but the preincubation of 125I-C1q with immune complexes enhanced binding two- to threefold. This binding was partially inhibited by preincubating platelets with either the collagen-like amino-terminal fragments of C1q (c-C1q) or a monoclonal antibody Fab fragment recognizing platelet Fc receptors. A more complete inhibition was achieved if platelets were preincubated with both agents. Similar observations were made using washed platelets and 125I-C1q associated with aggregated IgG. The role of C1q and platelet C1q receptors in enhancing aggregated-IgG binding to platelets was further supported by experiments demonstrating increased 125I-aggregated IgG binding to platelets not only after preincubation of 125I-aggregated IgG with C1q but also following platelet preincubation with C1q. These data suggest that C1q receptors may participate in the localization and presentation of C1q-associated immune complexes on the platelet surface and demonstrate that platelets contribute significantly to the C1q binding activity of peripheral blood.

摘要

以往的研究在纯化系统中使用单体C1q鉴定了人血小板上C1q的特异性受体。为了评估血小板C1q受体的生理潜能,在全血以及存在免疫复合物或聚集IgG的情况下对C1q结合进行了评估。从健康志愿者获取血液,直接收集到EDTA(1体积100mM EDTA:9体积全血)中,并加入纯化的、125I标记的C1q或与白蛋白-抗白蛋白免疫复合物相关的125I-C1q。样品在22或37℃孵育60分钟,对总细胞结合的C1q和血小板相关的C1q进行定量。血小板结合的单体C1q或免疫复合物相关的C1q占外周血细胞相关C1q总量的40-50%。C1q结合不受孵育温度的影响,但125I-C1q与免疫复合物的预孵育使结合增强了两到三倍。用C1q的胶原样氨基末端片段(c-C1q)或识别血小板Fc受体的单克隆抗体Fab片段预孵育血小板可部分抑制这种结合。如果血小板同时用这两种试剂预孵育,则可实现更完全的抑制。使用洗涤过的血小板和与聚集IgG相关的125I-C1q也得到了类似的观察结果。实验进一步证明,不仅125I-聚集IgG与C1q预孵育后,而且血小板与C1q预孵育后,125I-聚集IgG与血小板的结合增加,这进一步支持了C1q和血小板C1q受体在增强聚集IgG与血小板结合中的作用。这些数据表明,C1q受体可能参与C1q相关免疫复合物在血小板表面的定位和呈递,并表明血小板对外周血的C1q结合活性有显著贡献。

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