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C1q与C3或C4之间的复合物:经典补体途径激活的新型特异性标志物。

Complexes between C1q and C3 or C4: novel and specific markers for classical complement pathway activation.

作者信息

Wouters Diana, Wiessenberg Hans D, Hart Margreet, Bruins Peter, Voskuyl Alexandre, Daha Mohamed R, Hack C Erik

机构信息

Department of Immunopathology, Sanquin Research and Laboratory for Experimental and Clinical Immunology, Academic Medical Centre, Amsterdam, Netherlands.

出版信息

J Immunol Methods. 2005 Mar;298(1-2):35-45. doi: 10.1016/j.jim.2004.12.018.

DOI:10.1016/j.jim.2004.12.018
PMID:15847795
Abstract

Classical pathway activation is often assessed by measuring circulating levels of activated C4. However, this parameter does not discriminate between activation through the classical or the lectin pathway. We hypothesized that during classical pathway activation, complexes are formed between C1q and activated C4 or C3. Using ELISA, we investigated whether such complexes constitute specific markers for classical pathway activation. In vitro, C1q-C3d/C4d complexes were generated upon incubation of normal recalcified plasma with aggregated IgG or an anti-C1q mAb that activates C1 (mAb anti-C1q-130). In contrast, during incubation with C1s or trypsin, C1q-C3d/C4d complexes were not generated, which excludes an innocent bystander effect. Additionally, C1q-C3d/C4d complexes were not generated during activation of the alternative or the lectin pathway. Repeated freezing and thawing did not influence levels of C1q-C3d/C4d complexes in recalcified plasma. To measure C1q-complement complexes in plasma samples, we separated unbound complement proteins from C1q-C3d/C4d complexes in the samples prior to testing with ELISA. In samples from patients undergoing cardiopulmonary bypass surgery or suffering from rheumatoid arthritis, we found higher levels of C1q-C4 complexes than in samples from healthy individuals. We conclude that complexes between C1q and C4 or C3 are specific markers of classical complement pathway activation.

摘要

经典途径的激活通常通过测量活化C4的循环水平来评估。然而,该参数无法区分通过经典途径还是凝集素途径的激活。我们假设在经典途径激活过程中,C1q与活化的C4或C3之间会形成复合物。我们使用酶联免疫吸附测定法(ELISA)研究了这些复合物是否构成经典途径激活的特异性标志物。在体外,将正常重新钙化的血浆与聚集的IgG或激活C1的抗C1q单克隆抗体(抗C1q-130单克隆抗体)孵育后,会产生C1q-C3d/C4d复合物。相反,在与C1s或胰蛋白酶孵育期间,不会产生C1q-C3d/C4d复合物,这排除了无辜旁观者效应。此外,在替代途径或凝集素途径激活过程中不会产生C1q-C3d/C4d复合物。反复冻融不会影响重新钙化血浆中C1q-C3d/C4d复合物的水平。为了测量血浆样本中的C1q-补体复合物,我们在使用ELISA检测之前,将样本中的未结合补体蛋白与C1q-C3d/C4d复合物分离。在接受体外循环手术或患有类风湿性关节炎的患者样本中,我们发现C1q-C4复合物的水平高于健康个体的样本。我们得出结论,C1q与C4或C3之间的复合物是经典补体途径激活的特异性标志物。

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