首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Initiation of the alternative pathway of complement: recognition of activators by bound C3b and assembly of the entire pathway from six isolated proteins.
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Initiation of the alternative pathway of complement: recognition of activators by bound C3b and assembly of the entire pathway from six isolated proteins.

机译:补体替代途径的开始:通过结合的C3b识别激活剂并从六个分离的蛋白质组装整个途径。

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摘要

An intact alternative pathway of complement activation was assembled from six isolated proteins present at their respective physiological concentrations (C3, 1200 microgram/ml: factor B, 200 microgram/ml; factor D, 2 microgram/ml; beta1H, 560 microgram/ml; C3b inactivator, 34 microgram/ml; and native properdin, 20 microgram/ml). Initiation of the pathway required the presence of five of these proteins not including properdin. The initial C3 convertase of the system was shown to be a fluid-phase rather than a surface-bound enzyme. The ability of the pathway to discriminate between activator and nonactivator was found to reside in the bound C3b molecule. When bound to the surface of an activator through its labile binding site, C3b interacts with surface structures of the activator through another site on the molecule. This interaction results in diminished beta1H binding to C3b and thereby allows the bound C3b molecule to escape control and participate in C3 convertase formation. Thus, initiation of the alternative pathway is a two-step process, the first being non-specific and the second being discriminatory.
机译:完整的补体激活旁路途径是由六个分离的蛋白质组成的,这些蛋白质分别以各自的生理浓度存在(C3,1200微克/毫升:B因子,200微克/毫升; D因子,2微克/毫升; beta1H,560微克/毫升; C3b灭活剂为34微克/毫升;天然备解素为20微克/毫升。该途径的起始需要存在五个这样的蛋白质,不包括备解素。系统的初始C3转化酶显示为液相而不是表面结合酶。发现该途径区分活化剂和非活化剂的能力存在于结合的C3b分子中。当C3b通过其不稳定的结合位点与活化剂的表面结合时,C3b通过分子上的另一个位点与活化剂的表面结构相互作用。这种相互作用导致与C3b结合的beta1H减少,从而使结合的C3b分子逃避控制并参与C3转化酶的形成。因此,替代途径的启动是一个两步过程,第一步是非特异性的,第二步是歧视性的。

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