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β1H球蛋白对替代补体途径的调节作用。

Modulation of the alternative complement pathways by beta 1 H globulin.

作者信息

Whaley K, Ruddy S

出版信息

J Exp Med. 1976 Nov 2;144(5):1147-63. doi: 10.1084/jem.144.5.1147.

Abstract

C3b inactivator accelerator (A-C3bINA) was isolated from human plasma. An antiserum produced against the purified protein gave a reaction of identity with beta 1 H, a well-documented contaminant of C3 preparations. Beta 1 H appears to be composed of a single polypeptide chain containing a significant quantity of carbohydrate, and having a sedimentation coefficient of 5.6 on analytical, and 6.4 on sucrose density gradient ultracentrifugation. Its mol wt based on SDS polyacrylamide gel electrophoresis and equilibrium sedimentation is approximately 150,000, whereas it elutes from Sephadex G200 with an apparent mol wt of 300,000, suggesting that beta 1 H is an asymmetric molecule. Beta 1 H potentiates the inactivation of C3b by C3b inactivator, binds to EAC43 to limit the formation of EAC43bB and EAC43bBP, and in contrast to C3b inactivator, it increases the rate of loss of hemolytic sites from EAC43bB and EAC43bBP. For the C3b inactivator-potentiating effect, beta 1 H and C3b inactivator must necessarily be simultaneously present. The kinetics of inactivation of C3b by C3b inactivator and beta 1 H are first order, suggesting that potentiation is not a multistep process. The mechanisms of binding to C3b and inhibition of the alternative pathway convertases C3bB and C3bBP are currently unknown.

摘要

C3b灭活因子加速剂(A - C3bINA)是从人血浆中分离出来的。针对纯化蛋白产生的抗血清与β1H产生了同一性反应,β1H是C3制剂中一种有充分记录的污染物。β1H似乎由一条含有大量碳水化合物的单多肽链组成,在分析超速离心时沉降系数为5.6,在蔗糖密度梯度超速离心中沉降系数为6.4。基于SDS聚丙烯酰胺凝胶电泳和平衡沉降法,其分子量约为150,000,而从葡聚糖G200洗脱时表观分子量为300,000,这表明β1H是一种不对称分子。β1H增强C3b灭活因子对C3b的灭活作用,与EAC43结合以限制EAC43bB和EAC43bBP的形成,与C3b灭活因子相反,它增加了EAC43bB和EAC43bBP溶血位点的丧失速率。对于C3b灭活因子增强作用,β1H和C3b灭活因子必须同时存在。C3b灭活因子和β1H对C3b的灭活动力学是一级反应,这表明增强作用不是一个多步骤过程。目前尚不清楚β1H与C3b结合以及抑制替代途径转化酶C3bB和C3bBP的机制。

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