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一种用于定量人工表面上补体激活产物(iC3b、C3d、SC5b-9)吸附量的流式细胞免疫测定法。

A flow cytometric immunoassay to quantify adsorption of complement activation products (iC3b, C3d, SC5b-9) on artificial surfaces.

作者信息

Gemmell C H

机构信息

Department of Medicine, University of Toronto.

出版信息

J Biomed Mater Res. 1997 Dec 15;37(4):474-80. doi: 10.1002/(sici)1097-4636(19971215)37:4<474::aid-jbm5>3.0.co;2-i.

DOI:10.1002/(sici)1097-4636(19971215)37:4<474::aid-jbm5>3.0.co;2-i
PMID:9407295
Abstract

Crosslinked agarose microspheres and various polystyrene microspheres were analyzed for complement components after incubation with serum at 37 degrees C for times up to 2 h. Quantification involved direct flow cytometric analysis of the beads after the bound complement proteins were indirectly fluorescently tagged by use of a monoclonal antibody against a complement protein: C5b-9, iC3b, C3d, C4d, Bb, C3a, and C1q. Calibration with fluorescein microbead standards demonstrated that the membrane attack complex (SC5b-9) was surface bound on all surfaces and that the surface concentration gradually increased to levels as high as 0.5 micrograms/cm2. Further, the surface bound represented a substantial percentage of the total generated. The iC3b level on polystyrene beads rapidly reached 0.09 micrograms/cm2 and the C3d levels were an order of magnitude less. On agarose beads the iC3b levels continually rose to 0.17 micrograms/cm2 and, as before, the C3d levels were substantially lower. The surface concentration of C4d and Bb on both surfaces were significant but less than 1.0 ng/cm2. There was minimal evidence of C3a and C1q adsorption for any surface. Use of amino-polystyrene beads moderately reduced the level of bound iC3b, C3d, and SC5b-9, whereas carboxylated beads reduced the levels by almost a factor of two. The appreciable amounts of iC3b and SC5b-9 consistently noted on the artificial surfaces tested in this paper suggests that for these two activation products in vitro analysis of material induced complement activation should also include surface analysis.

摘要

将交联琼脂糖微球和各种聚苯乙烯微球与血清在37℃孵育长达2小时后,分析其补体成分。定量分析包括在通过使用针对补体蛋白(C5b - 9、iC3b、C3d、C4d、Bb、C3a和C1q)的单克隆抗体对结合的补体蛋白进行间接荧光标记后,对微球进行直接流式细胞术分析。用荧光微球标准品校准表明,膜攻击复合物(SC5b - 9)在所有表面均有表面结合,且表面浓度逐渐增加至高达0.5微克/平方厘米的水平。此外,表面结合物占总生成量的相当大比例。聚苯乙烯微球上的iC3b水平迅速达到0.09微克/平方厘米,而C3d水平低一个数量级。在琼脂糖微球上,iC3b水平持续上升至0.17微克/平方厘米,和之前一样,C3d水平显著更低。两种表面上C4d和Bb的表面浓度均显著,但低于1.0纳克/平方厘米。几乎没有证据表明任何表面有C

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