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从Raji细胞膜中增溶调节C3b功能的活性物质。

Solubilization of an activity regulating C3b function from Raji cell membranes.

作者信息

Carlson P, Ruddy S, Conrad D H

出版信息

Immunology. 1982 May;46(1):163-73.

Abstract

A fraction of isolated Raji cell membranes solubilized with 2m KBr which was capable of inhibiting C3-dependent rosettes was examined for its ability to inhibit the alternative pathway of complement. It was shown to decrease alternative pathway-dependent haemolysis of sheep erythrocytes and to accelerate decay of factor B from these cells. It had no effect on C2 decay, the classical pathway analog of factor B. Inhibitory activity solubilized from Raji cells was not removed by immunoadsorption with anti-factor H or anti-factor I, two well-characterized serum C3b-control proteins. It also differed in two functional respects from these proteins. Firstly, it failed to result in cleavage of a peptide bone in C3 which is characteristic of factor I; secondly, its inhibitory activity did not synergize with factor I in inhibiting the alternative pathway, unlike factor H. These results suggest that Raji cells contain a regulatory factor in their membranes for the alternative pathway of complement which is distinct from factors H and I.

摘要

用2m KBr溶解的、能够抑制C3依赖性玫瑰花结形成的部分分离的Raji细胞膜,检测其抑制补体替代途径的能力。结果显示,它能降低绵羊红细胞依赖替代途径的溶血作用,并加速这些细胞中B因子的衰变。它对C2衰变(B因子的经典途径类似物)没有影响。用抗H因子或抗I因子(两种特性明确的血清C3b控制蛋白)进行免疫吸附,不能去除从Raji细胞中溶解出的抑制活性。它在两个功能方面也与这些蛋白不同。首先,它不能导致C3中肽键的裂解,而这是I因子的特征;其次,与H因子不同,其抑制活性在抑制替代途径方面不能与I因子协同作用。这些结果表明,Raji细胞的膜中含有一种补体替代途径的调节因子,它与H因子和I因子不同。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8711/1555332/72437b618303/immunology00226-0166-a.jpg

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