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慢性冷凝集素病患者新生C3b与红细胞结合效率增加。

Increased efficiency of binding of nascent C3b to the erythrocytes of chronic cold agglutinin disease.

作者信息

Parker C J, Soldato C M, Telen M J

出版信息

J Clin Invest. 1984 Sep;74(3):1050-62. doi: 10.1172/JCI111472.

Abstract

The pathogenesis of chronic cold agglutinin disease (CCAD) has been enigmatic. To determine if abnormal erythrocyte membrane constituents might provide the stimulus for antibody production, we compared the electrophoretic pattern of radiolabeled membrane glycoproteins of four patients with CCAD to that of normal control erythrocytes. For the CCAD erythrocytes, fluorographs revealed the appearance of an abnormal band whose molecular weight was estimated at 126,000 D. Using two-dimensional gel analysis and immunoblotting techniques, it was determined that the 126,000 D glycoprotein consisted predominately of polymeric glycophorin-alpha. Previous investigations had suggested that abnormalities in glycophorin-alpha influence the functional activity of the complement system. When purified complement (C)3 was activated in the fluid-phase by cobra venom factor complexes, CCAD erythrocytes bound nascent C3b 7-27 times more efficiently than normal erythrocytes. Normal erythrocytes could be induced to manifest the appearance of the 126,000 D band, and the increased efficiency of binding of nascent C3b by incubation with CCAD serum or with the purified cold agglutinin antibody plus autologous serum, but not with the purified antibody alone or the purified antibody plus EDTA-chelated autologous serum. These studies demonstrate that the interactions of IgM cold-reacting antibody and complement with glycophorin induce changes in the biophysical properties of the erythrocyte membrane which modify subsequent interactions with complement.

摘要

慢性冷凝集素病(CCAD)的发病机制一直不明。为了确定异常的红细胞膜成分是否可能为抗体产生提供刺激,我们将4例CCAD患者的放射性标记膜糖蛋白的电泳图谱与正常对照红细胞的电泳图谱进行了比较。对于CCAD红细胞,荧光自显影片显示出现了一条异常带,其分子量估计为126,000道尔顿。使用二维凝胶分析和免疫印迹技术确定,126,000道尔顿的糖蛋白主要由聚合血型糖蛋白α组成。先前的研究表明,血型糖蛋白α的异常会影响补体系统的功能活性。当纯化的补体(C)3在液相中被眼镜蛇毒因子复合物激活时,CCAD红细胞结合新生C3b的效率比正常红细胞高7 - 27倍。正常红细胞可以通过与CCAD血清或纯化的冷凝集素抗体加自体血清孵育而诱导出现126,000道尔顿的条带,并提高结合新生C3b的效率,但单独使用纯化抗体或纯化抗体加EDTA螯合的自体血清则不能。这些研究表明,IgM冷反应抗体和补体与血型糖蛋白的相互作用会诱导红细胞膜生物物理性质的变化,从而改变随后与补体的相互作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9726/425264/37f4c5770373/jcinvest00135-0394-a.jpg

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