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人IgG针对6型A组链球菌的调理活性要求:净碱性电荷和完整的Fc区域。

Requirements for the opsonic activity of human IgG directed to type 6 group A streptococci: net basic charge and intact Fc region.

作者信息

Fischetti V A

出版信息

J Immunol. 1983 Feb;130(2):896-902.

PMID:6336773
Abstract

By two independent techniques for separating human opsonic IgG for group A type 6 streptococci into fast- and slow-migrating fractions, it was found that the opsonic activity was localized within the basic charge population. This charge dependence was found to be a characteristic of the IgG isolated from three individuals. When the fast- and slow-migrating IgG fractions were tested for their ability to bind to purified M6 protein, antibodies in both opsonic and nonopsonic populations exhibited binding activity, with the majority being located within the opsonic IgG in two of the three individuals; the third displayed greater binding in the nonopsonic population. The functional difference observed in the antibody populations to this M antigen may be a reflection of the net charge within the area of the antibody binding site, which suggests that the opsonic antibodies need to bind to acidic residues along the outer surface of the fibrillar M protein molecule. F(ab')2 fragments prepared from both human and rabbit type 6 opsonic IgG were still able to bind to the M6 molecule but were unable to mediate opsonization of type 6 streptococci. However, the F(ab')2 fragments had the capacity to enhance or amplify the opsonic activity of low concentrations of opsonic IgG molecules. The results suggest that the M protein molecule may function as an active inhibitor of phagocytosis and that F(ab')2 fragments from opsonic IgG have the capacity to neutralize the "active" determinants on the molecule, thus allowing lower concentrations of IgG with functional Fc receptors to mediate phagocytosis.

摘要

通过两种独立的技术,将针对A群6型链球菌的人调理素IgG分离为快速迁移和慢速迁移组分,发现调理活性定位于碱性电荷群体中。这种电荷依赖性是从三个个体中分离出的IgG的特征。当测试快速迁移和慢速迁移的IgG组分与纯化的M6蛋白结合的能力时,调理素群体和非调理素群体中的抗体均表现出结合活性,在三个个体中的两个个体中,大多数结合活性位于调理素IgG中;第三个个体在非调理素群体中表现出更强的结合活性。在针对这种M抗原的抗体群体中观察到的功能差异可能反映了抗体结合位点区域内的净电荷,这表明调理素抗体需要结合到纤维状M蛋白分子外表面的酸性残基上。从人和兔6型调理素IgG制备的F(ab')2片段仍能够与M6分子结合,但无法介导6型链球菌的调理作用。然而,F(ab')2片段具有增强或放大低浓度调理素IgG分子调理活性的能力。结果表明,M蛋白分子可能作为吞噬作用的活性抑制剂起作用,并且来自调理素IgG的F(ab')2片段具有中和该分子上“活性”决定簇的能力,从而允许具有功能性Fc受体的较低浓度的IgG介导吞噬作用。

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