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人免疫球蛋白A与B族链球菌II型的非免疫性结合

Nonimmune binding of human immunoglobulin A to type II group B streptococci.

作者信息

Anthony B F, Concepcion N F, Puentes S M, Payne N R

机构信息

Department of Pediatrics, Harbor-UCLA Medical Center, University of California, Los Angeles School of Medicine, Torrance 90509.

出版信息

Infect Immun. 1990 Jun;58(6):1789-95. doi: 10.1128/iai.58.6.1789-1795.1990.

DOI:10.1128/iai.58.6.1789-1795.1990
PMID:2187808
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC258724/
Abstract

The binding of 125I-labeled human myeloma immunoglobulin A (IgA) to four type II strains and one nontypable strain of group B streptococci was measured after streptococcal chains were broken by brief sonication. Some IgA binding was observed with all strains, but specific binding (binding that was inhibited by excess unlabeled IgA, was dose dependent, and was saturable) occurred only with those strains possessing the trypsin-sensitive beta component of the c protein. Similar amounts of binding were observed with myeloma IgA and IgA1 purified from normal serum. Specific binding was more rapid at 25 degrees C than at 0 or 37 degrees C and reached a plateau in 6 to 8 h. Binding was drastically reduced (85 to 90%) when streptococci had been heated (90 degrees C for 1 h). Most radioactivity bound to group B streptococci could be displaced (greater than 60% in 3 days) by the addition of excess unlabeled IgA. The binding capacity of one strain (10(8) streptococci in 1 ml of buffer) was saturated by approximately 24 micrograms of IgA. When transformed for Scatchard analysis, these data indicated that there was a specific binding capacity of 16,000 molecules of monomeric serum IgA per single streptococcal cell. The dissociation constant for IgA binding was 19.3 nM. Since enzyme-linked immunosorbent assay studies showed that the myeloma IgA used for the studies described above was IgA1, our quantitative data apply only to the binding of this subclass to group B streptococci. However, an enzyme-linked immunosorbent-filtration assay showed that both IgA1 and IgA2 bound to a type II group B streptococcus bearing the c protein.

摘要

在用短暂超声处理破坏链球菌链后,测定了125I标记的人骨髓瘤免疫球蛋白A(IgA)与四株II型菌株和一株B组链球菌不可分型菌株的结合情况。在所有菌株中均观察到一定程度的IgA结合,但只有那些具有对胰蛋白酶敏感的c蛋白β组分的菌株才会出现特异性结合(即被过量未标记IgA抑制、呈剂量依赖性且可饱和的结合)。从正常血清中纯化的骨髓瘤IgA和IgA1观察到相似的结合量。特异性结合在25℃时比在0℃或37℃时更快,并且在6至8小时内达到平台期。当链球菌被加热(90℃ 1小时)时,结合显著降低(85%至90%)。加入过量未标记IgA后,与B组链球菌结合的大部分放射性可被置换(3天内大于60%)。一株菌株(1ml缓冲液中有108个链球菌)的结合能力在加入约24μg IgA时达到饱和。经转换用于Scatchard分析后,这些数据表明每个单个链球菌细胞对单体血清IgA的特异性结合能力为16,000个分子。IgA结合的解离常数为19.3 nM。由于酶联免疫吸附测定研究表明上述研究中使用的骨髓瘤IgA是IgA1,我们的定量数据仅适用于该亚类与B组链球菌的结合。然而,酶联免疫吸附过滤测定表明,IgA1和IgA2均与携带c蛋白的II型B组链球菌结合。

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本文引用的文献

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