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决定补体激活中同种型特异性差异的人免疫球蛋白G的结构特征。

Structural features of human immunoglobulin G that determine isotype-specific differences in complement activation.

作者信息

Tao M H, Smith R I, Morrison S L

机构信息

Department of Microbiology and Molecular Genetics, University of California, Los Angeles 90024.

出版信息

J Exp Med. 1993 Aug 1;178(2):661-7. doi: 10.1084/jem.178.2.661.

Abstract

Although very similar in sequence, the four subclasses of human immunoglobulin G (IgG) differ markedly in their ability to activate complement. Glu318-Lys320-Lys322 has been identified as a key binding motif for the first component of complement, C1q, and is present in all isotypes of Ig capable of activating complement. This motif, however, is present in all subclasses of human IgG, including those that show little (IgG2) or even no (IgG4) complement activity. Using point mutants of chimeric antibodies, we have identified specific residues responsible for the differing ability of the IgG subclasses to fix complement. In particular, we show that Ser at position 331 in gamma 4 is critical for determining the inability of that isotype to bind C1q and activate complement. Additionally, we provide further evidence that levels of C1q binding do not necessarily correlate with levels of complement activity, and that C1q binding alone is not sufficient for complement activation.

摘要

尽管人类免疫球蛋白G(IgG)的四个亚类在序列上非常相似,但它们激活补体的能力却有显著差异。Glu318-Lys320-Lys322已被确定为补体第一成分C1q的关键结合基序,并且存在于所有能够激活补体的Ig同种型中。然而,该基序存在于人类IgG的所有亚类中,包括那些补体活性很低(IgG2)甚至没有(IgG4)的亚类。通过嵌合抗体的点突变体,我们确定了负责IgG亚类补体结合能力差异的特定残基。特别是,我们发现γ4亚类中第331位的丝氨酸对于决定该同种型无法结合C1q并激活补体至关重要。此外,我们提供了进一步的证据表明,C1q结合水平不一定与补体活性水平相关,并且仅C1q结合不足以激活补体。

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本文引用的文献

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The Clq receptor site on immunoglobulin G.免疫球蛋白G上的Clq受体位点。
Nature. 1980 Nov 27;288(5789):338-44. doi: 10.1038/288338a0.
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Immunoglobulin G: functional sites.免疫球蛋白G:功能位点。
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