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螺旋寡核苷酸与两种单克隆MRL-1pr/1pr抗DNA自身抗体的紫外线交联。重链和轻链与DNA结合的变化。

Ultraviolet cross-linking of helical oligonucleotides to two monoclonal MRL-1pr/1pr anti-DNA autoantibodies. Variations in H and L chain binding to DNA.

作者信息

Jang Y J, Stollar B D

机构信息

Department of Biochemistry, School of Medicine, Tufts University, Boston, MA 02111.

出版信息

J Immunol. 1990 Nov 15;145(10):3353-9.

PMID:2230120
Abstract

Experiments were performed to determine whether both H and L chains of different anti-native DNA autoantibodies are uniformly involved in binding to DNA. Two purified monoclonal mouse (MRL-1pr/1pr) IgG autoantibodies, H241 and 2C10, were tested. They both bound synthetic helical oligonucleotides of 10 to 20 base pairs in a gel electrophoresis retardation assay but differed in their preferences for given base sequences. Exposure of antibody-radiolabeled oligonucleotide mixtures to UV light (254 nm) for 10 min led to specific covalent cross-linking of oligonucleotide to both the H and the L chains of H241 but only to the H chain of 2C10. Single labeling events were detected without higher aggregation. The oligonucleotides were not cross-linked to unrelated IgG, even after 2 h of irradiation. Cross-linked (radioactively labeled) H and L chains of H241 and 2C10 were isolated from denaturing electrophoresis gels and digested with lysyl endopeptidase and/or staphylococcal V8 protease. H241 and 2C10 H chains each yielded a major labeled peptide fragment, but the peptides from the two antibodies were different. These experiments measured only some of the antibody-DNA interactions, probably with bases in the major groove of the DNA. They indicated that two MRL-1pr/1pr IgG anti-native DNA antibodies differ in their H and L chain contacts with DNA and provide an approach to identifying affinity-labeled binding sites in the antibodies.

摘要

进行实验以确定不同抗天然DNA自身抗体的重链(H链)和轻链(L链)是否均参与与DNA的结合。测试了两种纯化的单克隆小鼠(MRL-1pr/1pr)IgG自身抗体H241和2C10。在凝胶电泳阻滞试验中,它们都能结合10至20个碱基对的合成螺旋寡核苷酸,但对特定碱基序列的偏好不同。将抗体放射性标记的寡核苷酸混合物暴露于紫外线(254nm)下10分钟,导致寡核苷酸与H241的H链和L链均发生特异性共价交联,但仅与2C10的H链发生交联。检测到单个标记事件,没有更高的聚集现象。即使照射2小时后,寡核苷酸也未与无关的IgG发生交联。从变性电泳凝胶中分离出交联的(放射性标记的)H241和2C10的H链和L链,并用赖氨酰内肽酶和/或葡萄球菌V8蛋白酶进行消化。H241和2C10的H链各自产生一个主要的标记肽片段,但来自两种抗体的肽不同。这些实验仅测量了一些抗体与DNA的相互作用,可能是与DNA大沟中的碱基相互作用。它们表明两种MRL-1pr/1pr IgG抗天然DNA抗体在其H链和L链与DNA的接触方面存在差异,并提供了一种鉴定抗体中亲和标记结合位点的方法。

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引用本文的文献

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J Clin Invest. 1996 Oct 15;98(8):1843-50. doi: 10.1172/JCI118985.
2
Abnormalities in the regulation of variable region genes that encode for antibodies to DNA may be a central factor in the pathogenesis of systemic lupus erythematosus.编码针对DNA抗体的可变区基因调控异常可能是系统性红斑狼疮发病机制中的一个核心因素。
Ann Rheum Dis. 1993 May;52(5):378-83. doi: 10.1136/ard.52.5.378.